6,681 Matching Annotations
  1. Apr 2024
    1. Reviewer #2 (Public Review):

      Summary:

      The authors have developed marker selection and k-means (k=2) based binary clustering algorithm for the first-level supervised clustering of the CyTOF dataset. They built a seamless pipeline that offers the multiple functionalities required for CyTOF data analysis.

      Strengths:

      The strength of the study is the potential use of the pipeline for the CyTOF community as a wrapper for multiple functions required for the analysis. The concept of the first line of binary clustering with known markers can be practically powerful.

      Weaknesses:

      The weakness of the study is that there's little conceptual novelty in the algorithms suggested from the study and the benchmarking is done in limited conditions.

    1. Reviewer #2 (Public Review):

      This useful investigation of learning-driven dynamics of cortical and some subcortical structures combines a novel in-scanner learning paradigm with interesting analysis approaches. The new task for reward-based motor learning is compelling and goes beyond the current state of the art. The results are of interest to neuroscientists working on motor control and reward-based learning.

      Comments on revised version:

      The revision has produced a stronger manuscript. Thank you for your thorough responses to the comments and concerns.

    1. Reviewer #2 (Public Review):

      Summary:

      In this manuscript, the authors start by showing that HCN loss-of-function mutation causes a decrease in spiking in bitter GRNs (bGRN) while leaving sweet GRN (sGRN) response in the same sensillum intact. They show that a perturbation of HCN channels in sweet-sensing neurons causes a similar decrease while increasing the response of sugar neurons. They were also able to rescue the response by exogenous expression. Ectopic expression of HCN in bitter neurons had no effect. Next, they measure the sensillum potential and find that sensillum potential is also affected by HCN channel perturbation. These findings lead them to speculate that HCN in sGRN increases sGRN spiking which in turn affects bGRNs. To test this idea that carried out multiple perturbations aimed at decreasing sGRN activity. They found that decreasing sGRN activity by either using receptor mutant or by expressing Kir (a K+ channel) in sGRN increased bGRN responses. These responses also increase the sensillum potential. Finally, they show that these changes are behaviorally relevant as conditions that increase sGRN activity decrease avoidance of bitter substances.

      Strengths:

      There is solid evidence that perturbation of sweet GRNs affects bitter GRN in the same sensillum. The measurement of transsynaptic potential and how it changes is also interesting and supports the authors' conclusion.

      Weaknesses:<br /> The ionic basis of how perturbation in GRN affects the transepithelial potential which in turn affects the second neuron is not clear.

    1. Reviewer #2 (Public Review):

      The authors used a whole genome CRISPR screen to identify targetable synthetic lethalities associated with PPM1D mutations, known poor prognosis and currently undruggable factors in leukemia. The authors identified the cytosolic superoxide dismutase (SOD1, Cu/Zn SOD) as a major protective factor in PPMD1 mutant vs. wt cells, and their study investigates associated mechanisms of this protection. Using both genetic depletion and small molecule inhibitors of SOD1, the authors conclude that SOD1 loss exacerbates mitochondrial dysfunction, ROS levels and DNA damage phenotypes in PPM1D mutant cells, decreasing cell growth in AML cells. The data strongly support that PPMD1 mutant cells have high levels of total peroxides and elevated DNA breaks, and that genetic depletion of SOD1 decreases cell growth in two AML cell lines. However, the authors don't explain how superoxide radical (which is not damaging by itself) induces such damage, the on-target effects of the SOD1 inhibitors at the concentrations is not clear, the increase in total hydroperoxides is not supported by loss of SOD1, the changes in mitochondrial function are small, and there is no assessment of how the mitochondrial SOD2 expression or function, which dismutates mitochondrial superoxide, is altered. Overall these studies do not distinguish between signal vs. damaging aspects of ROS in their models and do not rule out an alternate hypothesis that loss of SOD1 increases superoxide production by cytosolic NADPH activity which would significantly alter ROS-driven regulation of kinase/phosphatase signal modulation, affecting cell growth and proliferation as well as DNA repair. Additionally, with the exception of growth defects demonstrated with sgSOD1, the majority of data are acquired using two chemical inhibitors, LCS1 and ATN-224, without supporting evidence that these inhibitors are acting in an on-target manner.

      Overall, the authors address an important problem by seeking targetable vulnerabilities in PPM1D mutant AML cells, it is clear SOD1 deletion induces strong growth defects in the AML cell lines tested, most of the approaches are appropriate for the outcomes being evaluated, and the data are technically solid and well-presented. The major weakness lies in which redox pathways and ROS species are evaluated, how the resulting data are interpreted, and gaps in the follow-up experiments. Due to these omissions, as currently presented, the broader impact of these findings are unclear.

      These specific concerns are outlined in detail below and I offer some suggestions regarding how to clarify the mechanisms underlying their initial observation of SOD1 synthetic lethality:

      (1) Fig. 1 - SOD1 appears to be clustered with several other genes in the volcano plot (including FANC proteins). Did any other ROS-detoxifying enzymes show similar fitness scores? The effects of the SOD1 sgRNA are striking, however it would be useful to see qPCR or immunoblot data confirming robust depletion.

      Does SOD1 co-expression in PPM1-mutant patient AML correspond to poorer disease outcomes? This can be evaluated in publicly available patient datasets and would support the idea of SOD1 synthetic lethality.

      It would also be useful to know (given the subsequent results) whether expression of the SOD2, the mitochondrial superoxide dismutase, is altered in response to SOD1 loss.

      (2) Fig. 2 - What are the relative SOD1 levels in the mutant PPM1D vs. wt. cell lines? The effects of the chemical inhibitors are stronger in MOLM-13 than the other two lines. These data could also point to whether LCS-1 and ATN-224 cytotoxicity is on-target or off-target at these concentrations, which is a key issue not currently addressed in these studies. This is a particular concern as the OCI-AML2 line shows a stronger growth defect with CRISPR SOD1 KO (in Fig 1) but the smallest effects with these chemical inhibitors.

      While endogenous mitochondrial superoxide levels are elevated in PPM1D mutant lines, it is entirely unclear why SOD1 inhibition should affect mitochondrial superoxide as it detoxifies cytosolic superoxide. Also unclear why DCFDA signal (which measures total hydroperoxides) is *increased* under SOD1 inhibition - SOD1 dismutates superoxide radicals into hydrogen peroxide, therefore unless SOD2 is compensating for SOD1 loss, one might expect hydroperoxides to be lower (unless some entirely different oxidase is increasing their levels). None of these outcomes appear to be considered. Finally, it is not explained how lipid peroxidation, which requires production of hydroxyl or similarly high potency radicals, is being caused by increased superoxide or peroxides. One possibility is there is an increase in labile iron, in which case this phenotype would be rescued by the iron chelator desferal, and by the lipophilic antioxidant, ferrostatin.

      Do the sgSOD1 cells also show similar increases in MitoSox green, DCFDA and BODIPY signal? These experiments would clarify whether the effects with the inhibitors are directly related directly to SOD1 loss or if they represent off-target effects from the inhibitors and/or compensatory changes in SOD2.

      (3) Fig. 3 - the effects on mitochondrial respiratory parameters, while statistically significant, do not seem biologically striking. Also, these data are shown for OCI-AML2 cells which show the smallest cytotoxic effects with the SOD1 inhibitors among the 3 lines tested. They do however show the most robust growth defect with sgSOD1. This discrepancy could suggest that mitochondrial dysfunction does not underlie the observed growth defect and/or the inhibitor cytotoxicity is not on-target. Ideally mitochondrial profiling should also be carried out on this cell line with inducible SOD1 depletion. Have the authors assessed whether the mitochondrial Bcl family proteins are affected by the inhibitors?

      (4) Fig. 4 - Currently the data in this figure do not support the authors claim that PPM1D-mutant cells have impaired antioxidant defense mechanisms, leading to an elevation in ROS levels and reliance on SOD1 for protection. It should be noted that oxidative stress specifically refers to adverse cellular effects of increasing ROS, not baseline levels of various redox parameters. Ideally levels of GSSG/GSH would be a better measure of potential redox stress tolerance than the total antioxidant capacity assay. Finally, oxidative stress can be assessed by challenging the wt and mutant PPM1D cell lines with oxidant stressors such as paraquat which elevates superoxide or drugs like erastin which elevate mitochondrial ROS. The immunoblot shows negligible changes in the antioxidant proteins assayed. Again, this blot should include SOD2 which is the most relevant antioxidant in the context of mitochondrial superoxide.

      (5) Fig. 5 - These data support that DNA breaks are elevated in PPM1D mutant vs. wt cells. However, the data with the chemical SOD1 inhibitor again do not convince that the enhanced levels are due to on-target effects on SOD1. Use of the alkaline comet assay is appropriate for these studies and the 8-oxoguanine data do indicate contributions from oxidative DNA base damage. But these are unlikely to result directly from altered superoxide levels, as this species cannot directly oxidize DNA bases or cause DNA strand breaks.

      The following points summarize my specific experimental and textual recommendations:

      (1) These studies require an assessment of on-target efficacy of the inhibitors at the relevant concentration ranges. Ideally, they should have minimal effects against SOD1 knockout cell lines (acute challenge at a time point before the growth defects become apparent) and show better efficacy in SOD1-overexpressing lines. Key experiments (changes in superoxide, OCR profiling, DNA alkaline comet assay) would be more convincing if they are carried out with SOD1 knockout lines to compare against the inhibitor effects (3-4 days after introducing sgSOD1 when growth defects are not apparent).

      (2) Instead of using NAC, which elevates glutathione synthesis but also has several known side-effects, the authors may want to determine whether Tempol, a SOD mimetic can rescue the effects of SOD1 knockout or inhibition. This would directly prove that SOD1 functional loss underlies the observed growth defect and cytotoxicity from genetic SOD1 knockdown or chemical inhibition.

      (3) The complete lack of consideration of SOD2 in these studies is a missed opportunity as it reduces mitochondrial superoxide levels but elevates hydrogen peroxide levels. It would be very interesting to see whether SOD1 inhibition leads to compensatory increases in SOD2. SOD2 can be easily measured by immunoblot. Furthermore, measuring total superoxide via hydroethidium in a flow cytometric assay vs. mitochondrial ROS in PPM1D mut vs. wt cells and under SOD1 knockout would enable a determination of which species dominates (cytosolic or mitochondrial). These experiments are required to fill some logical gaps in interpretation of their redox data.

      (4) Given the DNA breaks observed in PPM1D mutant cells, it is highly recommended the authors assess whether iron levels are elevated in mut vs. wt cells and whether desferal can rescue observed SOD1 inhibition defects.

      (5) The authors may want to assess whether Rac1 or NADPH oxidase activity is altered in the SOD1 KO in wt vs. PPM1D cells. Their results may be the consequence of compromised ROS-driven survival signaling or DNA repair rather than direct ROS-induced damage, which is not caused directly by superoxide (or hydrogen peroxide).

      (6) It is recommended the discussion focus more strongly on how the signaling function of superoxide vs. its reactions with other molecular entities to induce genotoxic outcomes could be contributing to the observed phenotypes. The discussion of FANC proteins, which were targets with similar fitness scores but not experimentally investigated at all, is an unwarranted digression.

    1. Reviewer #2 (Public Review):

      Boocock and colleagues present an approach whereby eQTL analysis can be carried out by scRNA-Seq alone, in a one-pot-shot experiment, due to genotypes being able to be inferred from SNPs identified in RNA-Seq reads. This approach obviates the need to isolate individual spores, genotype them separately by low-coverage sequencing, and then perform RNA-Seq on each spore separately. This is a substantial advance and opens up the possibility to straightforwardly identify eQTLs over many conditions in a cost-efficient manner. Overall, I found the paper to be well-written and well-motivated, and have no issues with either the methodological/analytical approach (though eQTL analysis is not my expertise), or with the manuscript's conclusions.

      I do have several questions/comments.

      393 segregant experiment:<br /> For the experiment with the 393 previously genotyped segregants, did the authors examine whether averaging the expression by genotype for single cells gave expression profiles similar to the bulk RNA-Seq data generated from those genotypes? Also, is it possible (and maybe not, due to the asynchronous nature of the cell culture) to use the expression data to aid in genotyping for those cells whose genotypes are ambiguous? I presume it might be if one has a sufficient number of cells for each genotype, though, for the subsequent one-pot experiments, this is a moot point.

      Figure 1B:<br /> Is UMAP necessary to observe an ellipse/circle - I wouldn't be surprised if a simple PCA would have sufficed, and given the current discussion about whether UMAP is ever appropriate for interpreting scRNA-Seq (or ancestry) data, it seems the PCA would be a preferable approach. I would expect that the periodic elements are contained in 2 of the first 3 principal components. Also, it would be nice if there were a supplementary figure similar to Figure 4 of Macosko et al (PMID 26000488) to indeed show the cell cycle dependent expression.

      Aging, growth rate, and bet-hedging:<br /> The mention of bet-hedging reminded me of Levy et al (PMID 22589700), where they saw that Tsl1 expression changed as cells aged and that this impacted a cell's ability to survive heat stress. This bet-hedging strategy meant that the older, slower-growing cells were more likely to survive, so I wondered a couple of things. It is possible from single-cell data to identify either an aging, or a growth rate signature? A number of papers from David Botstein's group culminated in a paper that showed that they could use a gene expression signature to predict instantaneous growth rate (PMID 19119411) and I wondered if a) this is possible from single-cell data, and b) whether in the slower growing cells, they see markers of aging, whether these two signatures might impact the ability to detect eQTLs, and if they are detected, whether they could in some way be accounted for to improve detection.

      AIL vs. F2 segregants:<br /> I'm curious if the authors have given thought to the trade-offs of developing advanced intercross lines for scRNA-Seq eQTL analysis. My impression is that AIL provides better mapping resolution, but at the expense of having to generate the lines. It might be useful to see some discussion on that.

      10x vs SPLit-Seq<br /> 10x is a well established, but fairly expensive approach for scRNA-Seq - I wondered how the cost of the 10x approach compares to the previously used approach of genotyping segregants and performing bulk RNA-Seq, and how those costs would change if one used SPLiT-Seq (see PMID 38282330).

    1. Reviewer #2 (Public Review):

      Summary:

      In this manuscript, using Staphylococcus aureus as a model organism, Panda et al. aim to understand how organic acids inhibit bacterial growth. Through careful characterization and interdisciplinary collaboration, the authors present valuable evidence that acetic acid specifically inhibits the activity of Ddl enzyme that converts 2 D-alanine amino acids into D-ala-D-ala dipeptide, which is then used to generate the stem pentapeptide of peptidoglycan (PG) precursors in the cytoplasm. Thus, a high concentration of acetic acid weakens the cell wall by limiting PG-crosslinking (which requires a D-ala portion). However, S. aureus maintains a high intracellular D-ala concentration to circumvent acetate-mediated growth inhibition.

      Strengths:

      The authors utilized a well-established transposon mutant library to screen for mutants that struggle to grow in the presence of acetic acid. This screen allowed authors to identify that a strain lacking intact alr1, which encodes for alanine racemase (converts L-ala to D-ala), is unable to grow well in the presence of acetic acid. This phenotype is rescued by the addition of external D-ala. Next, the authors rule out the contribution of other pathways that could lead to the production of D-ala in the cell. Finally, by analyzing D-ala and D-ala-D-ala concentrations, as well as muropeptide intermediates accumulation in different mutants, the authors pinpoint Ddl as the specific target of acetic acid. In fact, the synthetic overexpression of ddl alone overcomes the toxic effects of acetic acid. Using genetics, biochemistry, and structural biology, the authors show that Ddl activity is specifically inhibited by acetic acid and likely by other biologically relevant organic acids. Interestingly, this mechanism is different from what has been reported for other organisms such as Escherichia coli (where methionine synthesis is affected). It remains to be seen if this mechanism is conserved in other organisms that are more closely related to S. aureus, such as Clostridioides difficile and Enterococcus faecalis.

      Weaknesses:

      Although the authors have conclusively shown that Ddl is the target of acetic acid, it appears that the acetic acid concentration used in the experiments may not truly reflect the concentration range S. aureus would experience in its environment. Moreover, Ddl is only significantly inhibited at a very high acetate concentration (>400 mM). Thus, additional experiments showing growth phenotypes at lower organic acid concentrations may be beneficial. Another aspect not adequately discussed is the presence of D-ala in the gut environment, which may be protective against acetate toxicity based on the model provided.

    1. Reviewer #2 (Public Review):

      Jarysta and colleagues set out to define how similar GNAI/O family members contribute to the shape and orientation of stereocilia bundles on auditory hair cells. Previous work demonstrated that loss of particular GNAI proteins, or inhibition of GNAIs by pertussis toxin, caused several defects in hair bundle morphogenesis, but open questions remained which the authors sought to address. Some of these questions include whether all phenotypes resulting from expression of pertussis toxin stemmed from GNAI inhibition; which GNAI family members are most critical for directing bundle development; whether GNAI proteins are needed for basal body movements that contribute to bundle patterning. These questions are important for understanding how tissue is patterned in response to planar cell polarity cues.

      To address questions related to the GNAI family in auditory hair cell development, the authors assembled an impressive and nearly comprehensive collection of mouse models. This approach allowed for each Gnai and Gnao gene to be knocked out individually or in combination with each other. Notably, a new floxed allele was generated for Gnai3 because loss of this gene in combination with Gnai2 deletion was known to be embryonic lethal. Besides these lines, a new knockin mouse was made to conditionally express untagged pertussis toxin following cre induction from a strong promoter. The breadth and complexity involved in generating and collecting these strains makes this study unique, and likely the authoritative last word on which GNAI proteins are needed for which aspect of auditory hair bundle development.

      Appropriate methods were employed by the authors to characterize auditory hair bundle morphology in each mouse line. Conclusions were carefully drawn from the data and largely based on excellent quantitative analysis. The main conclusions are that GNAI3 has the largest effect on hair bundle development. GNAI2 can compensate for GNAI3 loss in early development but incompletely in late development. The Gnai2 Gnai3 double mutant recapitulates nearly all the phenotypic effects associated with pertussis toxin expression and also reveals a role for GNAIs in early movement of the basal body. This comprehensive study builds on earlier reports, both uncovering new functions and putting previously putative functions on solid ground.

    1. Reviewer #3 (Public Review):

      Summary: Through a rigorous methodology, the authors demonstrated that within 11 different primates, the shape of the brain followed a universal scaling law with fractal properties. They enhanced the universality of this result by showing the concordance of their results with a previous study investigating 70 mammalian brains, and the discordance of their results with other folded objects that are not brains. They incidentally illustrated potential applications of this fractal property of the brain by observing a scale-dependant effect of aging on the human brain.

      Strengths:<br /> - New hierarchical way of expressing cortical shapes at different scales derived from previous report through implementation of a coarse-graining procedure<br /> - Investigation of 11 primate brains and contextualisation with other mammals based on prior literature<br /> - Proposition of tool to analyse cortical morphology requiring no fine tuning and computationally achievable<br /> - Positioning of results in comparison to previous works reinforcing the validity of the observation.<br /> - Illustration of scale-dependance of effects of brain aging in the human.

      Weaknesses:<br /> - The notion of cortical shape, while being central to the article, is not really defined, leaving some interpretation to the reader<br /> - The organization of the manuscript is unconventional, leading to mixed contents in different sections (sections mixing introduction and method, methods and results, results and discussion...). As a result, the reader discovers the content of the article along the way, it is not obvious at what stages the methods are introduced, and the results are sometimes presented and argued in the same section, hindering objectivity.<br /> To improve the document, I would suggest a modification and restructuring of the article such that: 1) by the end of the introduction the reader understands clearly what question is addressed and the value it holds for the community, 2) by the end of the methods the reader understands clearly all the tools that will be used to answer that question (not just the new method), 3) by the end of the results the reader holds the objective results obtained by applying these tools on the available data (without subjective interpretations and justifications), and 4) by the end of the discussion the reader understands the interpretation and contextualisation of the study, and clearly grasps the potential of the method depicted for the better understanding of brain folding mechanisms and properties.

    1. Reviewer #2 (Public Review):

      Summary:

      Carabalona and colleagues investigated the role of the membrane-deforming cytoskeletal regulator protein Abba (MTSS1L/MTSS2) in cortical development to better understand the mechanisms of abnormal neural stem cell mitosis. The authors used short hairpin RNA targeting Abba20 with a fluorescent reporter coupled with in-utero electroporation of E14 mice to show changes to neural progenitors. They performed flow cytometry for in-depth cell cycle analysis of Abba-shRNA impact on neural progenitors and determined an accumulation in the S phase. Using culture rat glioma cells and live imaging from cortical organotypic slides from mice in utero electroporated with Abba-shRNA, the authors found Abba played a prominent role in cytokinesis. They then used a yeast-two-hybrid screen to identify three high-confidence interactors: Beta-Trcp2, Nedd9, and Otx2. They used immunoprecipitation experiments from E18 cortical tissue coupled with C6 cells to show Abba's requirement for Nedd9 localization to the cleavage furrow/cytokinetic bridge. The authors performed a shRNA knockdown of Nedd9 by in-utero electroporation of E14 mice and observed similar results as with the Abba-shRNA. They tested a human variant of Abba using in-utero electroporation of cDNA and found disorganized radial glial fibers and misplaced, multipolar neurons, but lacked the impact of cell division seen in the shRNA-Abba model.

      Strengths:

      A fundamental question in biology about the mechanics of neural stem cell division.

      Directly connecting effects in Abba protein to downstream regulation of RhoA via Nedd9.

      Incorporation of human mutation in ABBA gene.

      Use of novel technologies in neurodevelopment and imaging.

      Weaknesses:

      Unexplored components of the pathway (such as what neurogenic populations are impacted by Abba mutation) and unleveraged aspects of their data (such as the live imaging) limit the scope of their findings and leave significant questions about the effect of ABBA on radial glia development.

      (1) The claim of disorganized radial glial fibers lacks quantifications.<br /> On page 11, the authors claim that knockdown of Abba leads to changes in radial glial morphology observed with vimentin staining. Here they claim misoriented apical processes, detached end feet, and decreased number of RGP cells in the VZ. However, they do not provide quantification of process orientation to better support their first claim. Measurements of radial glia fiber morphology (directionality, length) and angle of division would be metrics that can be applied to data. Some of these analyses could be done in their time-lapse microscopy images, such as to quantify the number of cell divisions during their period of analysis (though that is short-15 hours).

      (2) It is unclear where the effect is:

      -In RG or neuroblasts? Is it in cell cleavage that results in the accumulation of cells at VZ (as sometimes indicated by their data like in Figure 2A or 4D)? Interrogation of cell death (such as by cleaved caspase 3) would also help. Given their time-lapse, can they identify what is happening to the RG fiber? The authors describe a change in "migration" but do not show evidence for this for either progenitor or neuroblast populations. Given they have nice time-lapse imaging data, could they visualize progenitor versus young neuron migration? Analysis of neuroblasts (such as with doublecortin expression in the tissue) would also help understand any issues in migration (of neurons v stem cells).

      -At cleavage furrow? In abscission? There is high-resolution data that highlights the cleavage furrow as the location of interest (Figure 3A), however, there is also data (Figure 3B) to suggest Abba is expressed elsewhere as well and there is an overall soma decrease. More detail of the localization of Abba during the division process would be helpful for example, could cleavage furrow proteins, such as Aurora B, co-localization (and potentially co-IP) help delineate subpopulations of Abba protein? Furthermore, the FRET imaging is a unique way to connect their mutation with function - could they measure/quantify differences at furrow compared to the rest of soma to further corroborate that the Abba-associated RhoA effect was furrow-enriched?

      -The data highlights nicely that a furrow doesn't clearly form when ABBA expression and subsequent RhoA activity are decreased (in Figure 3 or 5A). Does this lead to cells that can't divide because of poor abscission, especially since "rounding" still occurs? Or abnormal progenitors (with loss of fiber or inability to support neuroblast migration)? Or abnormal progression of progenitors to neuroblasts?

      (3) Limited to a singular time point of mouse cortical development

      On page 13, the authors outline the results of their Y2H screen with the identification of three high-confidence interactors. Notably, they used an E10.5-E12.5 mouse brain embryo library rather than one that includes E14, the age of their in-utero electroporation mice. Many of the authors' claims focus on in-utero electroporation of shRNA-Abba of E14 mice that are then evaluated at E16-18. Justification for the focus on this age range should be included to support that their findings can then be applied to all mouse corticogenesis.

      (4) Detail of the effect of the human variant of the ABBA mutation in mice is lacking.

      Their identification of the R671W mutation is interesting and the IUE model warrants more characterization, as they did with their original KD experiments.

      -Could they show that Abba protein levels are decreased (in either cell lines or electroporated tissue)?

      -While time-lapse morphology might not have been performed, more analysis on cell division phenotype (such as plane of division and radial glia morphology) would be helpful.

    1. Reviewer #2 (Public Review):

      The manuscript details an investigation aimed at developing a protocol to render centimeter-scale formalin-fixed paraffin-embedded specimens optically transparent and suitable for deep immunolabeling. The authors evaluate various detergents and conditions for epitope retrieval such as acidic or basic buffers combined with high temperatures in entire mouse brains that had been paraffin-embedded for months. They use various protein targets to test active immunolabeling and light-sheet microscopy registration of such preparations to validate their protocol. The final procedure, called MOCAT pipeline, briefly involves 1% Tween 20 in citrate buffer, heated in a pressure cooker at 121 {degree sign}C for 10 minutes. The authors also note that part of the delipidation is achieved by the regular procedure.

      Major Strengths<br /> - The simplicity and ease of implementation of the proposed procedure using common laboratory reagents distinguish it favorably from more complex methods.

      - Direct comparisons with existing protocols and exploration of alternative conditions enhance the robustness and practicality of the methodology.

      Final considerations<br /> The evidence presented supports the effectiveness of the proposed method in rendering thick FFPE samples transparent and facilitating repeated rounds of immunolabeling.

      The developed procedure holds promise for advancing tissue and 3D-specific determination of proteins of interest in various settings, including hospitals, basic research, and clinical labs, particularly benefiting neuroscience research.

      The methodological findings suggest that MOCAT could have broader applications beyond FFPE samples, differentiating it from other tissue-clearing approaches in that the equipment and chemicals needed are broadly accessible.

    1. Reviewer #2 (Public Review):

      In this manuscript, Yang et al. present a modeling framework to understand the pattern of response biases and variance observed in delayed-response orientation estimation tasks. They combine a series of modeling approaches to show that coupled sensory-memory networks are in a better position than single-area models to support experimentally observed delay-dependent response bias and variance in cardinal compared to oblique orientations. These errors can emerge from a population-code approach that implements efficient coding and Bayesian inference principles and is coupled to a memory module that introduces random maintenance errors. A biological implementation of such operation is found when coupling two neural network modules, a sensory module with connectivity inhomogeneities that reflect environment priors, and a memory module with strong homogeneous connectivity that sustains continuous ring attractor function. Comparison with single-network solutions that combine both connectivity inhomogeneities and memory attractors shows that two-area models can more easily reproduce the patterns of errors observed experimentally. This, the authors take as evidence that a sensory-memory network is necessary, but I am not convinced about the evidence in support of this "necessity" condition. A more in-depth understanding of the mechanisms operating in these models would be necessary to make this point clear.

      Strengths:

      The model provides an integration of two modeling approaches to the computational bases of behavioral biases: one based on Bayesian and efficient coding principles, and one based on attractor dynamics. These two perspectives are not usually integrated consistently in existing studies, which this manuscript beautifully achieves. This is a conceptual advancement, especially because it brings together the perceptual and memory components of common laboratory tasks.

      The proposed two-area model provides a biologically plausible implementation of efficient coding and Bayesian inference principles, which interact seamlessly with a memory buffer to produce a complex pattern of delay-dependent response errors. No previous model had achieved this.

      Weaknesses:

      The correspondence between the various computational models is not fully disclosed. It is not easy to see this correspondence because the network function is illustrated with different representations for different models and the correspondence between components of the various models is not specified. For instance, Figure 1 shows that a specific pattern of noise is required in the low-dimensional attractor model, but in the next model in Figure 2, the memory noise is uniform for all stimuli. How do these two models integrate? What element in the population-code model of Figure 2 plays the role of the inhomogeneous noise of Figure 1? Also, the Bayesian model of Figure 2 is illustrated with population responses for different stimuli and delays, while the attractor models of Figures 3 and 4 are illustrated with neuronal tuning curves but not population activity. In addition, error variance in the Bayesian model appears to be already higher for oblique orientations in the first iteration whereas it is only first shown one second into the delay for the attractor model in Figure 4. It is thus unclear whether variance inhomogeneities appear already at the perceptual stage in the attractor model, as it does in the population-code model. Of course, correspondences do not need to be perfect, but the reader does not know right now how far the correspondence between these models goes.

      The manuscript does not identify the mechanistic origin in the model of Figure 4 of the specific noise pattern that is required for appropriate network function (with higher noise variance at oblique orientations). This mechanism appears critical, so it would be important to know what it is and how it can be regulated. In particular, it would be interesting to know if the specific choice of Poisson noise in Equation (3) is important. Tuning curves in Figure 4 indicate that population activity for oblique stimuli will have higher rates than for cardinal stimuli and thus induce a larger variance of injected noise in oblique orientations, based on this Poisson-noise assumption. If this explanation holds, one wonders if network inhomogeneities could be included (for instance in neural excitability) to induce higher firing rates in the cardinal/oblique orientations so as to change noise inhomogeneities independently of the bias and thus control more closely the specific pattern of errors observed, possibly within a single memory network.

      The main conclusion of the manuscript, that the observed patterns of errors "require network interaction between two distinct modules" is not convincingly shown. The analyses show that there is a quantitative but not a qualitative difference between the dynamics of the single memory area compared to the sensory-memory two-area network, for specific implementations of these models (Figure 7 - Figure Supplement 1). There is no principled reasoning that demonstrates that the required patterns of response errors cannot be obtained from a different memory model on its own. Also, since the necessity of the two-area configuration is highlighted as the main conclusion of the manuscript, it is inconvenient that the figure that carefully compares these conditions is in the Supplementary Material.

      The proposed model has stronger feedback than feedforward connections between the sensory and memory modules. This is not a common assumption when thinking about hierarchical processing in the brain, and it is not discussed in the manuscript.

    1. Reviewer #2 (Public Review):

      The authors have studied subpopulations of individual neurons recorded in the thalamus and subthalamic nucleus (STN) of awake humans performing a simple cognitive task. They have carefully designed their task structure to eliminate motor components that could confound their analyses in these subcortical structures, given that the data was recorded in patients with Parkinson's Disease (PD) and diagnosed with an Essential Tremor (ET). The recorded data represents a promising addition to the field. The analyses that the authors have applied can serve as a strong starting point for exploring the kinds of complex signals that can emerge within a single neuron's activity. Pereira et. al conclude that their results from single neurons indicate that task-related activity occurs, purportedly separate from previously identified sensory signals. These conclusions are a promising and novel perspective for how the field thinks about the emergence of decisions and sensory perception across the entire brain as a unit.

      Despite the strength of the data that was obtained and the relevant nature of the conclusions that were drawn, there are certain limitations that must be taken into consideration:

      (1) The authors make several claims that their findings are direct representations of consciousness identifiable in subcortical structures. The current context for consciousness does not sufficiently define how the consciousness is related to the perceptual task.

      (2) The current work would benefit greatly from a description and clarification of what all the neurons that have been recorded are doing. The authors' criteria for selecting subpopulations with task-relevant activity are appropriate, but understanding the heterogeneity in a population of single neurons is important for broader considerations that are being studied within the field.

      (3) The authors have omitted a proper set of controls for comparison against the active trials, for example, where a response was not necessary. Please explain why this choice was made and what implications are necessary to consider.

    1. Reviewer #2 (Public Review):

      Summary:

      Here the authors describe a model for tracking time-varying coupling between neurons from multi-electrode spike recordings. Their approach extends a GLM with static coupling between neurons to include dynamic weights, learned by a long-short-term-memory (LSTM) model. Each connection has a corresponding LSTM embedding and is read out by a multi-layer perceptron to predict the time-varying weight.

      Strengths:

      This is an interesting approach to an open problem in neural data analysis. I think, in general, the method would be interesting to computational neuroscientists.

      Weaknesses:

      It is somewhat difficult to interpret what the model is doing. I think it would be worthwhile to add some additional results that make it more clear what types of patterns are being described and how.

      Major Issues:

      Simulation for dynamic connectivity. It certainly seems doable to simulate a recurrent spiking network whose weights change over time, and I think this would be a worthwhile validation for this DyNetCP model. In particular, I think it would be valuable to understand how much the model overfits, and how accurately it can track known changes in coupling strength. If the only goal is "smoothing" time-varying CCGs, there are much easier statistical methods to do this (c.f. McKenzie et al. Neuron, 2021. Ren, Wei, Ghanbari, Stevenson. J Neurosci, 2022), and simulations could be useful to illustrate what the model adds beyond smoothing.

      Stimulus vs noise correlations. For studying correlations between neurons in sensory systems that are strongly driven by stimuli, it's common to use shuffling over trials to distinguish between stimulus correlations and "noise" correlations or putative synaptic connections. This would be a valuable comparison for Figure 5 to show if these are dynamic stimulus correlations or noise correlations. I would also suggest just plotting the CCGs calculated with a moving window to better illustrate how (and if) the dynamic weights differ from the data.

    1. Reviewer #2 (Public Review):

      In this paper, Boi et al. thoroughly classified the electrophysiological and morphological characteristics of serotonergic and dopaminergic neurons in the DRN and examined the alterations of these neurons in the 6-OHDA-induced mouse PD model. Using whole-cell patch clamp recording, they found that 5-HT and dopamine (DA) neurons in the DRN are electrophysiologically well-distinguished from each other. In addition, they characterized distinct morphological features of 5-HT and DA neurons in the DRN. Notably, these specific features of 5-HT and DA neurons in the DRN exhibited different changes in the 6-OHDA-induced PD model. Then the authors utilized desipramine (DMI) to separate the effects of nigrostriatal DA depletion and noradrenalin (NA) depletion which are induced by 6-OHDA. Interestingly, protection from NA depletion by DMI pretreatment reversed the changes in 5-HT neurons, while having a minor impact on the changes in DA neurons in the DRN. These data indicate that the role of NA lesion in the altered properties of DRN 5-HT neurons by 6-OHDA is more critical than the one of DA lesion.

      Overall, this study provides foundational data on the 5-HT and DA neurons in the DRN and their potential involvement in PD symptoms. Given the defects of the DRN in PD, this paper may offer insights into the cellular mechanisms that may underlie non-motor symptoms associated with PD. Despite the importance of the primary claim proposed by the authors, however, the interpretation of the authors on some DMI experiments is not explained well.

    1. Reviewer #2 (Public Review):

      The authors examine the impact of optogenetic inhibition of hippocampal axon terminals in the retrosplenial cortex (RSP) during the performance of a working memory T-maze task. Performance on a delayed non-match-to-place task was impaired by such inhibition. The authors also report that inhibition is associated with faster decision-making and that the effects of inhibition can be observed over several subsequent trials. The work seems reasonably well done and the role of hippocampal projections to retrosplenial cortex in memory and decision-making is very relevant to multiple fields. However, the work should be expanded in several ways before one can make firm conclusions on the role of this projection in memory and behavior.

      (1) The work is very singular in its message and the experimentation. Further, the impact of the inhibition on behavior is very moderate. In this sense, the results do not support the conclusion that the hippocampal projection to retrosplenial cortex is key to working memory in a navigational setting.

      (2) There are no experiments examining other types of behavior or working memory. Given that the animals used in the studies could be put through a large number of different tasks, this is surprising. There is no control navigational task. There is no working memory test that is non-spatial. Such results should be presented in order to put the main finding in context.

      (3) The actual impact of the inhibition on activity in RSP is not provided. While this may not be strictly necessary, it is relevant that the hippocampal projection to RSP includes, and is perhaps dominated by inhibitory inputs. I wonder why the authors chose to manipulate hippocampal inputs to RSP when the subiculum stands as a much stronger source of afferents to RSP and has been shown to exhibit spatial and directional tuning of activity. The points here are that we cannot be sure what the manipulation is really accomplishing in terms of inhibiting RSP activity (perhaps this explains the moderate impact on behavior) and that the effect of inhibiting hippocampal inputs is not an effective means by which to study how RSP is responsive to inputs that reflect environmental locations.

      (4) The impact of inhibition on trials subsequent to the trial during which optical stimulation was actually supplied seems trivial. The authors themselves point to evidence that activation of the hyperpolarizing proton pump is rather long-lasting in its action. Further, each sample-test trial pairing is independent of the prior or subsequent trials. This finding is presented as a major finding of the work, but would normally be relegated to supplemental data as an expected outcome given the dynamics of the pump when activated.

      (5) In the middle of the first paragraph of the discussion, the authors make reference to work showing RSP responses to "contextual information in egocentric and allocentric reference frames". The citations here are clearly deficient. How is the Nitzan 2020 paper at all relevant here?

      (6) The manuscript is deficient in referencing and discussing data from the Smith laboratory that is similar. The discussion reads mainly like a repeat of the results section.

    1. Reviewer #3 (Public Review):

      The manuscript by Yang et al. investigated in mice how hypobaric hypoxia can modify the RBC clearance function of the spleen, a concept that is of interest. Via interpretation of their data, the authors proposed a model that hypoxia causes an increase in cellular iron levels, possibly in RPMs, leading to ferroptosis, and downregulates their erythrophagocytic capacity.

      Comments on revised version:

      The manuscript has now improved with all the new data, supporting the model proposed by the authors. However, it remains not very easy to follow for the conclusions and experimental details. Some of the most important remaining comments are listed below:

      (1) Lines 401-406 - The conclusions in this new fragment sound a bit overstated - the authors do not directly measure erytrophagocytosis capacity, only the total RBC parameters in the circulation. The increase is also very mild biologically between sham and splenectomized mice in HH conditions.

      (2) scRNA seq data are still presented in a way that is very difficult to understand. The readers could not see from the graphics that macrophages are depleted. The clusters are not labelled - some clusters in the bin 'macrophahes+DC' seem actually to be more represented in Fig. 3E; Fig. 3F does not correspond to Fig. 3D. It would be maybe more informative to present like in Figure D side by side NN versus HH? The authors could consider moving the data from supplements that relate to RPMs to the main figure and making it consistent for the Clusters - eg, the authors show data for Cluster 0 in the supplement, and the same Cluster is not marked as macrophages in the main figure. This is quite difficult to follow.

      (3) Figure 3G has likely mislabeled axis for F4/80 and CD11b - such mistakes should be avoided in a second revised version of the manuscript, and this data is now redundant with the data shown as new Figure 5A.

      (4) The data from new Figure 4 should be better mentioned in the main body of the manuscript - all panels are mentioned twice in the text, first speaking about the decline of labelled RBCs and second referring to phagocytic capacity, whereas this figure only illustrates the decline of labelled RBCs, not directly phagocytic capacity of RPMs. What is lacking, as opposed to typical RBC life span assay, is the time '0' ('starting point') - this is particularly important as we can observe a big drop in labelled RBCs for eg 7 days between NN and HH group, actually implying increased removal of labelled RBCs within the first days of hypoxia exposure. What should be better labelled in this figure is that the proportion of RBCs are labelled RBCs not all RBCs (Y axis in individual panels). Overall, the new Figure 4 brings new data to the study, but how it is presented and discussed is not at the 'state-of-the-art' level (eg, missing the time '0') and is not very straightforward to the reader.

      (5) In Figure 7, the experiments with Tuftsin are not very easy to follow, especially for the major conclusions. In panels A and B, the focus is the drug itself under NN conditions, with RBC removal as a readout. Then, in the next panels, the authors introduce HH, and then look at the F4/80 and iron staining. What was exactly the major point the authors wanted to make here?

      (6) The data from Figure 8 are informative but do not address the individual cell types - eg, a drop in HO1 or FT may be due to the depletion of RPMs. An increase of TFR1 could be due to the retention of RBCs, the same as maybe labile iron. The data from PBMC are only very loosely linked to these phenotypes observed in the total spleen, and the reason for the regulation of the same proteins in PBMC might be different. It goes back to the data in Figure 3A-C, where also total splenocytes are investigated for their viability.

      (7) Can the authors provide the data for the purity (eg cell surface markers) of their primary splenic macrophage cultures? Only ensuring that these are macrophages or addressing the readouts from Figure 8 in RPMs could link ferroptosis to RPMs under HH conditions.

      (8) All the data are not presented as individual data points which is not widely applied in papers.

      (9) No gating strategies are nicely illustrated or described.

    1. Reviewer #3 (Public Review):

      Previously, it has been shown the essential role of IDA peptide and HAESA receptor families in driving various cell separation processes such as abscission of flowers as a natural developmental process, of leaves as a defense mechanism when plants are under pathogenic attack or at the lateral root emergence and root tip cell sloughing. In this work, Olsson et al. show for the first time the possible role of IDA peptide in triggering plant innate immunity after the cell separation process occurred. Such an event has been previously proposed to take place in order to seal open remaining tissue after cell separation to avoid creating an entry point for opportunistic pathogens. The elegant experiments in this work demonstrate that IDA peptide is triggering the defense-associated marker genes together with immune specific responses including release of ROS and intracellular CA2+. Thus, the work highlights an intriguing direct link between endogenous cell wall remodeling and plant immunity. Moreover, the upregulation of IDA in response to abiotic and especially biotic stimuli are providing a valuable indication for potential involvement of HAE/IDA signalling in other processes than plant development.

      Comments on revised version:

      We thank the authors for addressing our previous comments. Overall, we are satisfied with the improvements and appreciate the hard work that has gone into this manuscript. We wish you all the best on the further publication pathway.

    1. Reviewer #2 (Public Review):

      This manuscript explores the interplay between Legionella Dot/Icm effectors that modulate ubiquitination of the host GTPase Rab10. Rab10 undergoes phosphoribosyl-ubiquitination (PR-Ub) by the SidE family of effectors which is required for its recruitment to the Legionella containing vacuole (LCV). Through a series of elegant experiments using effector gene knockouts, co-transfection studies and careful biochemistry, Kubori et al further demonstrate that:

      (1) The SidC family member SdcB contributes to the polyubiquitination (poly-Ub) of Rab10 and its retention at the LCV membrane.

      (2) The transglutaminase effector, MavC acts as an inhibitor of SdcB by crosslinking ubiquitin at Gln41 to lysine residues in SdcB.

    1. Reviewer #2 (Public Review):

      Summary:

      This study focuses on the 5-HT3 serotonin receptor, a pentameric ligand-gated ion channel important in chemical neurotransmission. There are many cryo-EM structures of this receptor with diverse ligands bound, however assignment of functional states to the structures remains incomplete. The team applies voltage-clamp fluorometry to measure, at once, both changes in ion channel activity, and changes in fluorescence. Four cysteine mutants were selected for fluorophore labeling, two near the neurotransmitter site, one in the ECD vestibule, and one at the ECD-TMD junction. Agonists, partial agonists, and antagonists were all found to yield similar changes in fluorescence, a proxy for conformational change, near the neurotransmitter site. The strength of the agonist correlated to a degree with propagation of this fluorescence change beyond the local site of neurotransmitter binding. Antagonists failed to elicit a change in fluorescence in the vestibular of the ECD-TMD junction sites. The VCF results further turned up evidence supporting intermediate (likely pre-active) states.

      Strengths:

      The experiments appear rigorous, the problem the team tackles is timely and important, the writing and the figures are for the most part very clear. We sorely need approaches orthogonal to structural biology to annotate conformational states and observe conformational transitions in real membranes- this approach, and this study, get right to the heart of what is missing.

      Weaknesses:

      The weaknesses in the study itself are overall minor, I only suggest improvements geared toward clarity. What we are still missing is application of an approach like this to annotate the conformation of the part of the receptor buried in the membrane; there is an important debate about which structure represents which state, and that is not addressed in the current study.

    1. Reviewer #2 (Public Review):

      Summary:

      In this manuscript, the authors describe a mechanism, by which fluorescently-labelled Collagen type I is taken up by cells via endocytosis and then incorporated into newly synthesized fibers via an ITGA11 and VPS33B-dependent mechanism. The authors claim the existence of this collagen recycling mechanism and link it to fibrotic diseases such as IPF and chronic wounds.

      Strengths:

      The manuscript is well-written, and experimentally contains a broad variation of assays to support their conclusions. Also, the authors added data of IPF patient-derived fibroblasts, patient-derived lung samples, and patient-derived samples of chronic wounds that highlight a potential in vivo disease correlation of their findings.

      The authors were also analyzing the membrane topology of VPS33B and could unravel a likely 'hairpin' like conformation in the ER membrane.

      Weaknesses:

      Experimental evidence is missing that supports the non-degradative endocytosis of the labeled collagen.

      The authors show and mention in the text that the endocytosis inhibitor Dyngo®4a shows an effect on collagen secretion. It is not clear to me how specific this readout is if the inhibitor affects more than endocytosis. This issue was unfortunately not further discussed. The authors use commercial rat tail collagen, it is unclear to me which state the collagen is in when it's endocytosed. Is it fully assembled as collagen fiber or are those single heterotrimers or homotrimers?

      The Cy-labeled collagen is clearly incorporated into new fibers, but I'm not sure whether the collagen is needed to be endocytosed to be incorporated into the fibers or if that is happening in the extracellular space mediated by the cells.

      In general for the collagen blots, due to the lack of molecular weight markers, what chain/form of collagen type I are you showing here?

      Besides the VPS33B siRNA transfected cells the authors also use CRISPR/Cas9-generated KO. The KO cells do not seem to be a clean system, as there is still a lot of mRNA produced. Were the clones sequenced to verify the KO on a genomic level? For the siRNA transfection, a control blot for efficiency would be great to estimate the effect size. To me it is not clear where the endocytosed collagen and VPS33B eventually meet in the cells and whether they interact. Or is ITGA11 required to mediate this process, in case VPS33B is not reaching the lumen?

      The authors show an upregulation of ITGA11 and VPS33B in IPF patients-derived fibroblasts, which can be correlated to an increased level of ColI uptake, however, it is not clear whether this increased uptake in those cells is due to the elevated levels of VPS33B and/or ITGA11.

    1. Reviewer #2 (Public Review):

      Summary:

      This manuscript uses FRET, 19F-NMR, and DEER/EPR solution measurements to examine the allosteric effects of a panel of BRAF inhibitors (BRAFi). These include first-generation aC-out BRAFi, and more recent Type I and Type II aC-in inhibitors. Intermolecular FRET measurements quantify Kd for BRAF dimerization and inhibitor binding to the first and second subunits. Distinct patterns are found between aC-in BRAFi, where Type I BRAFi binds equally well to the first and second subunits within dimeric BRAF. In contrast, Type II BRAFi shows stronger affinity for the first subunit and weaker affinity for the second subunit, an effect named "allosteric asymmetry". Allosteric asymmetry has the potential for Type II inhibitors to promote dimerization while favoring occupancy of only one subunit (BBD form), leading to the enrichment of an active dimer.

      Measurements of in vitro BRAF kinase activity correlate amazingly well with the calculated amounts of the half-site-inhibited BBD forms with Type II inhibitors. This suggests that the allosteric asymmetry mechanism explains paradoxical activation by this class of inhibitors. DEER/EPR measurements further examine the positioning of helix aC. They show systematic outward movement of aC with Type II inhibitors, relative to the aC-in state with Type I inhibitors, and further show that helix aC adopts multiple states and is therefore dynamic in apo BRAF. This makes a strong case that negative cooperativity between sites in the BRAF dimer can account for paradoxical kinase activation by Type II inhibitors by creating a half-site-occupied homodimer, BBD. In contrast, Type I inhibitors and aC-out inhibitors do not fit this model, and are therefore proposed to be explained by previously proposed models involving negative allostery between subunits in BRAF-CRAF heterodimers, RAS priming, and transactivation.

      Strengths:

      This study integrates orthogonal spectroscopic and kinetic strategies to characterize BRAF dynamics and determine how it impacts inhibitor allostery. The unique combination of approaches presented in this study represents a road map for future work in the important area of protein kinase dynamics. The work represents a worthy contribution not only to the field of BRAF regulation but to protein kinases in general.

      Weaknesses:

      Some questions remain regarding the proposed model for Type II inhibitors and its comparison to Type I and aC-out inhibitors that would be useful to clarify. Specifically, it would be helpful to address whether the activation of BRAF by Type II inhibitors, while strongly correlated with BBD model predictions in vitro, also depends on CRAF via BRAF-CRAF in cells and therefore overlaps with the mechanisms of paradoxical activation by Type I and aC-out inhibitors.

    1. Reviewer #2 (Public Review):

      Summary:

      A dominant hypothesis concerning the origin of life is that, before the appearance of the first enzymes, RNA replicated non-enzymatically by templating. However, this replication was probably not very efficient, due to the propensity of single strands to bind to each other, thus inhibiting template replication. This phenomenon, known as product inhibition, has been shown to lead to parabolic growth instead of exponential growth. Previous works have shown that this situation limits competition between alternative replicators and therefore promotes RNA population diversity. The present work examines this scenario in an agent-based model of RNA replication, taking into account finite population size, mutations and differences in GC content. The main results are (1) confirmation that parabolic growth promotes diversity, but that when the population size is small enough, sequences least efficient at replicating may nevertheless go extinct; (2) the observation that fitness is not only controlled by the replicability of sequences, but also by their GC content ; (3) the observation that parabolic growth attenuates the impact of mutations and, in particular, that the error threshold to which exponentially growing sequences are subject can be exceeded, enabling sequence identity to be maintained at higher mutation rates.

      Strengths:

      The analyses are sound and the observations intriguing. Indeed, while it has been noted previously that parabolic growth promotes coexistence, this is the first work to show that it can also mitigate the error threshold catastrophe, which is often presented as a major obstacle to our understanding of the origin of life.

      Weaknesses:

      A general weakness, which can however be seen as inherent in an agent-based model that aims to be more realistic than earlier, more phenomenological models, is the proliferation of parameters. The choice and values of these parameters are generally justified and, in many cases, several values are tested to assess the robustness of the results, but it can be difficult for the reader to identify the modeling choices that are truly critical from those that are less so.

    1. Reviewer #2 (Public Review):

      Maurer et al investigated the contribution of GAD2+ neurons in the preoptic area (POA), projecting to the tuberomammillary nucleus (TMN), to REM sleep regulation. They applied an elegant design to monitor and manipulate activity of this specific group of neurons: a GAD2-Cre mouse, injected with retrograde AAV constructs in the TMN, thereby presumably only targeting GAD2+ cells projecting to the TMN. Using this set-up in combination with technically challenging techniques including EEG with photometry and REM sleep deprivation, the authors found that this cell-type studied becomes active shortly (≈40sec) prior to entering REM sleep and remains active during REM sleep. Moreover, optogenetic inhibition of GAD2+ cells inhibits REM sleep by a third, and also impairs the rebound in REM sleep in the following hour. Thus, the data makes a convincing case for a role of GAD2+ neurons in the POA projecting to the TMN in REM sleep regulation.

    1. Reviewer #3 (Public Review):

      Summary:

      The work by Masala and colleagues highlights a striking artifact that can result from a particular viral method for expressing genetically encoded calcium indicators (GECIs) in neurons. In a cross-institutional collaboration, the authors find that viral transduction of GECIs in the hippocampus can result in aberrant slow-traveling calcium (Ca2+) micro-waves. These Ca2+ micro-waves are distinct from previously described ictal activity but nevertheless are likely a pathological consequence of overexpression of virally transduced proteins. Ca2+ micro-waves will most-likely obscure the physiology that most researchers are interested in studying with GECIs, and their presence indicates that the neural circuit is in an unintended pathological state. Interestingly this pathology was not observed using the same viral transduction methods in other brain regions. The authors recommend several approaches that may help other experimenters avoid this confound in their own data such as reducing the titer of viral injections or using recombinase-dependent expression. The intent of this manuscript is to raise awareness of the potential unintended consequences of viral overexpression, particularly for GECIs. A rigorous investigation into the exact causes of Ca2+ micro-waves or the mechanisms supporting them are beyond the authors' intended scope.

      Strengths:

      The authors clearly demonstrate that Ca2+ micro-waves occur in the CA1 and CA3 regions of the hippocampus following large volume, high titer injections of adeno-associated viruses (AAV1 and AAV9) encoding GECIs. The supplementary videos provide undeniable proof of their existence.

      By forming an inter-institutional collaboration, the authors demonstrate that this phenomenon is robust to changes in surgical techniques or imaging conditions.

      Weaknesses:

      I believe that the weaknesses of the manuscript are appropriately highlighted by the authors themselves in the discussion. The manuscript does not attempt to exhaustively characterize the conditions under which calcium micro-waves occur. Rather, the authors raise awareness of this problem.

    1. Reviewer #2 (Public Review):

      Summary:

      Roy et al. investigated the role of non-canonical DNA structures called G-quadruplexes (G4s) in long-range chromatin interactions and gene regulation. Introducing a G4 array into chromatin significantly increased the number of long-range interactions, both within the same chromosome (cis) and between different chromosomes (trans). G4s functioned as enhancer elements, recruiting p300 and boosting gene expression even 5 megabases away. The study proposes a mechanism where G4s directly influence 3D chromatin organization, facilitating communication between regulatory elements and genes.

      Strength:

      The findings are valuable for understanding the role of G4-DNA in 3D genome organization and gene transcription.

      Weaknesses:

      The study would benefit from more robust and comprehensive data, which would add depth and clarity.

      (1) Lack of G4 Structure Confirmation: The absence of direct evidence for G4 formation within cells undermines the study's foundation. Relying solely on in vitro data and successful gene insertion is insufficient.

      (2) Alternative Explanations: The study does not sufficiently address alternative explanations for the observed results. The inserted sequences may not form G4s or other factors like G4-RNA hybrids may be involved.

      (3) Limited Data Depth and Clarity: ChIP-qPCR offers limited scope and considerable variation in some data makes conclusions difficult.

      (4) Statistical Significance and Interpretation: The study could be more careful in evaluating the statistical significance and magnitude of the effects to avoid overinterpreting the results.

    1. Reviewer #3 (Public Review):

      Summary:

      The manuscript uses a combination of evolutionary approaches and structural/dynamics observations to provide mechanistic insights in the adaptation of the Spike protein during the evolution of SARS-COV-2 variants. The conclusion that CAP sites should be taken in particular account when considering the impact of the emergence of new strains and mutations is warranted.

      Strengths:

      The results presented in this work are very well outlined with well-written text, pleasant and well-described pictures, didactical and clear description of the methods, e.g. the discussion of how the MD equilibration procedure is applied and evaluated is clear and well argument.<br /> The citation of relevant similar results with different approaches strengthens the reasoning; in particular, comparing the calculated scores with previous experimentally obtained data is one of the strongest points of the manuscript.

      Weaknesses:

      There are no replicas of the molecular dynamics (MD) simulations, understandable since it's not a MD-focused paper. However, the comparison of multiple replicas could enhance the reliability of the findings.

    1. Reviewer #2 (Public Review):

      Summary:

      This paper by Olah et al. uncovers a previously unknown role of HCN channels in shaping synaptic inputs to L2/3 cortical neurons. The authors demonstrate using slice electrophysiology and computational modeling that, unlike layer 5 pyramidal neurons, L2/3 neurons have an enrichment of HCN channels in the proximal dendrites. This location provides a locus of neuromodulation for inputs onto the proximal dendrites from L4 without an influence on distal inputs from L1. The authors use pharmacology to demonstrate the effect of HCN channels on NMDA-mediated synaptic inputs from L4. The authors further demonstrate the developmental time course of HCN function in L2/3 pyramidal neurons. Taken together, this a well-constructed investigation of HCN channel function and the consequences of these channels on synaptic integration in L2/3 pyramidal neurons.

      Strengths:

      The authors use careful, well-constrained experiments using multiple pharmacological agents to asses HCN channel contributions to synaptic integrations. The authors also use a voltage clamp to directly measure the current through HCN channels across developmental ages. The authors also provide supplemental data showing that their observation is consistent across multiple areas of the cerebral cortex.

      Weaknesses:

      The gradient of the HCN channel function is based almost exclusively on changes in EPSP width measured at the soma. While providing strong evidence for the presence of HCN current in L2/3 neurons, there are space clamp issues related to the use of somatic whole-cell voltage clamps that should be considered in the discussion.

    1. Reviewer #2 (Public Review):

      The present study aims to investigate brain white matter predictors of back pain chronicity. To this end, a discovery cohort of 28 patients with subacute back pain (SBP) was studied using white matter diffusion imaging. The cohort was investigated at baseline and one-year follow-up when 16 patients had recovered (SBPr) and 12 had persistent back pain (SBPp). A comparison of baseline scans revealed that SBPr patients had higher fractional anisotropy values in the right superior longitudinal fasciculus SLF) than SBPp patients and that FA values predicted changes in pain severity. Moreover, the FA values of SBPr patients were larger than those of healthy participants, suggesting a role of FA of the SLF in resilience to chronic pain. These findings were replicated in two other independent datasets. The authors conclude that the right SLF might be a robust predictive biomarker of CBP development with the potential for clinical translation.

      Developing predictive biomarkers for pain chronicity is an interesting, timely, and potentially clinically relevant topic. The paradigm and the analysis are sound, the results are convincing, and the interpretation is adequate. A particular strength of the study is the discovery-replication approach with replications of the findings in two independent datasets.

      The following revisions might help to improve the manuscript further.

      - Definition of recovery. In the New Haven and Chicago datasets, SBPr and SBPp patients are distinguished by reductions of >30% in pain intensity. In contrast, in the Mannheim dataset, both groups are distinguished by reductions of >20%. This should be harmonized. Moreover, as there is no established definition of recovery (reference 79 does not provide a clear criterion), it would be interesting to know whether the results hold for different definitions of recovery. Control analyses for different thresholds could strengthen the robustness of the findings.

      - Analysis of the Chicago dataset. The manuscript includes results on FA values and their association with pain severity for the New Haven and Mannheim datasets but not for the Chicago dataset. It would be straightforward to show figures like Figures 1 - 4 for the Chicago dataset, as well.

      - Data sharing. The discovery-replication approach of the present study distinguishes the present from previous approaches. This approach enhances the belief in the robustness of the findings. This belief would be further enhanced by making the data openly available. It would be extremely valuable for the community if other researchers could reproduce and replicate the findings without restrictions. It is not clear why the fact that the studies are ongoing prevents the unrestricted sharing of the data used in the present study.

    1. Reviewer #2 (Public Review):

      Summary:

      Galanti et al investigate genetic variation in plant pest resistance using non-target reads from whole-genome sequencing of 207 field lines spontaneously colonized by aphids and mildew. They calculate significant differences in pest DNA load between populations and lines, with heritability and correlation with climate and glucosinolate content. By genome-wide association analyses they identify known defence genes and novel regions potentially associated with pest load variation. Additionally, they suggest that differential methylation at transposons and some genes are involved in responses to pathogen pressure. The authors present in this study the potential of leveraging non-target sequencing reads to estimate plant biotic interactions, in general for GWAS, and provide insights into the defence mechanisms of Thlaspi arvense.

      Strengths:

      The authors ask an interesting and important question. Overall, I found the manuscript very well-written, with a very concrete and clear question, a well-structured experimental design, and clear differences from previous work. Their important results could potentially have implications and utility for many systems in phenotype-genotype prediction. In particular, I think the use of unmapped reads for GWAS is intriguing.

      Weaknesses:

      I found that several of the conclusions are incomplete, not well supposed by the data and/or some methods/results require additional details to be able to be judged. I believe these analyses and/or additional clarifications should be considered.

  2. www.researchsquare.com www.researchsquare.com
    1. Reviewer #2 (Public Review):

      Summary:

      The manuscript by Gao et al. described a study identifying the role of FAK in fine-tuning the activation levels of ERK signaling in BRAF-V600E-driven colorectal cancer. The authors generated new mouse models combining Vill-Cre mediated BRAF-V600E expression with FAK deletion. Analyses of intestinal tumor phenotypes revealed that FAK-loss promotes BRAF-V600E-induced tumor formation, specifically in the cecum. Interestingly, these tumors closely resemble human sessile serrated adenoma/polyps. Using bioinformatics analysis, the authors found that FAK deletion upregulates the intestinal stem cell and fetal-type transcriptomic signatures compared to mice expressing BRAF-V600E alone. In addition, FAK-loss decreases the phosphorylation of ERK whereas it increases the expression of Lgr4 at both mRNA and protein levels. To mechanistically connect FAK-mediated downregulation of ERK and upregulation of Lgr4 in the context of BRAF-V600E mutation, results from biochemical experiments showed that MEK inhibitor treatment decreases the expression of NEDD4, a previously identified ubiquitin E3 ligase of Lgr4, which coincides with increased Lgr4 protein expression both in cells and in vivo. Moreover, the FAK-dependent modulation of ERK signaling is specific to BRAF-V600E-driven tumorigenesis only as knockout of FAK has no effect in Vill-Cre/KRAS-G12D mice. Collectively, the authors proposed a "just right" model in that a tunable FAK expression controls the optimal level of ERK pathway output needed for BRAF-V600E-induced cecal tumor formation.

      Strengths:

      This study provides new insights into the mechanisms underlying the serrated pathway-driven tumorigenesis in colorectal cancer. The newly established mouse model with compound mutations of BRAF and FAK offers a useful resource for future studies of the serrated pathway. The conclusions of this paper are mostly supported by data.

      Weaknesses:

      However, some aspects of the paper can be strengthened with additional mechanistically focused experiments.

      (1) Some of the conclusions of the paper mainly rely on bioinformatic analyses of RNA-seq data. For example, it has been noted in several places in the paper that the knockout of FAK in Vill-Cre/BRAF-V600E mice does not affect the transcriptional outcome downstream of ERK while ERK phosphorylation levels are decreased. This statement is based on the lack of significant difference in the MAPK signature according to GSEA. However, whereas a significant enrichment of certain pathways can be used as support evidence, the lack of enrichment does not necessarily indicate those pathways are not involved. Other experiments are needed to examine the expression of ERK target genes to confirm. Similarly, the upregulation of fetal stem cell signature in FAK knockout mice needs to be verified using other methods besides GSEA.

      (2) According to Figure 5i, the half-life of Lgr4 is around 48 hours in HT29 cells. However, it has been reported by at least two other publications cited in this paper (Ref. 44 and 45) that the half-life of Lgr4 is much shorter. This discrepancy is not explained.

      (3) The effect of decreased ERK signaling on NEDD4 expression has only been briefly explored in Figure 6. The mechanisms by which FAK-loss and/or inhibition of MEK/ERK activity regulate NEDD4 expression are currently unclear. Moreover, the levels of NEDD4 expression are only analyzed in one mouse per group in Figure 6a. Quantitative analysis of NEDD4 as well as Lgr4 expression in additional numbers of mice will provide more solid support for the inverse correlation between NEDD4 and Lgr4 proteins. Since MEK inhibitor treatment also increases Lgr4 mRNA expression as shown in Figure 5f-g, the relative contribution of this altered mRNA expression vs. NEDD4L-mediated ubiquitination has not been investigated.

      (4) It is an interesting finding that knockout FAK has no effect on KRAS-G12D-driven hyperplasia as shown in Figure 7. However, additional studies are needed to further explore the potential mechanisms by which FAK-loss specifically decreases EGFR/ERK signaling in the context of BRAF-V600E mutation.

    1. Reviewer #2 (Public Review):

      Summary:

      To investigate the evolutionary relationship between the RNAi pathway and innate immunity, this study uses biochemistry and structural biology to investigate the trimeric complex of Dicer-1, DRH-1 (a RIGI homologue) and RDE-4 , which exists in C. elegans. The three subunits were co-expressed to promote stable purification of the complex. This complex promoted ATP-dependent cleavage of blunt-ended dsRNAs. A detailed kinetic analysis was also carried out to determine the role of each subunit of the trimeric complex in both the specificity and efficiency of cleavage. These studies indicate that RDE-4 is critical for cleavage while DRC-1 is primarily involved in the specificity of the reaction, and DRH-1 promotes ATP hydrolysis. Finally, a moderate density (6-7 angstrom) cryo-EM structure of the trimeric complex is provided.

      Strengths:

      (1) Newly described methods for studying the C. elegans DICER complex<br /> (2) New structure, albeit only moderate resolution<br /> (3) Kinetic study of the complex in the presence and absence of individual subunits and mutations, provide detailed insight into the contribution of each subunit

      Weaknesses:

      (1) Limited insight due to limited structural resolution.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors noticed that there was an enhanced ability to detect nuclear pore proteins in trypanosomes using a streptavidin-biotin-based detection approach in comparison to conventional antibody-based detection, and this seemed particularly acute for phase-separated proteins. They explored this in detail for both standard imaging but also expansion microscopy and CLEM, testing resolution, signal strength, and sensitivity. An additional innovative approach exploits the proximity element of biotin labelling to identify where interacting proteins have been as well as where they are.

      Strengths:

      The data is high quality and convincing and will have obvious application, not just in the trypanosome field but also more broadly where proteins are tricky to detect or inaccessible due to phase separation (or some other steric limitations). It will be of wide utility and value in many cell biological studies and is timely due to the focus of interest on phase separation, CLEM, and expansion microscopy.

    1. Reviewer #2 (Public Review):

      Wang, Liu, et al. identified Rnf220 and Wdr5 as novel regulators of Hox gene expression during pons development. Phenotypic characterization of Rnf220 deficient mice with single-cell transcriptomics, qRT-PCR, and axonal tracing methods show that Rnf220 knockdown causes de-repression of Hox gene expression at multiple stages of pons development to regulate the final formation of the pontine nuclei neural circuit. Additionally, they also perform exhaustive expression analysis of multiple genes in the Hox family cluster to identify specific gene groups that are targeted by Rnf220. Furthermore, they also demonstrate that Rnf220 modulates Hox gene expression by directly binding to Wdr5, thus targeting it for ubiquitination and subsequent degradation. To elucidate the molecular mechanism of this interaction, they perform detailed immunoprecipitation assays and identify the precise Wdr5 amino acid residues that are targeted by Rnf220. Intriguingly, they show that inhibition of Wdr5 in Rnf220 deficient mice reverses the de-repression of Hox gene expression suggesting the direct involvement of Rnf220-Wdr5 interaction in modulating Hox gene expression during pons development. These data highlight the role of a new form of Hox gene regulation via the ubiquitination of epigenetic modulator Wdr5.

      The conclusions of this paper are mostly supported by the data provided, but the downstream molecular and tissue-level effects of Wdr5 knockdown/inhibition need to be further characterized to establish its definitive role in pons development.

      (1) Figure 1E shows that Rnf220 knockdown alone could not induce an increase in Hox expression without RA, which indicates that Rnf220 might endogenously upregulate Retinoic acid signaling. The authors should test if RA signaling is downstream of Rnf220 by looking at differences in the expression of Retinaldehyde dehydrogenase genes (as a proxy for RA synthesis) upon Rnf220 knockdown.

      (2) In Figure 2C-D further explanation is required to describe what criteria were used to segment the tissue into Rostral, middle, and caudal regions. Additionally, it is unclear whether the observed change in axonal projection pattern is caused due to physical deformation and rearrangement of the entire Pons tissue or due to disruption of Hox3-5 expression levels. Labeling of the tissue with DAPI or brightfield image to show the structural differences and similarities between the brain regions of WT and Rnf220 +/- will be helpful.

      (3) Line 192-195. These roles of PcG and trxG complexes are inconsistent with their initial descriptions in the text - lines 73-74.

      (4) In Figure 4D, the band in the gel seems unclear and erased. Please provide a different one. These data show that neither Rnf220 nor wdr5 directly regulates Hox gene expressions. The effect of double knockdown in the presence of RA suggests that they work together to suppress Hox gene expression via a different downstream target. This point should be addressed in the text and discussion section of the paper. example for the same data which shows a full band with lower intensity.

      (5) In Figure 4G the authors could provide some form of quantitation for changes in ubiquitination levels to make it easier for the reader. They should also describe the experimental procedures and conditions used for each of the pull-down and ubiquitination assays in greater detail in the methods section.

      (6) Figure 5 shows that neither Rnf220 nor wdr5 directly regulate Hox gene expressions. The effect of double knockdown in the presence of RA suggests that they work together to suppress Hox gene expression via a different downstream target. This point should be addressed in the text and discussion section of the paper.

      (7) In Figure 6, while the reversal of changes in Hox gene expression upon concurrent Rnf220; Wdr5 inhibition highlights the importance of Wdr5 in this regulatory process, the mechanistic role of wdr5 and its functional consequences are unclear. To answer these questions, the authors need to: (i) Assay for activated and repressive epigenetic modifications upon double knockdown of Rnf220 and Wdr5 similar to that shown in Figure 4- supplement 1. This will reveal if wdr5 functions according to its intended role as part of the TrxG complex. (ii) The authors need to assay for changes in axon projection patterns in the double knockdown condition to see if Wdr5 inhibition rescues the neural circuit defects in Rnf220 +/- mice.

    1. Reviewer #2 (Public Review):

      Summary:

      Bolamperti S. et al. 2023 investigates whether expression of TG-interacting factor (Tgif1) is essential for osteoblastic cellular activity regarding morphology, adherence, migration/recruitment, and repair. Towards this end, germ-line Tgif1 deletion (Tgif1-/-) mice or male mice lacking expression of Tgif1 in mature osteoblastic and osteocytic cells (Dmp1-Cre+; Tgif1fl/fl) and corresponding controls were studied in physiological, bone anabolic, and bone fracture-repair conditions. Both Tgif1-/- and Dmp1-Cre+; Tgif1fl/fl exhibited decreased osteoblasts on cancellous bone surfaces and adherent to collagen I-coated plates. Tgif1-/- mice exhibit impaired healing in the tibial midshaft fracture model, as indicated by decreased bone volume (BV/Cal.V), osteoid (OS/BS), and low osteoblasts (number and surface). Likewise, both Tgif1-/- and Dmp1-Cre+; Tgif1fl/fl show impaired PTH 1-34, (100 µg/kg, 5x/wk for 3 wks) osteoblast activation in vivo, as detected by increases in quiescent bone surfaces. Mechanistic in vitro studies then utilized primary osteoblasts isolated from Tgif1-/- mice and siRNA Tgif1 knockdown OCY454 cells to further investigate and identify the downstream Tgif1 target driving these osteoblastic impairments. In vitro, Tgif1-/- osteoblastic and Tgif1 knockdown OCY454 cells exhibit decreased migration, abnormal morphology, and decreased focal adhesions/cell. Unexpectantly though, localization assays revealed Tgif1 to primarily concentrate in the nucleus and not to co-localize with focal adhesions (paxillin, talin). Also, expression of major focal adhesion components (paxillin, talin, FAK, Src etc.) or the Cdc42 family was not altered by loss of Tgif1 expression. In contrast, PAK3 expression is markedly upregulated by loss of Tgif1. In silico analysis followed by mechanistic molecular assays involving ChIP, siRNA (Tgif1, PAK3), and transfection (rat PAK3 promoter) techniques show that Tgif1 physically binds to a specific site in the PAK3 promoter region. Further, the knockdown of PAK3 rescues the Tgif1-deficient abnormal morphology in OCY454 cells. This is the first study to identify the novel transcriptional repression of PAK3 by Tgif1 as well as the specific Tgif1 binding site within the PAK3 promoter.

      Strengths:

      This work has a plethora of strengths. The co-authors achieved their aim in eliciting the role of Tgif1 expression to osteoblastic cellular functions (morphology, spreading/attachment, migration). Further, this work is the first to depict the novel mechanism of Tgif1 transcriptional repression of PAK3 by a through usage of mechanistic molecular assays (In silico analysis, ChIP, siRNA, transfection etc.). The conclusions are well supported and justified by these findings, as the appropriate controls, sample sizes (statistical power), statistics, and assays were fully utilized.

      Claims and conclusions justified by data? Yes. absolutely

      Weaknesses:

      None. All reviewer comments were fully addressed.

    1. Reviewer #3 (Public Review):

      Summary:

      Nakai-Futatsugi et al. present a novel method to analyze the correlation between the degree of pigmentation and the gene expression profile of human-induced pluripotent stem cell-derived RPE (iPSC-RPE) cells at the single cell level. This was achieved with the use of ALPS (Automated Live imaging and cell Picking system), an invention developed by the same authors. Briefly, it allows one to choose and photograph a specific cell from a culture dish and proceed to single cell digital RNA-seq. The authors identify clusters of cells that present differential gene expression, but this showed no association with the degree of pigmentation of the cells. Further data analysis allowed the authors to correlate the degree of pigmentation to some degree with the expression of complement and lysosome-related genes.

      Strengths:

      An important amount of data related to gene expression and heterogeneity of the iPSC-RPE population has been generated in this work.

      Weaknesses:

      However, the justification of the analysis, and the physiological relevance of the hypothesis and the findings could be strengthened.

      Importantly, I fail to grasp from the introduction what is the previous evidence that leads to the hypothesis. Why would color intensity be related to the quality of cell transplantation? In fact, cell transplantation is not evaluated at all in this work. The authors mention "quality metrics for clinical use", but this concept is not further explained. Neither is the concept of "sufficient degree of pigmentation" explained.<br /> On the other hand, the positive correlation of cluster formation with complement and lysosome-related genes is not discussed.

      As a consequence it is very difficult to evaluate the impact of these findings on the field.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors conducted research on the role of SerpinE2 and HtrA1 in neural crest migration using Xenopus embryos. The data presented in this study was of high quality and supported the authors' conclusions. The discovery of the potential molecular connection between SerpinE2 and HtrA1 in neural crest cell migration in vivo is significant, as understanding this pathway could potentially lead to treatments for aggressive cancers and pregnancy-related disorders.

      Strengths:

      Previous research has shown that SerpinE2 and HtrA1 can have both positive and negative effects on cell migration, but their molecular interplay and role in neural crest migration are not well-established. This study is the first to reveal a potential connection between these two proteins in neural crest cell migration in vivo. The authors found that SerpinE2 promotes neural crest migration by inhibiting HtrA1. Additionally, overexpression of Sdc4 partly alleviates neural crest migration issues caused by SerpinE2 knockdown or HtrA1 overexpression. These findings suggest that the SeprinE2-HtrA1-Sdc4 pathway is crucial for neural crest migration.

      Weaknesses:

      To further increase the study's credibility, it may be helpful to use techniques like western blotting, qRT-PCR, or in situ hybridization to verify the efficiency of SerpinE2 and HtrA1 knockdown and/or overexpression.

    1. Reviewer #2 (Public Review):

      Summary:

      The manuscript expands the current bulk sequencing data deconvolution toolkit to include ATAC-seq. The EPIC-ATAC tool successfully predicts accurate proportions of immune cells in bulk tumour samples and EPIC-ATAC seems to perform well in benchmarking analyses. The authors achieve their aim of developing a new bulk ATAC-seq deconvolution tool.

      Strengths:

      The manuscript describes simple and understandable experiments to demonstrate the accuracy of EPIC-ATAC. They have also been incredibly thorough with their reference dataset collections. The authors have been robust in their benchmarking endeavours and measured EPIC-ATAC against multiple datasets and tools.

      Weaknesses:

      Currently, the tool has a narrow applicability in that it estimates the percentage of immune cells in a bulk ATAC-seq experiment.

      Comments:

      (1) Has any benchmarking been done on the runtime of the tool? Although EPIC-ATAC seems to "win" in benchmarking metrics, sometimes the differences are quite small. If EPIC-ATAC takes forever to run, compared to another tool that is a lot quicker, might some people prefer to sacrifice 0.01 in correlation for a quicker running tool?

      (2) In Figure 3B the data points look a bit squashed in the bottom-left corner. Could the plot be replotted with the data point spread out? There also seems to be some inter-patient variability. Could the authors comment on that?

      (3) Could the authors comment on the possibility of expanding EPIC-ATAC into more than a percentage prediction tool? Perhaps EPIC-ATAC could remove the immune cell signal from the bulk ATAC-seq data to "purify" the uncharacterised cells in silico, or generate pseudo-ATAC-seq tracks of the identified cell types.

    1. Reviewer #2 (Public Review):

      Summary:

      In their manuscript entitled "In vitro function, assembly and interaction of primary cell wall cellulose synthase homotrimers" Purushotham et al. purify and functionally and structurally characterize the primary cell wall cellulose synthase isoforms from soybeans. Overall, the manuscript is well-written and contributes several important observations.

      Strengths:

      The structural and functional characterization of all three primary cell wall CesA isoforms contributes significantly to important problems in plant biochemistry.

      The demonstration that the isolated CesA monomers and homotrimers are catalytically active in vitro, interact with each other, and show catalytic cooperativity between the homotrimers.

      Weaknesses:

      The paper could be further strengthened by addressing the following:

      Are the interactions between the homotrimers observed via the pull-down assays stable enough to co-elute on the sizing column or are they transient interactions?

      The authors show that the monomeric CesA isoforms can interact with each other using pull-down assays (Figure Supplement 4e). Are these interactions stable or transient? Have the authors tried running the mixed monomers over a sizing column? If you mix all three isoform monomers can you form heterotrimers?

      The authors demonstrate via truncation that the N-terminus of the CesA is not involved in the interactions between the isoforms and propose that the CSR hook-like extensions are the primary mediator of trimer-trimer interactions. This argument would be strengthened by equivalent truncation experiments in which the CSR region is removed.

      The statement on page 6 that "All CesA isoforms show greatest catalytic activity at neutral pH" seems to contradict the data in Figure 1e and the subsequent statements.

    1. Reviewer #2 (Public Review):

      In the manuscript entitled "Noncaloric monosaccharides induce excessive sprouting angiogenesis in zebrafish via foxo1a-marcksl1a signal". Liu et al. observed that glucose and noncaloric monosaccharides can prompt an excessive formation of blood vessels, particularly intersegmental vessels (ISVs). They propose that these branched vessels arise from the ectopic activation of quiescent endothelial cells (ECs) into tip cells. Moreover, through single-cell transcriptome sequencing analysis of embryonic endothelial cells exposed to glucose, they noted an increased proportion of arterial and capillary endothelial cells, proliferative endothelial cells, along with a series of upregulated genes in categories of blood vessel morphogenesis, development, and pro-angiogenesis. The authors provide evidence suggesting that caloric and noncaloric monosaccharides (NMS) induce excessive angiogenesis via the foxo1a-Marcksl1a pathway.

      The authors address an important problem about the effects of artificially sweetened beverages such as noncaloric monosaccharides on blood vessels. However, the study lacks adequate experimental data and comprehensive analyses to support the mechanistic conclusions, which require extensive revisions.

    1. Reviewer #2 (Public Review):

      This study investigates the excitability of neurons in the peri-infarct cortex during recovery from ischemic stroke. The excitability of neurons in the peri-infarct cortex during stroke recovery has produced contradictory findings: some studies suggest hyper-excitability to direct-brain stimulation, while others indicate diminished responsiveness to physical stimuli. However, most studies have used anesthetized animals, which can disrupt cortical activity and functional connectivity. The present study used two-photon Ca2+ imaging after focal photothrombotic stroke to examine neural activity patterns in awake mice. The authors found reduced neuronal spiking in the peri-infarct cortex that was strongly correlated with motor performance deficits. Additionally, the authors found disruptions in neural activation, functional connectivity, and assembly architecture in the immediate peri-infarct region but not in the distal cortex regions.

      The findings of this study are very important as they show that there is no measurable change in terms of neuronal activation and reorganization in distal regions of remapped cortical response areas after stroke.

    1. Reviewer #2 (Public Review):

      Summary:

      This study provides an important overview of infectious etiology for neurodevelopment delay.

      Strengths:

      Strong RNA evaluation.

      Weaknesses:

      The study lacks an overview of other infectious agents. The study should address the epigenetic contributors (PMID: 36507115) and the role of supplements in improving outcomes (PMID: 27705610).<br /> Addressing the above - with references included - is recommended.

    1. Reviewer #2 (Public Review):

      Summary:

      This is an important and very interesting report on a change in newborns' neural abilities to distinguish auditory signals as a function of the gestational age (GA) of the infant at birth (from 35 weeks GA to 40 weeks GA). The authors tested neural discrimination of sounds that were labeled 'happy' vs 'neutral' by listeners that represent two categories of sound, either human voices or auditory signals that mimic only certain properties of the human vocal signals. The finding is that a change occurs in neural discrimination of the happy and neutral auditory signals for infants born at or after 37 weeks of gestation, and not prior (at 35 or 36 weeks of gestation), and only for discrimination of the human vocal signals; no change occurs in discrimination of the nonhuman signals over the 35- to 40-week gestational ages tested. The neural evidence of discrimination of the vocal happy-neutral distinction and the absence of the discrimination of the control signals is convincing. The authors interpret this as a 'landmark' in infants' ability to detect changes in emotional vocal signals, and remark on the potential value of the test as a marker of the infants' interest in emotional signals, underscoring the fact that children at risk for autism spectrum disorder may not show the discrimination. Although the finding is novel and interesting, additional discussion is essential so that readers understand two potential caveats affecting this interpretation.

      Strengths:

      The event-related potential (ERP) method and results are clear, well-described, and convincing.

      Weaknesses/ Information needed:

      First, readers need to see spectrograms that show the 0-4000 Hz in more detail, rather than what is now shown (0-10,000 Hz). The vocal signals in clearer spectrograms will show I believe the initial consonant burst and formant frequencies that are unique to human speech and give rise to the perception of the consonant sounds in the vocal signals like 'dada' and 'tutu' that were tested. The control signals will presumably not show these abrupt acoustic changes at their onset, even though they appear (from the oscillograms) to approximate the amplitude envelope. The primary cue distinguishing the happy and neutral signals in both the vocal and control signals is the pitch of the signals (high vs low), but the burst of energy representing the consonants is only contained in the vocal signals; it has no comparable match in the control signals. It is possible that the presence of a sharp acoustic onset (a unique characteristic of consonants in human speech) is especially alerting to the infants, and that this acoustic cue, in the context of the pitch change, enhances discrimination in the vocal case. One way to test this would be to use only vowel sounds to represent the vocal signals, without consonants. Another critical detail that the authors need to include about the signals is an explanation of how the control signals were generated. The text states that the Fo and amplitude envelope of the vocal signals were mimicked in the control signals, but what was the signal used for the controls? Was a pure tone complex modulated, or was pink noise used to generate the control signals? Or were the original vocal signals simply filtered in some way to create the controls, which would preserve the Fo and amplitude envelope? If merely filtered, the control signals still may be perceived as 'vocal' signals, rather than as nonspeech (the Supplement contains the sounds, and some of the control sounds can be perceived, to my ear, as 'vocal' signals).

      Second, there is no information in the manuscript or supplement about the auditory environment of the participants, nor discussion of the fetus' ability to hear in the womb. In the womb, infants are listening to the mothers' bone-conducted speech (which is full of consonant sounds), and we know from published studies that infants can discern differences not only in the prosody of the speech they hear in the womb, but the phonetic characteristics of the mother's speech. The ability at 37 weeks GA or beyond to discriminate the pitch changes in the vocal, but not control signals, could thus be due to additional experience in utero to speech. Another experiential explanation is that the infants born at 37 weeks GA and beyond may be exposed to greater amounts of speech after birth, when compared to those born at 35 and 36 weeks GA, from the attending nurses and from their caregivers, and this speech is also full of consonant sounds. What these infants hear is likely to be 'infant-directed speech,' which is significantly higher in pitch, mirroring the signals tested here. At 37 weeks GA, infants are likely more robust, may sleep less, and are likely more alert. If infants' exposure to speech, either after birth, or their auditory ability to discern differences in speech in utero, is enhanced at 37 weeks GA and beyond, then an 'experience-related' explanation is a viable alternative to a maturational explanation, and should be discussed. Perhaps both are playing a role. As the authors state, many more signals need to be tested to discern how the effect should be interpreted, and other viable interpretations of the current results discussed.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors develop a highly detailed pipeline to analyze hemodynamic signals from in vivo two-photon fluorescence microscopy. This includes motion correction, segmentation of the vascular network, diameter measurements across time, mapping neuronal position relative to the vascular network, and analyzing vascular network properties (interactions between different vascular segments). For the segmentation, the authors use a Convolution Neural Network to identify vessel (or neural) and background pixels and train it using ground truth images based on semi-automated mapping followed by human correction/annotation. Considerable processing was done on the segmented images to improve accuracy, extract vessel center lines, and compute frame-by-frame diameters. The model was tested with artificial diameter increases and Gaussian noise and proved robust to these manipulations.

      Network-level properties include Assortativity - a measure of how similar a vessel's response is to nearby vessels - and Efficiency - the ease of flow through the network (essentially, the combined resistance of a path based on diameter and vessel length between two points).

      Strengths:

      This is a very powerful tool for cerebral vascular biologists as many of these tasks are labor intensive, prone to subjectivity, and often not performed due to the complexity of collecting and managing volumes of vascular signals. Modelling is not my specialty so I cannot speak too specifically, but the model appears to be well-designed and robust to perturbations. It has many clever features for processing the data.

      The authors rightly point out that there is a real lack in the field of knowledge of vascular network activity at single-vessel resolution. Network anatomy has been studied, but hemodynamics are typically studied either with coarse resolution or in only one or a few vessels at a time. This pipeline has the potential to change that.

      Weaknesses:

      The authors apply their method to in vivo data. However, there are some weaknesses in the design that make it hard to accept many of the conclusions and even to see that the method could yield much useful data with this type of application. Primarily, the acquisition of a large volume of tissue is very slow. In order to obtain a network of vascular activity, large volumes are imaged with high resolution. However, the volumes are scanned once every 42 seconds following stimulation. Most vascular responses to neuronal activation have come and gone in 42 seconds so each vessel segment is only being sampled at a single time point in the vascular response. So all of the data on diameter changes are impossible to compare since some vessels are sampled during the initial phase of the vascular response, some during the decay, and many probably after it has already returned to baseline. The authors attempt to overcome this by alternating the direction of the scan (from surface to deep and vice versa). But this only provides two sample points along the vascular response curve and so the problem still remains.

      A second problem is the use of optogenetic stimulation to activate the tissue. First, it has been shown that blue light itself can increase blood flow (Rungta et al 2017). The authors note the concern about temperature increases but that is not the same issue. The discussion mentions that non-transgenic mice were used to control for this with "data not shown". This is very important data given these earlier reports that have found such effects and so should be included. Secondly, there doesn't seem to be any monitoring of neural activity following the photo-stimulation. The authors repeatedly mention "activated" neurons and claim that vessel properties change based on distance from "activated" neurons. But I can't find anything to suggest that they know which neurons were active versus just labeled. Third, the stimulation laser is focused at a single depth plane. Since it is single-photon excitation, there is likely a large volume of activated neurons. But there is no way of knowing the spatial arrangement of neural activity and so again, including this as a factor in the analysis of vascular responses seems unjustified.

      The study could also benefit from more clear illustration of the quality of the model's output. It is hard to tell from static images of 3-D volumes how accurate the vessel segmentation is. Perhaps some videos going through the volume with the masks overlaid would provide some clarity. Also, a comparison to commercial vessel segmentation programs would be useful in addition to benchmarking to the ground truth manual data.

      Another useful metric for the model's success would be the reproducibility of the vessel responses. Seeing such a large number of vessels showing constrictions raises some flags and so showing that the model pulled out the same response from the same vessels across multiple repetitions would make such data easier to accept.

      A number of findings are questionable, at least in part due to these design properties.

      There are unrealistically large dilations and constrictions indicated. These are likely due to artifacts of the automated platform. Inspection of these results by eye would help understand what is going on.

      In Figure 6, there doesn't seem to be much correlation between vessels with large baseline level changes and vessels with large stimulus-evoked changes. It would be expected that large arteries would have a lot of variability in both conditions and veins much less. There is also not much within-vessel consistency. For instance, the third row shows what looks like a surface vessel constricting to stimulation but a branch coming off of it dilating - this seems biologically unrealistic.

      As mentioned, the large proportion of constricting capillaries is not something found in the literature. Do these happen at a certain time point following the stimulation? Did the same vessel segments show dilation at times and constriction at other times? In fact, the overall proportion of dilators and constrictors is not given. Are they spatially clustered? The assortativity result implies that there is some clustering, and the theory of blood stealing by active tissue from inactive tissue is cited. However, this theory would imply a region where virtually all vessels are dilating and another region away from the active tissue with constrictions. Was anything that dramatic seen?

      As mentioned, the claims about distance to active neurons are not meaningful if there is no measure of which neurons were active and which weren't. But even still, the claim is overly strong as the average distance to the nearest neuron for dilators was ~17 microns and for constrictors it was ~22 microns - about a half a neuronal soma difference.

      The distance to the nearest neuron likely will depend on depth as well - neurons are quite sparse superficially and very dense in layer 4. The capillary network varies much less (see Blinder et al 2016 Nature Neuroscience). So the distance of a neuron to the nearest capillary may not vary much with depth, but the distance from the capillary to the nearest neuron might vary quite a lot.<br /> Why were nearly all vessels > 5um diameter not responding >2SD above baseline? Did they have highly variable baselines or small responses? Usually, bigger vessels respond strongly to local neural activity.

    1. Reviewer #2 (Public Review):

      Summary:

      The research conducted by Yaning Cui and colleagues delves into understanding FLS2-mediated immunity. This is achieved by comparing the spatiotemporal dynamics of a FLS2-S938A mutant and FLS2-WT, especially in relation to their association with the remorin protein. To delineate the differences between the FLS2-S938A mutant and FLS2-WT, they utilized a plethora of advanced fluorescent imaging techniques. By analyzing surface dynamics and interactions involving the receptor signal co-receptor BAK1 and remorin proteins, the authors propose a model of how FLS2 and BAK1 are assembled and positioned within a remorin-specific nano-enviroment during FLS2 ligand-induced immune responses.

      Strengths:

      These techniques offer direct visualizations of molecular dynamics and interactions, helping us understand their spatial relationships and interactions during innate immune responses.

      Advanced cell biology imaging techniques are crucial for obtaining high-resolution insights into the intracellular dynamics of biomolecules. The demonstrated imaging systems are excellent examples to be used in studying plant immunity by integrating other functional assays.

      Weaknesses:

      It's essential to acknowledge that every fluorescence-based method, just like biochemical assays, comes with its unique limitations. These often pertain to spatial and temporal resolutions, as well as the sensitivity of the cameras employed in each setup. Meticulous interpretation is pivotal to guarantee an accurate depiction and to steer clear of potential misunderstandings when employing specific imaging systems to analyze molecular attributes. Moreover, a discerning interpretation and accurate image analysis can offer invaluable guidance for future studies on plant signaling molecules using these nice cell imaging techniques.

      For instance, although single-particle analysis couldn't conclusively link FLS2 and remorin, FLIM-FRET effectively highlighted their ligand-triggered association and the disengagement brought on by mutations. While these methodologies seemed to present differing outcomes, they were described in the manuscript as harmonious. In reality, these differences could highlight distinct protein populations active in immune responses, each accentuated differently by the respective imaging techniques due to their individual spatial and temporal limitations. Addressing these variations is imperative, especially when designing future imaging explorations of immune complexes.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors present a framework for exploiting shotgun metagenomics and metabolomics data along with constraint-based analysis (CBA) to study, in their case, the dynamics and interactions between the apple rootstock and rhizosphere's microbial community. This study should be considered as a follow-up of Berihu et al. (2022) where the shotgun data were first introduced. A set of 395 Metagenome-Assembled Genomes (MAGs) was derived from those reads and from the latter, using an automatic Genome-scale Metabolic Model (GSMM) reconstruction tool (CarveMe), 243 GSMMs. Metabolomics data from a set of studies were gathered to describe/represent root exudates. Flux Variability Analysis (FVA), a type of constraint-based analysis, was conducted iteratively. Three distinct in silico media were used (optimal, poor, and realistic, with the latter informed by metabolomics data) to examine the potential impact of root exudates on bacterial growth. Additionally, the study investigated the extent to which compounds secreted by bacteria could support the growth of other community members. Further, an exchange network representing all potential metabolic exchanges within the rhizosphere community was built and motifs on it were classified with healthy and/or symptomized soil.

      Strengths:

      The study provides a great starting point for how one can bring together shotgun metagenomics and other omics technologies such as metabolomics with metabolic modelling approaches. MAGs and the automatic reconstruction of corresponding GSMMs become more and more a common practice and frameworks for their analysis and interpretation are more than needed. The usage of FVA instead of the Flux Balance Analysis allows the authors to get all the range of potentially produced metabolites. The iterative approach can highlight what species are supported by the plant and which need the first to join the community while correlating microbial metabolic interactions with soil performance through differential abundance can bring up valid hypotheses to examine further. On top of that, avoiding modelling approaches that require community objective functions and optimization of that makes the simulation more realistic.

      Weaknesses:

      There are two main drawback approaches like the one described here, both related only partially to the authors' work yet with great impact in the presented framework. First, the usage of automatic GSMM reconstruction requires great caution. It is indicative of how the semi-curated AGORA models are still considered reconstructions and expect the user to parameterize those in a model. In this study, CarveMe was used. CarveMe is a well-known tool with several pros [1]. Yet, several challenges need to be considered when using it [2]. For example, the biomass function used might lead to an overestimation of auxotrophies. Also, as its authors admit in their reply paper, CarveMe does gap fill in a way [3]; models are constructed to ensure no gaps and also secure a minimum growth. However, curation of such a high number of GSMMs is probably not an option. Further, even if FVA is way more useful than FBA for the authors' aim, it does not yet ensure that when a species secretes one compound (let's say metabolite A), the same flux vector, i.e. the same metabolic functioning profile, secretes another compound (metabolite B) at the same time, even if the FVA solution suggests that metabolite B could be secreted in general.

      Besides those challenges, the suggested framework is promising and such approaches can work as the starting point for the next step in microbial ecology studies in general; from soil to marine and host ecosystems. The authors highlight perfectly this angle stating that this framework is currently conceptual and that it can be only used to formulate new hypotheses. Unbiased constraint-based approaches that focus on metabolite exchanges would benefit such approaches.

      [1] Mendoza, Sebastián N., et al. "A systematic assessment of current genome-scale metabolic reconstruction tools." Genome biology 20.1 (2019): 1-20.<br /> [2] Price, Morgan. "Erroneous predictions of auxotrophies by CarveMe." Nature Ecology & Evolution 7.2 (2023): 194-195.<br /> [3] Machado, Daniel, and Kiran R. Patil. "Reply to: Erroneous predictions of auxotrophies by CarveMe." Nature Ecology & Evolution 7.2 (2023): 196-197.<br /> [4] Ylva Katarina Wedmark, Jon Olav Vik, Ove Øyås bioRxiv 2023.09.05.556413; doi: https://doi.org/10.1101/2023.09.05.556413

  3. Mar 2024
    1. L'enseignant référent qui coordonne les équipes de suivi de la scolarisation est l'interlocuteur des familles pour la mise en place du projet personnalisé de scolarisation.
    2. L'Etat garantit le respect de la personnalité de l'enfant et de l'action éducative des familles
    3. Les familles sont associées à l'accomplissement de ces missions.
    4. La formation scolaire favorise l'épanouissement de l'enfant
    5. Tout enfant a droit à une formation scolaire qui, complétant l'action de sa famille, concourt à son éducation
    1. Reviewer #2 (Public Review):

      In this manuscript, Chen et al. reported that the core binding factor beta (Cbfβ), a heterodimeric subunit of the RUNX family transcription factors (TFs), is crucial in maintaining cartilage homeostasis and counteracting traumatic OA pathology. Using mouse models in which Cbfβ is conditionally inactivated in the Col2a1+ and Acan+ cells, the authors claimed that Cbfβ ablation led to articular cartilage (AC) degeneration, which is associated with aberrant cartilage gene expression and chondrocyte signaling, particularly the elevated Wnt/Catenin and the decreased Hippo/YAP and TGFβ signaling. The authors further showed that Cbfβ transcripts are decreased in human OA cartilage, and sustaining Cbfβ expression in mouse knee joints mitigated the severity of surgery-evoked OA.

      On the whole, the work reported is interesting and exciting. Genetic and biochemical data support key statements. Both in vivo and in vitro experiments were well designed with proper controls; semiquantitative data were digitalized and processed for statistical significance. Furthermore, new findings were adequately discussed in contrast to the current available knowledge. However, the conceptual novelty of this study is slightly compromised by recent publications showing that Cbfβ reduction is associated with OA (Che et al. 2023; Li et al. 2021). Also, the authors claimed that multiple signaling pathways were affected by Cbfβ ablation in cartilage cells; many of them, however, are indirect effects given the nature of Cbfβ as a TF. The authors also showed that pSMAD2/3 and active βCatenin decreased and increased upon Cbfβ depletion in the mouse AC cartilage. However, how the deficiency of Cbfβ, a widely expressed TF, affected the posttranslational modification of SMAD2/3 and βCatenin is unclear and needs further discussion. Overall, Cbfβ's role in cartilage and OA pathology is an emerging area of study; the authors provided a set of genetic evidences showing that Cbfβ is indispensable for cartilage homeostasis.

    1. Reviewer #2 (Public Review):

      The manuscript expands on the previous work from the lab where novel interactors of Rac1 GTPase (CYRI-A and B) provide localized inhibition by sequestration of activated Rac1. These novel regulators are fascinating as they complement the functions of the classical negative modulators of GTPases, GAPs and GDIs. The current manuscript focuses on the in vivo role of CYRI-B in pancreatic cancer progression, and distinct CYRI-B functions are shown for early and later stages. The in vivo data following CYRI-B depletion (no change in proliferation, reduced metastatic potential) is substantiated with in vitro analyses of receptor uptake, temporal recruitment of CYRI-B on macropinosomes and reduced chemotaxis.

      The authors describe in detail the role of CYRI-B in pancreatic adenocarcinoma, building from their prior studies mapping CYRI-B function in the regulation of polarity, motility and chemotaxis. The experiments are well-designed and performed, and the text was clearly written. However, the results partially support some of their conclusions. The interpretation of the data and the discussion in the context of human pancreatic tumours would help the understanding and impact of the work.

      The hypothesis is that depletion of CYRI-B would promote localized Rac1 activation at the membrane. However, the authors show that CYRI-B is found overexpressed in PDAC, consistent with other papers where its high expression correlates with poor outcome of many cancers. The prediction is that Rac1 functions modulated by CYRI-B would be inhibited in those tumours where CYRI-B is overexpressed. Is this the case and has it been formally demonstrated?

      Most experiments use the depletion of CYRI-B to probe its function. It would be useful to readers and important to elaborate on how the specific CYRI-B functions shown upon depletion would fit with the in vivo observation of CYRI-B overexpressed in tumours. For example, loss of CYRI-B reduces chemotaxis potential. How this result can be conciliated with the predicted increase in Rac1activation in the absence of CYRI-B? Conversely, a prediction of CYRI-B overexpression in human tumours would imply the inactivation of Rac1 whereas chemotaxis is promoted. The discussion could be improved with the addition of the authors' views and further explanations in this context.

      Similarly, it is confusing to extrapolate a proposed increase in LPAR1 internalization by macropinocytosis with CYRI-B overexpression in PDAC. It is predicted that Rac1 would be locally inhibited in this scenario, and thus micropinocytosis would be compromised. It will be good to spell out what the authors envisage happens. For example, uptake could be switched to another receptor uptake process that would not involve CYRI-B sequestration of Rac1. Discussion of the potential alternatives will strengthen the manuscript.

      "..LPAR1 is a cargo of CYRI-B dependent macropinocytosis" (page 21). This statement reads as an overinterpretation of the specificity of the process. It may suggest that there is a cargo selectivity by CYRI-B, which has not been formally demonstrated or is well accepted. Macropinocytosis is thought to occur as a bulk engulfment of the membrane and thus any receptor at the cell surface would be internalised non-specifically. The demonstrated reduction in LPAR1 uptake could be proportional to the interference with micropinocytosis rate by CYRI-B depletion for example

      Furthermore, the readers would benefit from more clear explanations of the differences and similarities between CYRI-A and CYRI-B. It will be important to clarify the specificity of the proposed functions of each protein. Both localize at the macropinosomes, modulate engulfment and regulate integrin a5b1 trafficking. It will be informative to specify if CYRI-A is also upregulated in human tumours, has a similar outcome as CYRI-B in vivo and also regulates LPAR1 uptake.

      Upon depletion of CYRI-B in pancreatic tumour cells in vivo, the presence of similar levels of jaundice is confusing. Less metastasis is detected in the mesentery. Are liver metastasis affected in the absence of CYRI-B?

    1. Reviewer #2 (Public Review):

      Schwann cells actively repair and regenerate peripheral nerves following tissue injury. Central to this process is the collective cell migration of 'cords' of Schwann cells, which guide the regenerating axons across an injury site. Previously published research from the Lloyd lab shows that at the injury site, Schwann cell cords are maintained via N-cadherin-based cell-cell adhesions; however, when cultured under low density conditions, Schwann cells display cell repulsion and contact inhibition of locomotion (CIL) phenotypes, suggesting Schwann cell behaviour is plastic. In this study, Hoving, Lloyd and colleagues build upon their previous work to show that Slit2/3/Robo signalling triggers cell repulsion between Schwann cells in an N-cadherin-dependent manner. This in turn induces contact inhibition of locomotion to propel Schwann cells to migrate collectively and with direction. The authors show that N-cadherin has a dual function in Schwann cell migration: to keep migrating Schwann cells together as a group, and concomitantly present Slit2/3 repulsive cues to cells to trigger cell repulsion locally. Their data also show that extracellular N-cadherin is required for cell repulsion, independent of cell-cell adhesion functions. The authors use a combination of in vitro Schwann cell cultures and live cell imaging, with an ex vivo precision cut tissue slice system to show that Slit2/3-dependent CIL underpins proper Schwann cell migration in an injury model.

      This is a very well executed and important study, which provides new insights into mechanisms of CIL and places CIL in the context of tissue repair and regeneration in adult tissues. The experiments are well designed, and the main findings and conclusions are based on robust and convincing data.

    1. Reviewer #2 (Public Review):

      It is well-known that repeated exposure to perceptual stimuli improves discrimination performance, but less is known about the effects on perceptual appearance. In the present work, the authors tackle this question and focus on one particular effect on perceptual appearance termed boundary avoidance, i.e. the tendency to perceive (or report) a stimulus as biased away from a discrimination boundary.

      In the study, participants performed either a motion discrimination task (clockwise or counterclockwise with respect to a reference axis) or an estimation task (reproducing the orientation of the motion stimulus). Participants were divided in three groups which either i) trained on the discrimination task, ii) trained on the estimation task or iii) received no training (control group). Performance in both tasks was assessed prior and after training. The main behavioral finding is that training (which did not involve feedback) improved discrimination performance and increased estimation precision, but at the same time appeared to increase the boundary avoidance effect. Thus, the authors conclude that perceptual learning improved performance at the cost of appearance.

      To explain these effects, the authors created a computational model in which performance improvements were implemented as a gain increase of neurons sensitive to the trained motion directions. Repulsive biases away from the reference orientation were implemented by a combination of two modeling choices: i) Even during estimation, participants perform an implicit categorization such that they assume that their percept was created by a stimulus in line with their categorization (clockwise or counterclockwise). This effectively biases their response away from the boundary. ii) There is an abundance of neurons tuned to the horizontal reference axis (the "boundary") which likewise leads to a repulsive bias. Overall, the authors conclude that the model was able to explain the major behavioral effects, including the a priori presence of repulsive biases, the increase in performance, the increase in estimation precision and the increase of the repulsive bias.

      It is well-known that repeated exposure to perceptual stimuli improves discrimination performance, but less is known about the effects on perceptual appearance. In the present work, the authors tackle this question and focus on one particular effect on perceptual appearance termed boundary avoidance, i.e. the tendency to perceive (or report) a stimulus as biased away from a discrimination boundary. On first glance, it was a pleasure reading this paper due to a number of aspects the authors got quite right in my opinion:<br /> - A clear and well-explained research question.<br /> - The results are generally well-presented. Much effort and expertise was put into the Figures and many helpful auxiliary Figures are included as a Supplement.<br /> - The writing was concise and clear.

      However, as outlined below, I'm afraid that the main conclusion of the study and the main motivation for computational modeling are not backed up by the data.

      (1) No evidence for a change in overestimation<br /> Overestimation is (rightly) defined by the authors as a bias of the perceived orientations towards more extreme values (visualized also in Fig. 2F). However, as acknowledged by the authors, there is nearly no evidence for such an effect. The modal estimation response (correct trials) doesn't change significantly between the sessions. The mean, which is the primary measure used by the authors, is not an appropriate measure for an overestimation, as it is severely biased by accuracy. It was unclear to me why it was chosen as the primary measure for nearly all figures and analyses, given that the authors were aware of (and reported) a more suited measure.

      In my opinion, the mode of the correct responses would be the best way to quantify the overestimation bias. An alternative would be looking at the average absolute (unsigned) distance from the boundary, possibly including both correct and incorrect responses. However, such a "mean of absolute differences" approach would be affected by lucky guessing trials, which could manifest in a probability mass close to the boundary (and the proportion of which changes with overall accuracy). Therefore I see the mode as the strongest and least confounded measure.

      (2) Nature of the biases<br /> Although, as outlined in 1), there might actually be no evidence for a *change* in overestimation bias, there clearly was a baseline overestimation bias. However, the reported biases appear extremely large. For instance, for the 2{degree sign} orientation the modal estimation is close to 20{degree sign}. To me this raises the question whether we're really dealing with a pure perceptual effect (18{degree sign} misperception seems quite suboptimal) or whether there are some other psychological effects at work that could be rather classified as a response bias.

      In particular, I wondered whether the baseline bias is partly explained by participants "wanting to make sure" they indicate the correct category in estimation and therefore bias their estimation response away from the ambiguous proximity of the cardinal axes? Does it require more effort to set estimation orientation close to a cardinal axis while still making sure that it has the correct categorical orientation. I guess there was no horizontal reference line on the screen which would help with this?

      The overall discrimination-focused task design might have contributed to this bias. First, because the participants trained on estimation also performed a discrimination task (pre/post) which very likely could have affected their response style. Second, the presented orientations during estimation were likewise 50:50 around the horizontal reference which could shift the focus towards "getting the sign right" rather than "getting the precise orientation right".

      (3) The mechanism of the model<br /> As a disclaimer a priori, I am not very familiar with this particular modeling literature (but this may be the case for other readers as well). For this reason I could have used a bit more guidance about how the model works. My understanding is that there a three key mechanisms: 1) Gain modulation which explains the improvement in discrimination; 2) Warping which partly explains boundary avoidance; 3) Implicit categorization which likewise partly explains boundary avoidance. In addition, there are two levels of analysis: 1) the pre-training state (a priori presence of a repulsive bias) and 2) learning effects (bias and performance increase through training). If the models were to be kept as part of a revised manuscript, my suggestion would be to structure the corresponding section in the Results ("Observer Model") a bit more along these anchors. I suggest also providing a bit more explanation already at this point. For instance, I consider the fact that implicit categorization effectively works through Bayes rule by assuming a uniform(?) prior over either the negative or positive orientation axis, as very relevant. I assume that other priors would have been conceivable for conditioning on the response, e.g. taking into account the actual (objective or subjective) distribution of orientations for the particular choice category, so this is a non-trivial modeling choice.<br /> Intuitively, I would have also thought that if more resources are devoted to the cardinal directions (and the decoder is unaware of this), this would lead to a bias *towards* the cardinal directions. If more neurons fire particularly strong to near-cardinal orientations (such as the +-4{degree sign} in training), why would the decoder be repulsed *away* from the cardinal orientation? I trust the authors that the presentation is correct, but to me, this was not obvious and I would have wished for some guidance.

    1. Reviewer #2 (Public Review):

      This manuscript describes a new algorithm for clonal family inference based on V and J gene identity, sequence divergence in the CDR3 region, and shared mutations outside the CDR3. Specifically, the algorithm starts by grouping sequences that have the same V and J genes and the same CDR3 length. It then performs single-linkage clustering on these groups based on CDR3 Hamming distance, then further refines these groups based on shared mutations.

      Although there are a number of algorithms that use a similar overall strategy, a couple of aspects make this work unique. First, a persistent challenge for algorithms such as this one is how to set a cutoff for single-linkage clustering: if it is too low, then one separates clusters that should be together, and if too high one joins together clusters that should be separate. Here the authors leverage a rich collection of probabilistic tools to make an optimal choice. Specifically, they model the probability distributions of within- and between-cluster CDR3 Hamming distances, with parameters depending on CDR3 length and the "prevalence" of clonal sequence pairs (i.e. family size distribution). This allows the algorithm to make optimal choices for separating clusters, given the particular chosen distance metric, and assuming the sample in question has been accurately modeled. Second, the algorithm uses a highly efficient means of doing single-linkage clustering on nucleotide sequences.

      This leads to a fast and highly performant algorithm on data meant to replicate the original sample used in algorithm design. The ideas are new and beautifully developed. The application to real data is interesting, especially the point about dN/dS.

      However, the paper leaves open the question of how this inference algorithm works on samples other than the one used for simulation and as a template for validation. If I understand the simulation procedure correctly - that one takes a collection of inferred trees from the real data, then re-draws the root sequence and the identity of the mutations on the branches - then the simulated data should be very close to the data used to develop the methods in the paper. This consideration seems especially important given that key methods in this paper use mutation counts and overall mutation counts are preserved.

      Repertoires come in all shapes and sizes: infants to adults, healthy to cancerous, and naive to memory to plasma-cell-just-after-vaccination. If this is being proposed as a general-purpose clonal inference algorithm rather than one just for this sample, then a more diverse set of validations are needed.

      It is unclear how to run the code. The software repo has a nice readme explaining the file layout, dependencies, and input file format, but the repo seems to be lacking an `inference.ipynb` mentioned there which runs an analysis. Perhaps this is a typo and refers to `inference.py`, which in addition to the documented cdr3 clustering, seems to have functions to run both clustering methods. However, it does not seem to have any documentation or help messages about how to run these functions.

      The results are not currently reproducible, because the simulated data is not available. The data availability statement says that no data have been generated for this manuscript, however simulated data has been generated, and that is a key aspect of the analysis in the paper.

      More detail is needed to understand the timing comparisons. The new software is clearly written to use many threads. Were the other software packages run using multiple threads? What type of machine was used for the benchmarks?

    1. Reviewer #2 (Public Review):

      I completely agree with the basic thrust of this study. Yes, of course, machine learning is FAR better than any variant of PCA for the paleosciences. I agree with the authors' critique early on that this point is not new per se - it is familiar to most of the founders of the field of GMM, including this reviewer. A crucial aspect is the dependence of ALL of GMM, PCA or otherwise, on the completely unexamined, unformalized praxis by which a landmark configuration is designed in the first place. I must admit that I am stunned by the authors' estimate of over 32K papers that have used PCA with GMM.

      But beating a dead horse is not a good way of designing a motor vehicle. I think the manuscript needs to begin with a higher-level view of the pathology of its target disciplines, paleontology and paleoanthropology, along the lines that David Hull demonstrated for numerical taxonomy some decades ago. That many thousands of bad methodologies require some sort of explanation all of their own in terms of (a) the fears of<br /> biologists about advanced mathematics, (b) the need for publications and tenure, (c) the desirability of covers of Nature and Science, and (d) the even greater glory of getting to name a new "species." This cumulative pathology of science results in paleoanthro turning into a branch of the humanities, where no single conclusion is treated as stable beyond the next dig, the next year or so of applied genomics, and the next chemical trace analysis. In short, the field is not cumulative.

      It is not obvious that the authors' suggestion of supervised machine learning will remedy this situation, since (a) that field itself is undergoing massive changes month by month with the advent of applications AI, and even more relevant (b) the best ML algorithms, those based on deep neural nets, are (literally) unpublishable - we cannot see how their decisions have actually been computed. Instead, to stabilize, the field will need to figure out how to base its inferences on some syntheses of actual empirical theories.

      It's not that this reviewer is cynical, but it is fair to suggest a revision conveying a concern for the truly striking lack of organized skepticism in the literature that is being critiqued here. A revision along those lines would serve as a flagship example of exactly the deeper argument that reference (17) was trying to seed, that the applied literature obviously needs a hundred times more of. Such a review would do the most good if it appeared in one of the same journals - AJBA, Evolution, Journal of Human Evolution, Paleobiology - where the bulk of the most highly cited misuses of PCA themselves have appeared.

    1. Reviewer #2 (Public Review):

      Summary:

      Wang and collaborators have evaluated the impact of inflammation on bone loss induced by Doxorubicin, which is commonly used in chemotherapy to treat various cancers. In mice, they show that a single injection of Doxorubicin induces systemic inflammation, leukopenia, and a significant bone loss associated with increased bone-resorbing osteoclast numbers. In vitro, the authors show that Doxorubicin activates the AIM2 and NLRP3 inflammasomes in macrophages and neutrophils. Importantly, they show that the full knockouts (germline deletions) of AIM2 (Aim2-/-) and NLRP3 (Nlrp3-/-) and Caspase 1 (Casp1-/-) limit (but do not completely abolish) bone loss induced 4 weeks after a single injection of Doxorubicin in mice. From these results, they conclude that Doxorubicin activates inflammasomes to cause inflammation-associated bone loss.

      Strength:

      This manuscript provides functional experiments demonstrating that NRLP3 and/or AIM2 loss-of-functions (and thus the systemic impairment of the inflammatory response) prevent bone-loss induced by Doxorubicin in mice.

      Weaknesses:

      Numerous studies have reported that Doxorubicin induces systemic inflammation and activates the inflammasome in myeloid cells and various other cell types. It is also known that systemic inflammation and Doxorubicin treatment lead to bone loss. Hence, the key conclusions drawn from this work have been known already or were very much expected. Therefore, the novelty appears somewhat limited. One important limitation is the lack of experiments that could determine which cell lineages are involved in bone loss induced by Doxorubicin in vivo, while the tools to do so exist. The characterization of the bone phenotype is incomplete, and unfortunately does not tell us whether the inflammasome is activated in some of the cell lineages present in bones in vivo. Another limitation is that the relative importance of the inflammasomes compared to cell senescence and autophagy, which are also induced by Doxorubicin, has not been evaluated. Hence the main molecular mechanisms responsible for bone loss induced by Doxorubicin in vivo remains unknown. Lastly, it would have been interesting, on a more clinical point of view, to compare the few relevant treatments that could limit the deleterious effect of Doxorubicin on bone loss while preserving the toxicity on tumor cells.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors previously generated renal Glut2 knockout mice, which have high levels of glycosuria but normal fasting glucose. They use this as an opportunity to investigate how compensatory mechanisms are engaged in response to glycosuria. They show that renal and hepatic glucose production, but not metabolism, is elevated in renal Glut2 male mice. They show that renal Glut2 male mice have elevated Crh mRNA in the hypothalamus, and elevated plasma levels of ACTH and corticosterone. They also show that temporary denervation of renal nerves leads to a decrease in fasting and fed blood glucose levels in female renal Glut2 mice, but not control mice. Finally, they perform plasma proteomics in male mice to identify plasma proteins with a greater than 25% (up or down) between the knockouts and controls.

      Strengths:

      The question that is trying to be addressed is clinically important: enhancing glycosuria is a current treatment for diabetes, but is limited in efficacy because of compensatory increases in glucose production.

      Weaknesses:

      (1) Although I appreciate that the initial characterization of the mice in another publication showed that both males and females have glycosuria, this does not mean that both sexes have the same mechanisms giving rise to glycosuria. There are many examples of sex differences in HPA activation in response to threat, for example. There is an unfounded assumption here that males and females have the same underlying mechanisms of glycosuria that undermines the significance of the findings.

      (2) The authors state that they induced the Glut2 knockout with taxomifen as in their previous publication. The methods of that publication indicate that all experiments were completed within 14 days of inducing the Glut2 knockout. This means that the last dose of tamoxifen was delivered 14 days prior to the experimental endpoint of each experiment. This seems like an important experimental constraint that should be discussed in this manuscript. Is the glycosuria that follows Glut2 knockout only a temporary change? If so, then the long-term change in glycosuria that follows SGLT2 inhibition in humans might not be best modelled by this knockout. Please specify when the surgeries to implant a jugular catheter or ablate the renal nerves performed relative to the Glut2 knockout in the Methods.

      (3) I am still unclear what group was used for controls. Are these wild-type mice who receive tamoxifen? Are they KspCadCreERT2;Glut2loxP/loxP mice who do not receive tamoxifen? This is important and needs to be specified.

      (4) The authors should report some additional control measures for the renal denervation that could also impact blood glucose and perhaps some of their other measures. The control measures, which one would like to see unimpacted by renal denervation, include body weights, food consumption and water intake, and glycosuria itself.

      (5) The graphical abstract shows a causal link between the hypothalamus and the liver that is unsupported by any of the current findings. That arrow should be removed or a question mark should be added next to the arrow.

      (6) Though the authors have toned down their language implying a causal link between the HPA measures and compensatory elevation of blood glucose in the face of glycosuria, the title still implies this causal link. It is still the case that their data do not support causation. There are many potential ways to establish a causal link but those experiments are not performed here. The renal afferents are correlated with Crh content of the PVN, but nothing has been done to show that the Crh content is important for elevating blood glucose. In light of this, the title should be toned down. Perhaps something like "Renal nerves maintain blood glucose production and elevated HPA activity in response to glycosuria". The link between HPA and glucose is not shown in this paper.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors identify the root cap as an important key region for establishing microbial symbioses with roots. By highlighting for the first time the crucial importance of tight regulation of a specific form of programmed cell death of root cap cells and the clearance of their cell corpses, they start unraveling the molecular mechanisms and its regulation at the root cap (e.g. by identifying an important transcription factor) for the establishment of symbioses with fungi (and potentially also bacterial microbiomes).

      Strengths:

      It is often believed that the recruitment of plant microbiomes occurs from bulk soil to rhizosphere to endosphere. These authors demonstrate that we have to re-think microbiome assembly as a process starting and regulated at the root tip and proceeding along the root axis.

      Weaknesses:

      The study is a first crucial starting point to investigate the spatial recruitment of beneficial microorganisms along the root axis of plants. It identifies e.g. an important transcription factor for programmed cell death, but more detailed investigations along the root axis are now needed to better understand - spatially and temporally - the orchestration of microbiome recruitment.

    1. Reviewer #2 (Public Review):

      Summary:

      This manuscript answers an important question about the transmission of Plasmodium parasites resistant to apicoplast inhibitors, specifically azithromycin. This study builds on previous work showing the inability to transmit parasites resistant to mitochondrial inhibitor, atovaquone, based on fitness defects in transmission stages in the mosquito. The transmissibility of drug-resistant parasites is grounded in the basic biology of the Plasmodium lifecycle and has implications for the selection of drug regimens for clinical treatment, so these questions are highly significant. The authors clearly demonstrate severe defects in mosquito stages of azithromycin-resistant (AZR) P. berghei (rodent species) inhibiting transmission of AZR parasites. However, surprisingly AZR P. falciparum (human species) is unaffected in mosquito stages, rather defects are observed in liver-stage development suggesting AZR P. falciparum can transmit but may not mount a productive blood infection. The differences in the observed defects in the 2 species are important and well demonstrated in the results but are obscured in the title/summary of the manuscript. The results demonstrate that AZR parasites are unlikely to spread.

      Strengths:

      The authors performed experiments with both P. berghei (rodent species) and P. falciparum (human species). P. falciparum is the more relevant species from a clinical standpoint, however, there are limitations to studying the full lifecycle of P. falciparum which only infects humans and some primates, for example requiring humanized mice without intact immune systems. Pberghei is commonly used in lifecycle analyses as a proxy for experimental tractability, however, there are cases where the biology of P. berghei does not reflect that in P. falciparum. So the use of both species is complementary and most informative. Specific modification of the apicoplast genome, where AZR mutations are located, is not currently possible so matched genotypes could not be produced but multiple AZR mutants were analyzed for each species. Acknowledging these limitations in the experimental systems available, the authors perform a thorough set of experiments to pinpoint the specific defects in AZR Pb vs Pf during mosquito and liver developmental stages. The results show phenotypic differences between AZR Pb and Pf in mosquito stages which was not expected but in line with differences in apicoplast biology of Pb vs Pf that are important to document and be aware of when using P. berghei as a model for P. falciparum development.

      Weaknesses:

      The claim that human AZR malaria parasites (P. falciparum) is not readily transmitted to mosquitoes is incorrect, as stated in the title and abstract. Strictly speaking, transmission refers to the infection of a human host by another via mosquitos. The evidence that AZR Pf is unaffected in mosquito development indicates that transmission is not reduced compared to WT Pf. Rather transmitted AZR Pf has disrupted liver stage development and may not mount a productive blood infection. This distinction between the phenotypes of AZR Pb vs Pf is surprising, significant (suggesting differences between Pb and Pf and/or specific mutations in Rpl4), and should be more accurately represented in the title/abstract. To their credit, the authors performed thorough experiments to pinpoint the specific defects in AZR Pb vs Pf, but the current claim about AZR Pf is misleading.

      Additional context:

      Clinical trials (MORDOR studies) in several African countries have shown that biannual administration of azithromycin reduces childhood mortality (PMID: 31167050). The mechanism of this survival benefit is unknown and may be multifactorial. The findings in this manuscript can also be considered in the context that azithromycin is a commonly used antibiotic and may be administered for purposes other than malaria treatment. In theory, AZR-resistant parasites could be selected in asymptomatic patients not receiving malaria treatment but receiving azithromycin. This study indicates that mass distribution of azithromycin for other clinical applications would not result in adverse effects on malaria transmissions in the same population.

    1. Reviewer #2 (Public Review):

      In the manuscript "Modulation of α-Synuclein Aggregation Amid Diverse Environmental Perturbation", Wasim et al describe coarse-grained molecular dynamics (cgMD) simulations of α-Synuclein (aSyn) at several concentrations and in the presence of molecular crowding agents or high salt. They begin by bench-marking their cgMD against all-atom simulations by Shaw. They then carry 2.4-4.3 µs cgMD simulations under the above-noted conditions and analyze the data in terms of protein structure, interaction network analysis, and extrapolated fluid mechanics properties. This is an interesting study because a molecular scale understanding of protein droplets is currently lacking, but I have a number of concerns about how it is currently executed and presented.

      (1) It is not clear whether the simulations have reached a steady state. If they have not, it invalidates many of their analysis methods and conclusions.

      (2) The benchmarking used to validate their cgMD methods is very minimal and fails to utilize a large amount of available all-atom simulation and experimental data.

      (3) They also miss opportunities to compare their simulations to experimental data on aSyn protein droplets.

      (4) Aspects such as network analysis are not contextualized by comparison to other protein condensed phases.

      (5) Data are not made available, which is an emerging standard in the field.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors had previously identified that a colorectal cancer cell line generates small extracellular vesicles (sEVs) via a mechanism where a larger intracellular compartment containing these sEVs is secreted from the surface of the cell and then tears to release its contents. Previous studies have suggested that intraluminal vesicles (ILVs) inside endosomal multivesicular bodies and amphisomes can be secreted by the fusion of the compartment with the plasma membrane. The 'torn bag mechanism' considered in this manuscript is distinctly different because it involves initial budding off of a plasma membrane-enclosed compartment (called the amphiectosome in this manuscript, or MV-lEV). The authors successfully set out to investigate whether this mechanism is common to many cell types and to determine some of the subcellular processes involved.

      The strengths of the study are:

      (1) The high-quality imaging approaches used, seem to show good examples of the proposed mechanism.

      (2) They screen several cell lines for these structures, also search for similar structures in vivo, and show the tearing process by real-time imaging.

      (3) Regarding the intracellular mechanisms of ILV production, the authors also try to demonstrate the different stages of amphiectosome production and differently labelled ILVs using immuno-EM.<br /> Several of these techniques are technically challenging to do well, and so these are critical strengths of the manuscript.

      The weaknesses are:

      (1) Most of the analysis is undertaken with cell lines. In fact, all of the analysis involving the assessment of specific proteins associated with amphiectosomes and ILVs are performed in vitro, so it is unclear whether these processes are really mirrored in vivo. The images shown in vivo only demonstrate putative amphiectosomes in the circulation, which is perhaps surprising if they normally have a short half-life and would need to pass through an endothelium to reach the vessel lumen unless they were secreted by the endothelial cells themselves.

      (2) The analysis of the intracellular formation of compartments involved in the secretion process (Figure 2_S5) relies on immuno-EM, which is generally less convincing than high-/super-resolution fluorescence microscopy because the immuno-labelling is inevitably very sporadic and patchy. High-quality EM is challenging for many labs (and seems to be done very well here), but high-/super-resolution fluorescence microscopy techniques are more commonly employed, and the study already shows that these techniques should be applicable to studying the intracellular trafficking processes.

      (3) One aspect of the mechanism, which needs some consideration, is what happens to the amphisome membrane, once it has budded off inside the amphiectosome. In the fluorescence images, it seems to be disrupted, but presumably, this must happen after separation from the cell to avoid the release of ILVs inside the cell. There is an additional part of Figure 1 (Figure 1Y onwards), which does not seem to be discussed in the text (and should be), that alludes to amphiectosomes often having a double membrane.

      (4) The real-time analysis of the amphiectosome tearing mechanism seemed relatively slow to me (over three minutes), and if this has been observed multiple times, it would be helpful to know if this is typical or whether there is considerable variation.

      Overall, I think the authors have been successful in identifying amphiectosomes secreted from multiple cell lines and demonstrating that the ILVs inside them have at least two origins (autophagosome membrane and late endosomal multivesicular body) based on the markers that they carry. The analysis of intracellular compartments producing these structures is rather less convincing and it remains unclear what cells release these structures in vivo.

      I think there could be a significant impact on the EV field and consequently on our understanding of cell-cell signalling based on these findings. It will flag the importance of investigating the release of amphiectosomes in other studies, and although the authors do not discuss it, the molecular mechanisms involved in this type of 'ectosomal-style' release will be different from multivesicular compartment fusion to the plasma membrane and should be possible to be manipulated independently. Any experiments that demonstrate this would greatly strengthen the manuscript.

      In general, the EV field has struggled to link up analysis of the subcellular biology of sEV secretion and the biochemical/physical analysis of the sEVs themselves, so from that perspective, the manuscript provides a novel angle on this problem.

    1. Reviewer #2 (Public Review):

      Summary:

      Overall, this study provides a thorough description of the formation of syncytia following wounding of the proliferation-competent diploid epithelium of the pupal notum. While this phenomenon has already been described briefly for this particular tissue by the Galko lab in Wang et al 2015, the authors provide a much more detailed description and characterisation of the process providing some novel insights (radial versus tangential border breakdown, cell shrinkage, timings, syncytia outcompeting mononucleated cells, etc.).

      Strengths:

      This paper provides an elegant, thorough, descriptive characterisation of syncytia-driven wound closure using state-of-the-art confocal live imaging of the pupal notum. The authors show that laser-induced wounding of this diploid, proliferation-competent epithelium results in the formation of syncytia of various sizes in the first few cell rows around the wound edge, which progressively become bigger as healing proceeds. This results in ~50% of cells becoming part of these syncytia. The cell fusion events were convincingly demonstrated by showing the disappearance of p120ctnRFP and E-Cadherin-GFP from cell-cell borders as well as cytoplasmic GFP mixing of GFP-positive cells with a GFP-negative cell.

      Apart from cell-cell fusion by border breakdown that mostly happens in the first 2h following wounding, the authors also found that at later stages of wound healing cell shrinkage following cytoplasmic mixing contributed to sycytia formation.

      Next, the authors provided some convincing evidence that syncytia outcompete mononuclear cells for being positioned in the first cell row around the wound.

      The authors then show that radial border breakdown occurs much less frequently than tangential border breakdown. They suggest that radial border breakdown reduces the requirement for cell-cell intercalations. They also hypothesise that tangential border breakdown might allow fused cells to share resources and provide more resources to be used near the wound edge, e.g. for actomyosin cable formation. To test this, the authors generate single-cell clones that overexpress Actin-GFP. They then show convincingly how a single Actin-GFP-positive cell in the second cell row fuses with one GFP-negative cell in the first cell row. The Actin-GFP signal then spreads in the fused cell and labels some previously unlabelled actin-rich structure near the wound edge which most likely is the actomyosin cable. This provides some evidence for resource sharing by cytoplasmic mixing following fusion.

      Weaknesses:

      The authors provide some convincing evidence that syncytia outcompete mononuclear cells for being positioned in the first cell row around the wound. The authors suggest that the syncytial cells might be better able to close the wound. However, some genetic studies would need to be done to establish this more convincingly. E.g. Could the authors genetically block syncytia formation and then show that these wounds now heal slower?

      The authors suggest that radial border breakdown reduces the requirement for cell intercalation. While this might be true it also raises the question of how the various syncytia facing the wound border change shape to allow the shrinkage of the first cell row over time to allow wound closure. None of the four movies included in the study shows the whole wound healing process until the later stages, making it hard to assess this. It would be good to include one such movie showing the syncytia in the whole wound and comment on this point.

      The authors hypothesise that tangential border breakdown might allow fused cells to share resources and provide more resources to be used near the wound edge, e.g. for actomyosin cable formation. They show convincingly through the fusion of a single Actin-GFP-positive cell in the second cell row with a GFP-negative cell in the first cell row that Actin-GFP spreads in the fused cell and labels the previously unlabelled actomyosin cable. While the hypothesis of resource sharing to improve healing is intriguing and makes sense, this experiment doesn't necessarily prove the benefit of resource sharing. It does show cytoplasmic mixing following fusion, now allowing the GFP-labelled actin to diffuse and be incorporated into the actomyosin cable. In a wild-type condition, fusion would not increase the total concentration of resources, although it would increase the total amount of resources within this bigger fused cell. The question is whether resource sharing without increasing the protein concentration is beneficial and increases the efficiency of certain wound healing mechanisms. There might be a benefit of cell fusion, if for example certain resources were only present in limited amounts or if protein transport could increase the concentration locally. To provide better evidence for the hypothesis that resource sharing improves wound healing, maybe the authors could look at the actomyosin cable in a wounded epithelium (such as in Figure 4E, F), in which all cells express MyoII-GFP. The authors could compare the average intensity of the actomyosin cable at the wound edge in mononucleated cells versus in syncytia. If resource sharing is indeed beneficial, it might be that the actomyosin cable is stronger/brighter in syncytia or it forms quicker.

      The biggest limitation of this study is that the authors don't address how the formation of these syncytia is regulated. While the manuscript in its current form provides some valuable new insights into syncytial-driven wound closure, it would be much more informative if it also provided some mechanistic details. The authors could test if some of the mechanisms shown to regulate syncytial formation in other types of syncytia-driven wound healing are also involved here. E.g. Yorkie was shown to negatively regulate cell fusion in adult syncytial-driven wound closure (Losick et al 2013). The authors could test for the effect of Yorkie-RNAi in the epithelium on wound closure and syncytia formation. Expression of the dominant negative RacN17 also blocked cell fusion in adult syncytial-driven wound closure (Losick et al 2013).

      Moreover, JNK activation was shown to be needed in larval syncytial-driven wound closure (Galko and Krasnow 2004). The authors could test JNK pathway reporters to assess pathway activation or test if the JNK pathway is needed for syncytial-driven wound closure by expressing a dominant-negative form of Basket JNK in the epithelium.

      Or could syncytia formation be regulated by changes in Integrin-mediated adhesion as shown by the Galko lab in Wang et al 2015? They show that wounding provoked a striking relocalization of PINCH and ILK, indicating the disassembly of functional FA complexes concomitant with syncytium formation. Maybe the authors could investigate some of these.

      Another general question that the authors raise but don't address enough is whether syncytia-driven wound closure in proliferation-competent epithelia is any different from the one in post-mitotic, polyploid epithelia. Since the mechanism regulating the former is not known, this remains unclear.

      Finally, it is not clear, whether syncytia in these proliferation-competent epithelia get resolved after wound healing. Do they get removed and replaced by mononucleated proliferation-competent cells or do the syncytia stay in the epithelium like a scar? The authors should provide some images of wound areas a few hours after wound closure is complete and comment on this.

      Minor points:

      Figure 3: It would be better to have the microcopy images alongside the quantifications.

      Figure 4A: The syncytium at the wound edge here doesn't look straight but wavy. Does it not form an actomyosin cable that straightens the front? Or are there lamellipodia/filopodia?

      248: The authors suggest an interesting hypothesis that mitochondria or ER could be pooled in fused cells. It would be nice to see some evidence: e.g. by labeling mitochondria and assessing where they are in syncytia versus mononucleated cells and whether they are concentrated around the wound edge.

      141-145 (Figure 4B and C) This example is not completely convincing. First, it is hard to see where the wound edge is. Second, it would be good to include an even later time point when the cell is clearly no longer at the wound edge.

    1. Reviewer #2 (Public Review):

      The authors investigated the role of inflammatory molecules in diastolic dysfunction and screened antiviral and cardioprotective pharmacological agents for their potential to reverse inflammation-mediated diastolic dysfunction. This study focuses on heart failure with preserved ejection fraction (HFpEF) in people living with HIV (PLWH), a condition often challenging to study due to the lack of suitable animal models. Using human-induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs), researchers simulated HFpEF in vitro. They observed that inflammatory cytokines impaired cardiomyocyte relaxation, mimicking HFpEF, while SGLT2 inhibitors and mitochondrial antioxidants reversed this effect. Exposure to serum from HIV patients did not induce dysfunction in hiPSC-CMs. These findings suggest hiPSC-CMs as a promising model for understanding HFpEF mechanisms and testing potential treatments.

      Comments to improve the study:

      The manuscript is well-written, and the results are well-illustrated. However, there are some topics that are not well-connected, and the rationale and hypothesis are not clearly defined beforehand, such as mitochondrial membrane potential, mitochondrial ROS, and angiogenic potential.

      As the hiPSC cardiomyocytes are treated with various reagents to measure diastolic dysfunction, it is important to confirm whether the treatment time and dose used were sufficient to exert a functional effect. Dose and time-dependent experiments are essential, or at least sufficient citations should be provided for selecting the dose for IFN and TNF.

      After IFN and TNF treatment, determining the expression levels of molecular markers of DD/HFpEF is crucial. Again, if sufficient evidence is available, it can be cited.

      The Methods section describes TMRE colocalization and immunofluorescence, but no images are provided.

      The concentration of TNF and IFN in patients is critical, which was acknowledged and discussed as a limitation of the study by the authors. Authors should consider this aspect, and if not feasible, clinical reports should be cited to provide a rough estimation of their concentration.

    1. Reviewer #2 (Public Review):

      Summary:

      Sterols, including desmosterol and cholesterol, play critical roles in male fertility including membrane rearrangements associated with sperm capacitation, steroidogenesis, and germ cell development. Relovska, Sona, et al. investigated the effects of global overexpression of classic cholesterol biosynthesis enzyme DHCR24 in a mouse model, focusing on the impacts on sperm function and male fertility. While mice were viable and did not exhibit altered plasma cholesterol levels or obesity, the authors demonstrated that concentrations of relevant sterols in sperm from transgenic mice were altered compared to WT mouse sperm, including the expected depletion of desmosterol. The transgenic males exhibited several indicators of reduced sperm function and fertility. Mitochondrial dysfunction was indicated by a noted depletion of localization in the distal middle-piece of up to approximately 20-25% of transgenic sperm flagella, and alterations in mitochondrial membrane potential and oxygen consumption rates in transgenic sperm were noted.

      Strengths:

      The authors demonstrate that DHCR24 overexpression was achieved and that sperm sterol levels are altered. The conclusions that global DHCR24 overexpression impacts mitochondrial localization and male fertility parameters are supported by the number of different supporting assessments utilized to reach these conclusions and this is a strength. Overall, the authors achieve their aim of demonstrating DHCR24 overexpression impacts on indicators of sperm function and fertility including reduced sperm counts and sperm motility, reduced fertility in mating trials with aged males, and reduced IVF success when sperm were capacitated in conditions of higher sperm concentrations in vitro. The authors further investigate sperm mitochondrial localization and function. While a mitochondrial sheath can form in sperm from transgenic mice, 25% of the sperm exhibit a shortened mitochondrial sheath where a distal portion of the middle piece of the sperm flagella lacks mitochondria and instead exhibits exposed outer dense fibers.

      Weaknesses:

      In the current study, the authors conclude that desmosterol may not act as an LXR activator in testicular cells based on assessment of relevant mRNA levels in whole testis that indicated the relevant transcripts were not altered in transgenic testes. However, caution should be taken in utilizing whole testis transcriptomics to rule out a role in specific cell populations within the testis with minor relative representation, such as macrophages or undifferentiated spermatogonia. This is an important distinction for a few reasons. The authors reveal through single-cell assessments of DHCR24 expression in WT testis that it is most highly expressed in undifferentiated spermatogonia. Further, the authors previously reported that DHCR24 over-expression in myeloid/macrophage populations did impact LXR activation impacting atherosclerosis. Taken together with emerging evidence that testis macrophages may impact spermatogonial fate decisions, the potential for DHCR24 to impact these minor testicular cell populations should not yet be ruled out. The significance of individual observations needs to be clarified through improved reporting of methodologies, specific biological and technical replicates, and statistical significance for each individual assessment. The lack of these details obfuscates the ability of the reader to interpret or replicate several reported observations which is a weakness.

      (1) The fertility trials indicate a reduced number of pups/litter in aged but not younger transgenic males. However, the data for the aged males includes three data points of 0 pups, which brings to question if the data points each represent the average pups/litter for individual males or individual litters with multiple litters separately included for fertile males. Clarification could help in interpreting whether litter sizes were reduced, or if litter frequency and/or fertility of individual males was reduced. In the latter case, behavioral infertility would not be excluded from consideration.

      (2) The statistical significance is not clear for altered acrosome reaction data, hyperactivated motility data, waveform analysis, mitochondrial membrane potential, and some of the sperm morphology assessments. In many assessments, the biological and technical replicates assessed need to be clarified.

      (3) Methods utilized for image assessment of waveform analysis and mitochondrial membrane potential are lacking detail sufficient for replication of the assessments or for reader interpretation of how conclusions were reached.

      Summary of impact:

      Overall, the novel observations in this study are consistent with a role for controlled sterol concentrations being important for male fertility and indicate that this model will be useful to further investigate sterol biosynthesis contributions to testis function including steroidogenesis, spermatogenesis, and sperm function including capacitation.

    1. Reviewer #2 (Public Review):

      Summary:

      This manuscript uses cell lines representative of germ line cells, somatic cells, and pluripotent cells to address the question of how the endocrine-disrupting compound BPS affects these various cells with respect to gene expression and DNA methylation. They find a relationship between the presence of estrogen receptor gene expression and the number of DNA methylation and gene expression changes. Notably, PGCLCs do not express estrogen receptors and although they do have fewer changes, changes are nevertheless detected, suggesting a nonconical pathway for BPS-induced perturbations. Additionally, there was a significant increase in the occurrence of BPS-induced epimutations near EREs in somatic and pluripotent cell types compared to germ cells. Epimutations in the somatic and pluripotent cell types were predominantly in enhancer regions whereas that in the germ cell type was predominantly in gene promoters.

      Strengths:

      The strengths of the paper include the use of various cell types to address the sensitivity of the lineages to BPS as well as the observed relationship between the presence of estrogen receptors and changes in gene expression and DNA methylation.

      Weaknesses:

      The weaknesses include the lack of reporting of replicates, superficial bioinformatic analysis, and the fact that exposures are more complicated in a whole organism than in an isolated cell line.

    1. Reviewer #3 (Public Review):

      Summary:

      In this manuscript, the authors conducted a comprehensive study of the X-linked miR-506 family miRNAs in mice on its origin, evolution, expression, and function. They demonstrate that the X-linked miR-506 family, predominantly expressed in the testis, may be derived from MER91C DNA transposons and further expanded by retrotransposition. By genetic deletion of different combinations of 5 major clusters of this miRNA family in mice, they found these miRNAs are not required for spermatogenesis. However, by further examination, the mutant mice show mild fertility problem and inferior sperm competitiveness. The authors conclude that the X-linked miR-506 miRNAs finetune spermatogenesis to enhance sperm competition.

      Strengths:

      This is a comprehensive study with extensive computational and genetic dissection of the X-linked miR-506 family providing a holistic view of its evolution and function in mice. The finding that this family miRNAs could enhance sperm competition is interesting and could explain their roles in finetuning germ cell gene expression to regulate reproductive fitness.

      Comments on revised version:

      The authors have addressed the concerns raised.

    1. Reviewer #2 (Public Review):

      How organism physiological state modulates establishment and perdurance of memories is a timely question that the authors aimed at addressing by studying the interplay between energy homeostasis and food-related conditioning in Drosophila. Specifically, they studied how starvation modulates the establishment of short-term vs long-term memories and clarified the role of the monoamine Octopamine in food-related conditioning, showing that it is not per se involved in formation of appetitive short-term memories but rather gates memory formation by suppressing LTM when energy levels are high. This work clarifies previously described phenotypes and provides insight about interconnections between energy levels, feeding and formation of short-term and long-term food-related memories.

      Strengths<br /> - Previous studies have documented the impact of Octopamine on different aspects of food-related behaviors (regulation of energy homeostasis, feeding, sugar sensing, appetitive memory...), but we currently lack a clear understanding of how these different functions are interconnected. The authors have used a variety of experimental approaches to systematically test the impact of internal energy levels in establishment of different forms of appetitive memory and the role of Octopamine in this process.

      - The authors have used a range of approaches, performed carefully controlled experiments and produced high quality data.

    1. Reviewer #2 (Public Review):

      Summary:

      In this manuscript, Mahapatra and Takahashi report on the physiological consequences of pharmacologically blocking either clathrin and dynamin function during compensatory endocytosis or of the cortical actin scaffold both in the calyx of Held synapse and hippocampal boutons in acute slice preparations

      Strengths:

      Although many aspects of these pharmacological interventions have been studied in detail during the past decades, this is a nice comprehensive and comparative study, which reveals some interesting differences between a fast synapse (Calyx of Held) tuned to reliably transmit at several 100 Hz and a more slow hippocampal CA1 synapse. In particular the authors find that acute disturbance of the synaptic actin network leads to a marked frequency-dependent enhancement of synaptic depression in the Calyx, but not in the hippocampal synapse This striking difference between both preparations is the most interesting and novel finding.

      Weaknesses:

      Unfortunately, however, these findings concerning the different consequences of actin depolymerization are not sufficiently discussed in comparison to the literature. My only criticism concerns the interpretation of the ML 141 and Lat B data. With respect to the Calyx data, I am missing a detailed discussion of the effects observed here in light of the different RRP subpools SRP and FRP. This is very important since Lee at al. (2012, PNAS 109 (13) E765-E774) showed earlier that disruption of actin inhibits the rapid transition of SRP SVs to the FRP at the AZ. The whole literature on this important concept is missing. Likewise, the role of actin for the replacement pool at a cerebellar synapse (Miki et al., 2016) is only mentioned in half a sentence. There is quite some evidence that actin is important both at the AZ (SRP to FRP transition, activation of replacement pool) and at the peri-active zone for compensatory endocytosis and release site clearance. Both possible underlying mechanisms (SRP to FRP transition or release site clearance) should be better dissected.

    1. Reviewer #3 (Public Review):

      Summary:

      This study implements an innovative neurofeedback procedure in rats, providing food reward upon detection of a sharp wave-ripple event (SWR) in the hippocampus. The elegant experimental design enables a within-animal comparison of the effects of this neurofeedback procedure as compared to a control condition in which equivalent reward is provided in a non-contingent manner. The neurofeedback procedure was found to increase SWR rate, followed by a compensatory reduction in SWR rate. These changes in SWR rate were not accompanied by any changes in memory performance on the memory-guided task.

      Strengths:

      The scientific premise for the study is outstanding. It addresses an issue of high importance, of developing ways to not merely describe correlations between SWRs (and their content) and memory performance, but to manipulate them. The authors argue clearly and convincingly that even studies that have performed causal manipulations of SWRs have important confounds and limitations, and most importantly for translational purposes, they are all invasive. So, the idea of developing a potentially non-invasive neurofeedback procedure for modulating SWRs is compelling both as an innovative new experimental manipulation in studies of SWRs, and as a potentially impactful therapeutic avenue.

      In addition to addressing an important issue with an innovative approach, the study has many other strengths. The data unambiguously show that the method is effective at increasing SWR rate in each individual subject. The experimental design allows within-subject comparison of neurofeedback and control trials, where the subjects wait an equivalent amount of time. The careful analyses of SWR properties and their content establish that neurofeedback SWRs are comparable to control SWRs. The data add further evidence to the notion that SWR rate is subject to homeostatic control. The paper is also exceptionally well written, and was a pleasure to read. So, there is a clear technical advance, in that there is now a method for increasing SWR rate non-invasively, which is rigorously established and characterized.

      Weaknesses:

      The one overall limitation I find with this study is that it is unclear to what extent the same (or better) results could have been obtained using behavior-feedback instead of neuro-feedback. Because SWR rates are generally higher during states of quiescence compared to active movement or task engagement, it is possible that reinforcing behaviorally detected quiescent states (e.g. low movement) would indirectly increase SWR rates. The authors include an important control analysis showing higher SWR rates in the neurofeedback condition even when movement speed is controlled for by subsetting the data, demonstrating that changes in movement speed cannot be the only explanation of the results. At the same time, the observation that all 4 subjects had lower movement speeds during neurofeedback compared to control trials suggests that neurofeedback is likely reinforcing both overt (behavior) and covert (SWR) processes. Understanding the relative contributions of each to the observed SWR increase would help clarify whether the neurofeedback approach is worth the additional effort and expense compared to behavioral feedback.

    1. Reviewer #2 (Public Review):

      This MEG study used co-registered eye-tracking and Rapid Invisible Frequency Tagging (RIFT) to track the effects of semantic parafoveal preview during natural sentence reading. Unpredictable target words could either be congruent or incongruent with sentence context. This modulated the RIFT response already while participants were fixating the preceding word. This indicates that the semantic congruency of the upcoming word modulates visual attention demands already in parfoveal preview.<br /> The quest for semantic parafoveal preview in natural reading has attracted a lot of attention in recent years, especially with the development of co-registered eye-tracking and EEG/MEG. Evidence from dynamic neuroimaging methods using innovative paradigms as in this study is important for this debate.

      Major points:

      (1) The authors frame their study in terms of "congruency with sentence context". However, it is the congruency between adjective-noun pairs that determines congruency (e.g. "blue brother" vs "blue jacket", and examples p. 16 and appendix). This is confirmed by Suppl Figure 1, which shows a significantly larger likelihood of refixations to the pre-target word for incongruent sentences, probably because the pre-target word is most diagnostic for the congruency of the target word. The authors discuss some possibilities why there is variability in parafoveal preview effects in the literature. It is more likely to see effects for this simple and local congruency, rather than congruency that requires and integration and comprehension of the full sentence. Future studies should investigate whether the observed effects depend on sentence context or local congruency.

      (2) The authors used MEG and provided a source estimate for the tagging response (Figure 2), which unsurprisingly is in visual cortex. The most important results are presented at the sensor level. This does not add information about the brain sources of the congruency affect, as the RIFT response probably reflects top-down effects on visual attention etc. The RIFT response can test for preview effects on visual brain responses but does not allow the localisation of context processing effects that cause them.

      (3) The earliest semantic preview effects occurred around 100ms after fixating the pre-target word (discussed around l. 323). This means that at this stage the brain must have processed the pre-target and the target word and integrated their meanings (at some level). Even in the single-word literature, semantic effects at 100 ms are provocatively early. Future studies should aim at reconciling these different findings.

      (4) As in previous EEG/MEG studies, the authors found a neural but no behavioural preview effect. As before, this raises the question whether the observed effect is really "critical" for sentence comprehension. If interpreted in terms of "information" and "attention", then one would expect a positive effect on behaviour, either reading speed or accuracy. The authors provide a correlation analysis with reading speed, but this does not allow causal conclusions: Some people may simply read slowly and therefore pay more attention and get a larger preview response. Some readers may hurry and therefore not pay attention and not get a preview response. In order to address this, one would have to control for reading speed and show an effect of RIFT response on comprehension performance (or vice versa, with a task that is not close to ceiling performance).

    1. Reviewer #3 (Public Review):

      Summary:

      Here the authors show global synchronization of cerebral blood flow (CBF) induced by oscillating visual stimuli in the mouse brain. The study validates the use of endogenous autofluorescence to quantify the vessel "shadow" to assess the magnitude of frequency-locked cerebral blood flow changes. This approach enables straightforward estimation of artery diameter fluctuations in wild-type mice, employing either low magnification wide-field microscopy or deep-brain fibre photometry. For the visual stimuli, awake mice were exposed to vertically oscillating stripes at a low temporal frequency (0.25 Hz), resulting in oscillatory changes in artery diameter synchronized to the visual stimulation frequency. This phenomenon occurred not only in the primary visual cortex but also across a broad cortical and cerebellar surface. The induced CBF changes adapted to various stimulation parameters, and interestingly, repeated trials led to plastic entrainment. The authors control for different artefacts that may have confounded the measurements such as light contamination and eye movements but found no influence of these variables. The study also tested horizontally oscillating visual stimuli, which induce the horizontal optokinetic response (HOKR). The amplitude of eye movement, known to increase with repeated training sessions, showed a strong correlation with CBF entrainment magnitude in the cerebellar flocculus. The authors suggest that parallel plasticity in CBF and neuronal circuits is occurring. Overall, the study proposes that entrained "vasomotion" contributes to meeting the increased energy demand associated with coordinated neuronal activity and subsequent neuronal circuit reorganization.

      Strengths:

      -The paper describes a simple and useful method for tracking vasomotion in awake mice through an intact skull.<br /> -The work controls for artefacts in their primary measurements.<br /> -There are some interesting observations, including the nearly brain-wide synchronization of cerebral blood flow oscillations to visual stimuli and that this process only occurs after mice are trained in a visual task.<br /> -This topic is interesting to many in the CBF, functional imaging, and dementia fields.

    1. Reviewer #2 (Public Review):

      Summary:

      This is a paper about the segmentation of visual stimuli based on speed cues. The experimental stimuli are random dot fields in which each dot moves at one of two velocities. By varying the difference between the two speeds, as well as the mean of the two speeds, the authors estimate the capacity of observers (human and non-human primates) to segment overlapping motion stimuli. Consistent with previous work, perceptual segmentation ability depends on the mean of the two speeds. Recordings from area MT in monkeys show that the neuronal population to compound stimuli often shows a bias towards the faster-speed stimuli. This bias can be accounted for with a computational model that modulates single-neuron firing rates by the speed preferences of the population. The authors also test the capacity of a linear classifier to produce the psychophysical results from the MT data.

      Strengths:

      Overall, this is a thorough treatment of the question of visual segmentation with speed cues. Previous work has mostly focused on other kinds of cues (direction, disparity, color), so the neurophysiological results are novel. The connection between MT activity and perceptual segmentation is potentially interesting, particularly as it relates to existing hypotheses about population coding.

      Weaknesses:

      Page 10: The relationship between (R-Rs) and (Rf-Rs) is described as "remarkably linear". I don't actually find this surprising, as the same term (Rs) appears on both the x- and y-axes. The R^2 values are a bit misleading for this reason.

      Figure 9: I'm confused about the linear classifier section of the paper. The idea makes sense - the goal is to relate the neuronal recordings to the psychophysical data. However the results generally provide a poor quantitative match to the psychophysical data. There is mention of a "different paper" (page 26) involving a separate decoding study, as well as a preprint by Huang et al. (2023) that has better decoding results. But the Huang et al. preprint appears to be identical to the current manuscript, in that neither has a Figure 12, 13, or 14. The text also says (page 26) that the current paper is not really a decoding study, but the linear classifier (Figure 9F) is a decoder, as noted on page 10. It sounds like something got mixed up in the production of two or more papers from the same dataset. In any case, I think that some kind of decoding analysis would really strengthen the current paper by linking the physiology to the psychophysics, but given the limitations of the linear classifier, a more sophisticated approach might be necessary -- see for example Zemel, Dayan, and Pouget, 1998. The authors might also want to check out closely related work by Treue et al. (Nature Neuroscience 2000) and Watamaniuk and Duchon (1992).

      What do we learn from the normalization model? Its formulation is mostly a restatement of the results - that the faster and slower speeds differentially affect the combined response. This hypothesis is stated quantitatively in equation 8, which seems to provide a perfectly adequate account of the data. The normalization model in equation 10 is effectively the same hypothesis, with the mean population response interposed - it's not clear how much the actual tuning curve in Figure 10A even matters, since the main effect of the model is to flatten it out by averaging the functions in Figure 10B. Although the fit to the data is reasonable, the model uses 4 parameters to fit 5 data points and is likely underconstrained; the parameters other than alpha should at least be reported, as it would seem that sigma is actually the most important one. And I think it would help to examine how robust the statistical results are to different assumptions about the normalization pool.

    1. Reviewer #2 (Public Review):

      Summary:

      The study investigates the representation of irrelevant stimuli in neural circuits using neural recordings from the primate prefrontal cortex during a passive object association task. They find a significant decrease in the linear decodability of irrelevant stimuli over the course of learning (in the time window in which the stimuli are irrelevant). They then compare these trends to RNNs trained with varying levels of noise and firing rate regularization and find agreement when these levels are at an intermediate value. In a complementary analysis, they found (in both RNNs and PFC) that the magnitude of relevant and irrelevant stimuli increased and decreased, respectively, during learning. These findings were interpreted in terms of a minimization of metabolic cost in the cortex.

      To understand how stimuli can be dynamically suppressed at times when they are irrelevant, the authors constructed and analyzed a reduced two-neuron model of the task. They found a mechanism in which firing rate regularization increased the probability of negative weights in the input, pushing the neural activities below the threshold. A similar mechanism was observed in RNNs.

      Strengths:

      The article is well-written and the figures are easily understood. The analyses are well explained and motivated. The article provides a valuable analysis of the effect of two parameters on representations of irrelevant stimuli in trained RNNs.

      Weaknesses:

      (1) The mechanism for suppressing dynamically relevant stimuli appears to be incomplete and does not explain clearly enough how representations of 'color' which are suppressed through negative input weights become un-suppressed in the presence of the second variable 'shape'.

      (2) Interpretation of results in terms of the effect of metabolic cost on cortical dynamics is not backed up by the presented data/analyses. The change in dynamics of 'color' representations in the prefrontal cortex only qualitatively matches RNN dynamics and may arise from other causes.

    1. Reviewer #2 (Public Review):

      Summary:

      The manuscript by Hike et al. entitled 'High-resolution awake mouse fMRI at 14 Tesla' describes the implementation of awake mouse BOLD-fMRI at high field. This work is timely as the field of mouse fMRI is working toward collecting high-quality data from awake animals. Imaging awake subjects offers opportunities to study brain function that are otherwise not possible under the more common anesthetized conditions. Not to mention the confounding effects that anesthesia has on neurovascular coupling. What has made progress in this area slow (relative to other imaging approaches like optical imaging) is the environment within the MRI scanner (high acoustic noise) - as well as the intolerance of head and body motion. This work adds to a relatively small, but quickly growing literature on awake mouse fMRI. The findings in the study include testing of an implanted head-coil (for MRI data reception). Two designs are described and the SNR of these units at 9.4T and 14T are reported. Further, responses to visual as well as whisker stimulation recorded in acclimated awake mice are shown. The most interesting finding, and most novel, is the observation that mice seem to learn to anticipate the presentation of the stimulus - as demonstrated by activations evident ~6 seconds prior to the presentation of the stimulus when stimuli are delivered at regular intervals (but not when stimuli are presented at random intervals). These kinds of studies are very challenging to do. The surgical preparation and length of time invested into training animals are grueling. I also see this work as a step in the right direction and evidence of the foundations for lots of interesting future work. However, I also found a few shortcomings listed below.

      Weaknesses:

      (1) The surface coil, although offering a great SNR boost at the surface, ultimately comes at a cost of lower SNR in deeper more removed brain regions in comparison to commercially available Bruker coils (at room temperature). This should be quantified. A rough comparison in SNR is drawn between the implanted coils and the Bruker Cryoprobe - this should be a quantitative comparison (if possible) - including any differences in SNR in deeper brain structures. There are drawbacks to the Cryoprobe, which can be discussed, but a more thorough comparison between the implanted coils, and other existing options should be provided (the Cryoprobe has been used previously in awake mouse experiments). Further, the details of how to build the implanted coils should be provided (shared) - this should include a parts list as well as detailed instructions on how to build the units. Also, how expensive are they? And can they be reused?

      (2) In the introduction, the authors state that "Awake mouse fMRI has been well investigated". I disagree with this statement and others in the manuscript that give the reader the impression that awake experiments are not a challenging and unresolved approach to fMRI experiments in mice (or rodents). Although there are multiple labs (maybe 15 worldwide) that have conducted awake mouse experiments (with varying degrees of success/thoroughness), we are far from a standardized approach. This is a strength of the current work and should be highlighted as such. I encourage the authors to read the recent systematic review that was published on this topic in Cerebral Cortex by Mandino et al. There are several elements in there that should influence the tone of this piece including awake mouse implementations with the Bruker Cryoprobe, prevalence of surgical preparations, and evaluations of stress.

      (3) The authors also comment on implanted coils reducing animal stress - I don't know where this comment is coming from, as this has not been reported in the literature (to my knowledge) and the authors don't appear to have evaluated stress in their mice.

      (4) Following on the above point, measures of motion, stress, and more details on the acclimation procedure that was implemented in this study should be included.

      (5) It wasn't clear to me at what times the loop versus "Figure 8" coil was being used, nor how many mice (or how much data) were included in each experiment/plot. There is also no mention of biological sex.

      (6) Building on the points above, the manuscript overall lacks experimental detail (especially since the format has the results prior to the methods).

      (7) An observation is made in the manuscript that there is an appreciable amount of negative BOLD signal. The authors speculate that this may come from astrocyte-mediated BOLD during brain state changes (and cite anesthetized rat and non-human primate experiments). This is very strange to me. First, the negative BOLD signal is not plotted (please do this), further, there are studies in awake mice that measure astrocyte activation eliciting positive BOLD responses (see Takata et al. in Glia, 2017).

    1. Reviewer #2 (Public Review):

      Weng et al. perform a comprehensive study of gene expression changes in young and old animals, in wild-type and daf-2 insulin receptor mutants, in the whole animal, and specifically in the nervous system. Using this data, they identify gene families that are correlated with neuronal ageing, as well as a distinct set of genes that are upregulated in neurons of aged daf-2 mutants. This is particularly interesting as daf-2 mutants show both extended lifespans and healthier neurons in aged animals, reflected by better learning/memory in older animals compared with wild-type controls. Indeed, the knockdown of several of these upregulated genes resulted in poorer learning and memory. In addition, the authors showed that several genes upregulated during ageing in wild-type neurons also contribute to learning and memory; specifically knockdown of these genes in young animals resulted in improved memory. This indicates that (at least in this small number of cases), genes that show increased transcript levels with age in the nervous system somehow suppress memory, potentially by having damaging effects on neuronal health.

      Finally, from a resource perspective, the neuronal transcriptome provided here will be very useful for C. elegans researchers as it adds to other existing datasets by providing the transcriptome of older animals (animals at day 8 of adulthood) and demonstrating the benefits of performing tissue-specific RNAseq instead of whole-animal sequencing.

      The work presented here is of high quality and the authors present convincing evidence supporting their conclusions. I only have a few comments/suggestions:

      (1) Do the genes identified to decrease learning/memory capacity in daf-2 animals (Figure 4d/e) also impact neuronal health? daf-2 mutant worms show delayed onset of age-related changes to neuron structure (Tank et al., 2011, J Neurosci). Does knockdown of the genes shown to affect learning also affect neuron structure during ageing, potentially one mechanism through which they modulate learning/memory?

      (2) The learning and memory assay data presented in this study uses the butanone olfactory learning paradigm, which is well established by the same group. Have the authors tried other learning assays when testing for learning/memory changes after the knockdown of candidate genes? Depending on the expression pattern of these genes, they may have more or less of an effect on olfactory learning versus for example gustatory or mechanosensory-based learning.

      (3) I have a comment on the 'compensatory vs dysregulatory' model as stated by the authors on page 7. I understand that this model presents the two main options, but perhaps this is slightly too simplistic: the gene expression that rises during ageing may be detrimental for memory (= dysregulatory), but at the same time may also be beneficial for other physiological roles in other tissues (=compensatory).

    1. Reviewer #2 (Public Review):

      The manuscript describes a new framework for thinking about the place and grid cell system in the hippocampus and entorhinal cortex in which these cells are fundamentally involved in supporting non-spatial information coding. If this framework were shown to be correct, it could have high impact because it would suggest a completely new way of thinking about the mammalian memory system in which this system is non-spatial. Although this idea is intriguing and thought-provoking, a very significant caveat is that the paper does not provide evidence that specifically supports its framework and rules out the alternate interpretations. Thus, although the work provides interesting new ideas, it leaves the reader with more questions than answers because it does not rule out any earlier ideas.

      Basically, the strongest claim in the paper, that grid cells are inherently non-spatial, cannot be specifically evaluated versus existing frameworks on the basis of the evidence that is shown here. If, for example, the author had provided behavioral experiments showing that human memory encoding/retrieval performance shifts in relation to the predictions of the model following changes in the environment, it would have been potentially exciting because it could potentially support the author's reconceptualization of this system. But in its current form, the paper merely shows that a new type of model is capable of explaining the existing findings. There is not adequate data or results to show that the new model is a significantly better fit to the data compared to earlier models, which limits the impact of the work. In fact, there are some key data points in which the earlier models seem to better fit the data.

      Overall, I would be more convinced that the findings from the paper are impactful if the author showed specific animal memory behavioral results that were only supported by their memory model but not by a purely spatial model. Perhaps the author could run new experiments to show that there are specific patterns of human or animal behavior that are only explained by their memory model and not by earlier models. But in its current form, I cannot rule out the existing frameworks and I believe some of the claims in this regard are overstated.

      In addition to the broader concerns noted above regarding the absence of any specific behavioral data that are explained by their model and not by existing spatial models, I am additionally concerned that this manuscript does not explain a number of important key empirical results in the rodent grid cell literature.

      * The paper does not fully take into account all the findings regarding grid cells, some of which very clearly show spatial processing in this system. For example, findings on grid-by-direction cells (e.g., Sargolini et al. 2006) would seem to suggest that the entorhinal grid system is very specifically spatial and related to path integration. Why would grid-by-direction cells be present and intertwined with grid cells in the author's memory-related reconceptualization? It seems to me that the existence of grid-by-direction cells is strong evidence that at least part of this network is specifically spatial.

      * I am also concerned that the paper does not do enough to address findings regarding how the elliptical shape of grid fields shifts when boundaries of an environment compress in one direction or change shape/angles (Lever et al., & Krupic et al). Those studies show compression in grid fields based on boundary position, and I don't see how the authors' model would explain these findings.

      * Are findings regarding speed modulation of grid cells problematic for the paper's memory results?

      * A further issue is that the paper does not seem to adequately address developmental findings related to the timecourses of the emergence of different cell types. In their simulation, researchers demonstrate the immediate emergence of grid fields in a novel environment, while noting that the stabilization of place cell positions takes time. However, these simulation findings contradict previous empirical developmental studies (Langston et al., 2010). Those studies showed that head direction cells show the earliest development of spatial response, followed by the appearance of place cells at a similar developmental stage. In contrast, grid cells emerge later in this developmental sequence. The gradual improvement in spatial stability in firing patterns likely plays a crucial role in the developmental trajectory of grid cells. Contrary to the model simulation, grid cells emerge later than place cells and head direction cells, yet they also hold significance in spatial mapping.

      * The model simulations suggest that certain grid patterns are acquired more gradually than others. For instance, egocentric grid cells require the stabilization of place cell memories amidst ongoing consolidation, while allocentric grid cells tend to reflect average place field positions. However, these findings seemingly conflict with empirical studies, particularly those on the conjunctive representation of distance and direction in the earliest grid cells. Previous studies show no significant differences were found in grid cells and grid cells with directional correlates across these age groups, relative to adults (Wills et al., 2012). This indicates that the combined representation of distance and direction in single mEC cells is present from the earliest ages at which grid cells emerge.

    1. Reviewer #2 (Public Review):

      Summary:

      This valuable study investigates how statistical learning may facilitate a target detection task and whether the facilitation effect is related to statistical learning of word boundaries. Solid evidence is provided that target detection and word segmentation rely on different statistical learning mechanisms.

      Strengths:

      The study is well designed, using the contrast between the learning of words of uniform length and words of variable length to dissociate general statistical learning effects and effects related to word segmentation.

      Weaknesses:

      The study relies on the contrast between word length effects on target detection and word learning. However, the study only tested the target detection condition and did not attempt to replicate the word segmentation effect. It is true that the word segmentation effect has been replicated before but it is still worth reviewing the effect size of previous studies.

      The paper seems to distinguish prediction, anticipation, and statistical learning, but it is not entirely clear what each term refers to.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors present a comprehensive technical overview of the challenging acquisition of large-scale cortical activity, including surgical procedures and custom 3D-printed headbar designs to obtain neural activity from large parts of the dorsal or lateral neocortex. They then describe technical adjustments for stable head fixation, light shielding, and noise insulation in a 2-photon mesoscope and provide a workflow for multisensory mapping and alignment of the obtained large-scale neural data sets in the Allen CCF framework. Lastly, they show different analytical approaches to relate single-cell activity from various cortical areas to spontaneous activity by using visualization and clustering tools, such as Rastermap, PCA-based cell sorting, and B-SOID behavioral motif detection.

      The study contains a lot of useful technical information that should be of interest to the field. It tackles a timely problem that an increasing number of labs will be facing as recent technical advances allow the activity measurement of an increasing number of neurons across multiple areas in awake mice. Since the acquisition of cortical data with a large field of view in awake animals poses unique experimental challenges, the provided information could be very helpful to promote standard workflows for data acquisition and analysis and push the field forward.

      Strengths:

      The proposed methodology is technically sound and the authors provide convincing data to suggest that they successfully solved various challenging problems, such as motion artifacts of large imaging preparations or high-frequency noise emissions, during 2-photon imaging. Overall, the authors achieved their goal of demonstrating a comprehensive approach for imaging neural data across many cortical areas and providing several examples that demonstrate the validity of their methods and recapitulate and further extend some recent findings in the field. A particular focus of the results is to emphasize the need for imaging large population activity across cortical areas to identify cross-area information processing during active behaviors.

      Weaknesses:

      The manuscript contains a lot of technical details and might be challenging for readers without previous experimental experience. However, the different paragraphs illuminate a large range of technical aspects and challenges of large-scale functional imaging. Therefore, the work should be a valuable source of solutions for a diverse audience.

    1. Reviewer #2 (Public Review):

      Summary:

      The aim of this paper was to elucidate the role of the dorsal HP and intermediate HP (dHP and iHP) in value-based spatial navigation through behavioral and pharmacological experiments using a newly developed VR apparatus. The authors inactivated dHP and iHP by muscimol injection and analyzed the differences in behavior. The results showed that dHP was important for spatial navigation, while iHP was critical for both value judgments and spatial navigation. The present study developed a new sophisticated behavioral experimental apparatus and proposed a behavioral paradigm that is useful for studying value-dependent spatial navigation. In addition, the present study provides important results that support previous findings of differential function along the dorsoventral axis of the hippocampus.

      Strengths:

      The authors developed a VR-based value-based spatial navigation task that allowed separate evaluation of "high-value target selection" and "spatial navigation to the target." They were also able to quantify behavioral parameters, allowing detailed analysis of the rats' behavioral patterns before and after learning or pharmacological inactivation.

      Weaknesses:

      Although differences in function along the dorsoventral axis of the hippocampus is an important topic that has received considerable attention, differences in value coding have been shown in previous studies, including the work of the authors; the present paper is an important study that supports previous studies, but the novelty of the findings is not that high, as the results are from pharmacological and behavioral experiments only.

    1. Reviewer #2 (Public Review):

      Summary:

      Developing a mechanical model of C. elegans is difficult to do from basic principles because it moves at low (but not very small) Reynolds number, is itself visco-elastic, and often is measured moving at a solid/liquid interface. The ElegansBot is a good first step at a kinetic model that reproduces a wide range of C. elegans motility behavior.

      Strengths:

      The model is general due to its simplicity and likely useful for various undulatory movements. The model reproduces experimental movement data using realistic physical parameters (e.g. drags, forces, etc). The model is predictive (semi?) as shown in the liquid to solid gait transition. The model is straightforward in implementation and so likely is adaptable to modification and addition of control circuits.

      Comments on revised version:

      This is a revised manuscript. I'm happy with the changes made, including the specific responses to my previous concerns.

    1. Reviewer #3 (Public Review):

      Laham et al. present a manuscript investigating the function of adult-born granule cells (abGCs) projecting to the CA2 region of the hippocampus during social memory. It should be noted that no function for the general DG to CA2 projection has been proposed yet. The authors use targeted ablation, chemogenetic silencing and in vivo ephys to demonstrate that the abGCs to CA2 projection is necessary for the retrieval of a remote social memories such as the memory of one's mother. They also use in vivo ephys to show that abGCs are necessary for differential CA2 network activity, including theta-gamma coupling and sharp wave-ripples, in response to novel versus familiar social stimuli.

      The question investigated is important since the function of DG to CA2 projection remained elusive a decade after its discovery. Overall, the results are interesting but focused to the social memory of the mother and their description in the manuscript and figures is too cursory. For example, raw interaction times must be shown before their difference. The assumption that mice exhibit social preference between familiar or novel individuals such as mother and non-mother based on social memory formation, consolidation and retrieval should be better explained throughout the manuscript. Thus, when describing the results, the authors should comment on changes in preference and how this can be interpreted as a change in social memory retrieval. Several critical experimental details such as the total time of presentation to the mother and non-mother stimulus mice are also lacking from the manuscript. The in vivo e-phys results are interesting as well but even more succinct with no proposed mechanism as to how abGCs could regulate SWR and PAC in CA2.

      The manuscript is well-written with the appropriate references. The choice of behavioral test is somewhat debatable however. It is surprising the authors chose to use a direct presentation test (presentation of the mother and non-mother in alternance) instead of the classical 3-chamber test which is particularly appropriate to investigate social preference. Since the authors focused exclusively on this preference, the 3-chamber test would have been more adequate in my opinion. It would greatly strengthened the results if the authors could repeat a key experiment from their investigation using such test. In addition, the authors only impaired the mother's memory. An additional experiment showing that disruption of the abGCs to CA2 circuit impairs social memory retrieval in general would allow to generalize the findings to social memories in general. As the manuscript stands, the authors can only conclude as to the importance of this circuit for the memory of the mother. Developmental memory implies the memory of familiar kin as well.

      The in vivo ephys section (Figure 3) is interesting but even more minimalistic and it is unclear how abGCs projection to CA2 can contribute to SWR and theta-gamma PAC. In figure 1, the authors suggest that abGCs project preferentially to PV+ neurons in CA2. At minima, the authors should discuss how the abGCs to PV+ neurons to CA2 pyramidal neurons circuit can facilitate SWR and theta-gamma PAC.

      Finally, proposing a function for 4-6-week-old abGCs projecting to CA2 begs two questions: What are abGCs doing once they mature further and more generally, what is the function of the DG to CA2 projection? It would be interesting for the authors to comment on these questions in the discussion.

      Revision:

      The authors have followed my recommendations except for the ones suggesting new experiments. As a result, the clarity of the manuscript and the links between evidence and claims have improved by the message is quite reduced. Many important questions remain open such as: What makes mother's memories so special they require the abGC projection to CA2 unlike other types of social memories? Do abGCs truly connect CA2 PV+ interneurons and how does this connection shape sharp-wave ripples in CA2?

    1. Reviewer #2 (Public Review):

      Summary:

      Methods to infer action potentials from fluorescence-based measurements of intracellular calcium dynamics are important for optical measurements of activity across large populations of neurons. The variety of existing methods can be separated into two broad classes: a) model-independent approaches that are trained on ground truth datasets (e.g., deep networks), and b) approaches based on a model of the processes that link action potentials to calcium signals. Models usually contain parameters describing biophysical variables, such as rate constants of the calcium dynamics and features of the calcium indicator. The method presented here, PGBAR, is model-based and uses a Bayesian approach. A novelty of PGBAR is that static parameters and state variables are jointly estimated using particle Gibbs sampling, a sequential Monte Carlo technique that can efficiently sample the latent embedding space.

      Strengths:

      A main strength of PGBAR is that it provides probability distributions rather than point estimates of spike times. This is different from most other methods and may be an important feature in cases when estimates of uncertainty are desired. Another important feature of PGBAR is that it estimates not only the state variable representing spiking activity but also other variables such as baseline fluctuations and stationary model variables, in a joint process. PGBAR can therefore provide more information than various other methods. The information in the GitHub repository is well-organized.

      Weaknesses:

      On the other hand, the accuracy of spike train reconstructions is not higher than that of other model-based approaches, and clearly lower than the accuracy of a model-independent approach based on a deep network. The authors demonstrate convincingly that PGBAR can resolve inter-spike intervals in the range of 5 ms using fluorescence data obtained with a very fast genetically encoded calcium indicator at very high sampling rates (line scans at >= 1 kHz). It would be interesting to more systematically compare the performance of PGBAR to other methods in this regime of high temporal resolution, which has not been explored much.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors have diligently addressed most of the points raised during the review process (except the important point of "additional in vitro experiments [...] needed to investigate the implication of circHIPK3 in bladder cancer cell phenotype" for which no additional experiments were performed), resulting in an improvement in the study. The data are now described with clarity and conciseness, enhancing the overall quality of the manuscript.

      Strengths:

      New, well-defined molecular mechanism of circRNAs involvement in bladder cancer.

      Weaknesses:

      Lack of solid translational significance data.

    1. Reviewer #2 (Public Review):

      The manuscript has been revised according to Reviewer's suggestions. Recommendations for the Authors have been almost entirely followed. However, there are some points where the authors state that they have made changes, but the text does not show this. The revised version would have gained in clarity if it was with track changes and numbered rows. In particular, I cannot see the following changes:

      Lines 104-105: Did you mean: "We confirmed that optogenetic stimulation of PiCo neurons in ChATcre:Vglut2FlpO:ChR2 mice exposed to CIH triggers swallow and laryngeal activation similar to the control mice exposed to room air (Huff et al., 2023)." Otherwise, the sentence is not clear.<br /> Thank you, this has been changed

      Lines 228-232: "PiCo-triggered swallows are characterized by a significant decrease in duration compared to swallows evoked by water in ChATcre:Ai32 mice (265 {plus minus} 132ms vs 144 {plus minus} 101ms; paired t-test: p= 0.0001, t= 5.21, df= 8), Vglut2cre:Ai32 mice (308 {plus minus} 184ms vs 125 {plus minus} 44ms; paired t-test: p= 0.0003, t= 6.46, df= 7), and ChATcre:Vglut2FlpO:ChR2 mice (230 {plus minus} 67ms vs 130 {plus minus} 35ms; paired t-test: p= 0.0005, t= 5.62, df= 8) exposed to CIH (Table S1).".<br /> Thank you, this has been changed

      Lines 283-290: "Thus, CIH does not alter PiCo's ability to coordinate the timing for swallowing and breathing. Rather, our data reveals that CIH disrupts the swallow motor sequence likely due to changes in the interaction between PiCo and the SPG, presumably the cNTS.

      While it has previously been demonstrated that PiCo is an important region in swallow-breathing coordination (Huff et al., 2023), previous studies did not demonstrate that PiCo is involved in swallow pattern generation itself. Thus, here we show for the first time that CIH resulted in the instability of the swallow motor pattern activated by stimulating PiCo, suggesting PiCo plays a role in its modulation.".<br /> Thank you, this has been changed

      Line 437: Mice of the ChATcre:Ai32, Vglut2cre:Ai32 and ChATcre:Vglut2FlpO:ChR2 lines were kept in collective cages with food and water ad libitum placed inside custom-built chambers.<br /> Thank you, this has been changed.

      Overall, the manuscript has been improved.

    1. Reviewer #2 (Public Review):

      Summary:

      In the present study, the authors investigated the neural coding mechanisms for D1- and D2-expressing striatal direct and indirect pathway MSNs in interval timing by using multiple strategies. They concluded that D2-MSNs and D1-MSNs have opposing temporal dynamics yet disrupting either type produced similar effects on behavior, indicating the complementary roles of D1- and D2- MSNs in cognitive processing. However, the data was incomplete to fully support this major finding. One major reason is the heterogenetic responses within the D1-or D2-MSN populations. In addition, there are additional concerns about the statistical methods used. For example, the majority of the statistical tests are based on the number of neurons, but not the number of mice. It appears that the statistical difference was due to the large sample size they used (n=32 D2-MSNs and n=41 D1-MSNs), but different neurons recorded in the same mouse cannot be treated as independent samples; they should use independent mouse-based statistical analysis.

      Strengths:

      The authors used multiple approaches including awake mice behavior training, optogenetic-assistant cell-type specific recording, optogenetic or pharmacological manipulation, neural computation, and modeling to study neuronal coding for interval timing.

      Weaknesses:

      (1) More detailed behavior results should be shown, including the rate of the success switches, and how long it takes to wait in the second nose poke to get a reward. For line 512 and the Figure 1 legend, the reviewer is not clear about the reward delivery. The methods appear to state that the mouse had to wait for 18s, then make nose pokes at the second port to get the reward. What happens if the mouse made the second nose poke before 18 seconds, but then exited? Would the mouse still get the reward at 18 seconds? Similarly, what happens if the mice made the third or more nosepokes within 18 seconds? It is important to clarify because, according to the method described, if the mice made a second nose poke before 18 seconds, this already counted as the mouse making the "switch." Lastly, what if the mice exited before 6s in the first nosepoke?

      (2) There are a lot of time parameters in this behavior task, the description of those time parameters is mentioned in several parts, in the figure legend, supplementary figure legend, and methods, but was not defined clearly in the main text. It is inconvenient, sometimes, confusing for the readers. The authors should make a schematic diagram to illustrate the major parameters and describe them clearly in the main text.

      (3) In Line 508, the reviewer suggests the authors pay attention to those trials without "switch". It would be valuable to compare the MSN activity between those trials with or without a "switch".

      (4) The definition of interval is not very clear. It appears that the authors used a 6-second interval in analyzing the data in Figure 2 and Figure 3. But from my understanding, the interval should be the time from time "0" to the "switch", when the mice start to exit from the first nose poke.

      (5) For Figure 2 C-F, the authors only recorded 32 D2-MSNs in 4 mice, and 41 D1-MSNs in 5 mice. The sample size is too small compared to the sample size usually used in the field. In addition to the small sample size, the single-cell activity exhibited heterogeneity, which created potential issues. For both D1 and D2 MSNs, the authors tried to make conclusions on the "trend" of increasing in D2-MSNs and decreasing in D1-MSNs populations, respectively, during the interval. However, such a conclusion is not sufficiently supported by the data presented. It looks like the single-cell activity patterns can be separated into groups: one is a decreasing activity group, one is an increasing activity group and a small group for on and off response. Because of the small sample size, the author should pay attention to the variance across different mice (which needs to be clearly presented in the manuscript), instead of pooling data together and analyzing the mean activity.

      (6) For Figure 2, from the activity in E and F, it seems that the activity already rose before the trial started, the authors should add some longer baseline data before time zero for clarification and comparison, and show the timing of the actual start of the activity with the corresponding behavior. What behavior states are the mice in when initiating the activity?

      (7) The authors were focused on the "switch " behavior in the task, but they used an arbitrary 6s time window to analyze the activity, and tried to correlate the decreasing or increasing activities of MSNs to the neural coding for time. A better way to analyze is to sort the activity according to the "switch" time, from short to long intervals. This way, the authors could see and analyze whether the activity of D1 or D2 MSNs really codes for the different length of interval, instead of finding a correlation between average activity trends and the arbitrary 6s time window.

    1. Reviewer #2 (Public Review):

      Summary:

      In this study, the authors find that the deletion of a sulfate transporter in yeast, Sul1, leads to the extension of replicative lifespan. They investigate mechanisms underlying this extension and claim that the effects on longevity can be separated from sulfate transport, and are instead linked to a previously proposed transceptor function of the Sul1 transporter. Through RNA sequencing analysis, the authors find that Sul1 loss triggers activation of several stress response pathways, and conclude that deletion of two pathways, autophagy or Msn2/4, partially prevents lifespan extension in cells lacking Sul1. Overall, while it is well-appreciated that activation of Msn2/4 or autophagy is beneficial for lifespan extension in yeast, the results of this study would add an important new mechanism by which this could achieved, through perceived sulfate starvation. However, as described below, several of the experiments utilized to support the authors' conclusion are not experimentally sound, and significant additional experimentation is required to support the authors' claims throughout the manuscript.

      Strengths:

      The major strength of the study is the robust RNA-seq data that identified differentially expressed genes in cells lacking Sul1. This facilitated the authors' focus on two of these pathways, autophagy and the Msn2/4 stress response pathway.

      Weaknesses:

      Several critical experimental flaws need to be addressed by the authors to more rigorously test their hypothesis.

      (1) The lifespan assays throughout the manuscript contain inconsistencies in the mean lifespan of the wild-type strain, BY4741. For example, in Figure 1A, the lifespan of BY4741 is 24.3, and the extended lifespan of the sul1 mutant is 31. However, although all mutants tested in Figure 1B also have lifespans close to 30 cell divisions, the wild-type control is also at 30 divisions in those experiments as well. This is problematic, as it makes it impossible to conclude anything about the lifespan extension of various mutants with inconsistencies in the wild-type lifespan. Additionally, the mutants analyzed in 1B are what the authors use to claim that loss of the transporter does not extend lifespan through sulfate limitation, but instead through a signaling function. Thus, it remains unclear whether loss of sul1 extends lifespan at all, and if it does, whether this is separable from cellular sulfate levels.

      (2) While the authors use mutants in Figure 1 that should have differential effects on sulfate levels in cells, the authors need to include experiments to measure sulfate levels in their various mutant cells to draw any conclusions about their data.

      3) Similar to point 2, the authors focused their RNA sequencing analysis on the deletion of sul1 and did not include important RNA seq analysis of the specific Sul1 mutation or other mutants in Figure 1B that do not exhibit lifespan extension. The prediction is that they should not see the activation of stress response pathways in these mutants as they do not see lifespan extension, but this needs to be tested.

      (4) While the RNA-seq data is robust in Figure 2 as well as the follow-up quantitative PCR and trehalose/glycogen assays in 2A-B, the follow-up imaging assays for Msn2/4 localization in Figure 2 are not robust and are difficult to interpret. The authors need to include more high-resolution imaging or at least a close-up of the cells in Figure 3C.

      (5) The autophagy assays utilized in Figure 4 appear to all be done with a C-terminal GFP-tagged Atg8 protein. As C-terminal GFP is removed from Atg8 prior to conjugation to phosphatidylethanolamine, microscopy assays of this reporter cannot be utilized to report on autophagy activity or flux. Instead, the authors need to utilize N-terminally tagged Atg8, which they can monitor for vacuole uptake as an appropriate readout of autophagy levels. As it stands, the authors cannot draw any conclusions about autophagy activity in their studies.

    1. Reviewer #2 (Public Review):

      Summary:

      Bestry et al. investigated the effects of prenatal alcohol exposure (PAE) and high methyl donor diet (HMD) on offspring DNA methylation and behavioral outcomes using a mouse model that mimics common patterns of alcohol consumption in pregnancy in humans. The researchers employed whole-genome bisulfite sequencing (WGBS) for unbiased assessment of the epigenome in the newborn brain and liver, two organs affected by ethanol, to explore tissue-specific effects and to determine any "tissue-agnostic" effects that may have arisen prior to the germ-layer commitment during early gastrulation. The authors found that PAE induces measurable changes in offspring DNA methylation. DNA methylation changes induced by PAE coincide with non-coding regions, including enhancers and promoters, with the potential to regulate gene expression. Though the majority of the alcohol-sensitive differentially methylated regions (DMRs) were not conserved in humans, the ones that were conserved were associated with clinically relevant traits such as facial morphology, educational attainment, intelligence, autism, and schizophrenia Finally, the study provides evidence that maternal dietary support with methyl donors alleviates the effects of PAE on DNA methylation, suggesting a potential prenatal care option.

      Strengths:

      The strengths of the study include the use of a mouse model where confounding factors such as genetic background and diet can be well controlled. The study performed whole-genome bisulfite sequencing, which allows a comprehensive analysis of the effects of PAE on DNA methylation.

      Weaknesses:

      Transcriptome analysis to test if the identified DMRs indeed affect gene expression would help determine the potential function of the identified methylation changes.

    1. Reviewer #2 (Public Review):

      This work started with transcriptomic profiling of ductal cells to identify the upregulation of calcineurin in the zebrafish after beta-cell ablation. By suppressing calcineurin with its chemical inhibitor cyclosporin A and expressing a constitutively active form of calcineurin ubiquitously or specifically in ductal cells, the authors found that inhibited calcineurin activity promoted beta-cell regeneration transiently while ectopic calcineurin activity hindered beta-cell regeneration in the pancreatic tail. They also showed similar effects in the basal state but only when it was within a particular permissive window of Notch activity. To further investigate the roles of calcineurin in the ductal cells, the authors demonstrated that calcineurin inhibition additionally induced the proliferation of the ductal cells in the regenerative context or under a limited level of Notch activity. Interestingly, the enhanced proliferation was followed by a depletion of ductal cells, suggesting that calcineurin inhibition would exhaust the ductal cells. Based on the data, the authors proposed a very attractive and intriguing model of the role of calcineurin in maintaining the balance of the progenitor proliferation and the endocrine differentiation. However, the conclusions of this paper are only partially supported by the data as some evidence of the lineage between ductal cells and beta cells remains suggestive.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors have generated human iPSC cells constitutively expressing the mNG21-10 and tested them by endogenous tagging multiple genes with mNG211 (several tagged iPS cell lines clones were isolated). With this tool they have explored several weakly expressed cytokinesis genes gained insights into how cytokinesis occurs.

      Strengths:

      (i) Human iPSC cells are used

      Weaknesses:

      (i) The manuscript is extremely incremental, no improvements are present in the split-Fluorescent (split-FP) protein variant used nor in the approach for endogenous tagging with split-FPs (both of them are already very well established and used in literature as well as in different cell types).

      (ii) The fluorescence intensity of the split mNeonGreen appears rather low, for example in Figure 2C the H2BC11, ANLN, SOX2 and TUBB3 signals are very noisy (differences between the structures observed are almost absent). For low expression targets this is an important limitation. This is also stated by the authors but image restoration could not be the best solution since a lot of biologically relevant information will be lost anyway.

      (iii) there is no comparison with other existing split-FP variants, methods, or imaging and it is unclear what the advantages of the system are.

    1. Reviewer #2 (Public Review):

      Summary:

      The manuscript by Kokinovic et al. presents evidence that a significant portion of striatal projection neurons (SPNs) are spontaneously active early in development. This spontaneous activity (as measured in ex vivo brain slices) is due to intrinsic mechanisms, and subsides over the course of the first few postnatal weeks in a cell-type specific way: striosome direct and indirect pathway SPNs (dSPNs and iSPNs, respectively) remain spontaneously active until postnatal days 10-14, by which time matrix dSPNs and iSPNs have become entirely silent. The authors suggest that this early spontaneous activity may be in part due to M1 muscarinic receptor signaling. Through chemogenetic inhibition of striosome SPNs (of which dSPNs target dopaminergic neurons of the SNc), the authors present evidence that critical postnatal windows of SPN activity shape the strength of GABAergic innervation of the SNc (measured in adults). This study provides a useful and solid characterization of the functional, postnatal compartmental development of the striatum. However, some weaknesses in the experimental design should be addressed before definitively concluding that postnatal striosome SPN activity determines its functional innervation of dopaminergic SNc neurons.

      Specific Comments:

      (1) While certainly interesting and possibly true, evidence for the necessity of early striosome dSPN activity in shaping their functional innervation of dopaminergic SNc neurons is not entirely convincing. The functional measure of GABAergic innervation of dopamine neurons is inferred from mIPSCs. As the authors state, dopaminergic neurons have numerous other sources of GABAergic inputs in addition to striosome dSPNs. So while manipulating striosome activity may ultimately alter the overall GABAergic innervation of SNc dopamine neurons, the specificity of this to striosome dSPN inputs is not known. Optogenetic stimulation of striosome->SNc neurons after chemogenetic silencing would help support the authors' interpretation. Related to this point, while striatonigral projections form embryonically, is there evidence that striosome->SNc synapses are indeed functional by P6-14 when CNO is delivered?

      (2) One big caveat that needs to be addressed is that all measures of early postnatal spontaneous SPN activity were performed in ex vivo slices. Are SPNs active (in pathway/compartmental specific ways) in vivo during this time? If it is unknown, is there other evidence (e.g. immediate early gene expression, etc...) that may suggest this is indeed the case in vivo?

      (3) It appears that 8mM KCl (external) was only used while measuring spontaneous calcium oscillations, not spontaneous spiking (Figure 2). Was there any evidence of spontaneous calcium activity in the lower KCl concentration (3mM?) used for cell-attached recordings? One caveat is that experiments demonstrating that SPNs fire spontaneously in the presence of AMPA receptor blockers (Figure S1) were presumably performed in 3mM KCl. Does elevated KCl increases spontaneous EPSPs during the ages examined? If so, are the calcium oscillations shown in Figure 2 synaptically driven or intrinsically generated? Somewhat related, speculation on why M1 receptor blockade reduces calcium oscillations but not spontaneous spikes in striosome dSPNs would be useful.

      (4) Several statements in the introduction could use references.

    1. Reviewer #2 (Public Review):

      The authors sought to establish the role played by N343 glycosylation on the SARS-CoV-2 S receptor binding domain structure and binding affinity to the human host receptor ACE2 across several variants of concern. The work includes both computational analysis in the form of molecular dynamics simulations and experimental binding assays between the RBD and ganglioside receptors.

      The work extensively samples the conformational space of the RBD beginning with atomic coordinates representing both the bound and unbound states and computes molecular dynamics trajectories until equilibrium is achieved with and without removing N343 glycosylation. Through comparison of these simulated structures, the authors are able to demonstrate that N343 glycosylation stabilizes the RBD. Prior work had demonstrated that glycosylation at this site plays an important role in shielding the RBD core and in this work, the authors demonstrate that removal of this glycan can trigger a conformational change to reduce water access to the core without it. This response is variant-dependent and variants containing interface substitutions that increase RBD stability, including Delta substitution L452R, do not experience the same conformational change when the glycan is removed. The authors also explore structures corresponding to Alpha and Beta in which no structure-reinforcing substitutions were identified and two Omicron variants in which other substitutions with an analogous effect to L452R are present.

      The authors experimentally assessed these inferred structural changes by measuring the binding affinity of the RBD for the oligosaccharides of the mono-sialylated gangliosides GM1os and GM2os with and without the glycan at N343. While GM1os and GM2os binding is influenced by additional factors in the Beta and Omicron variants, the comparison between Delta and Wuhan-hu-1 is clear: removal of the glycan abrogated binding for Wuhan-hu-1 and minimally affected Delta as predicted by structural simulations.

      In summary, these findings suggest, in the words of the authors, that SARS-CoV-2 has evolved to render the N-glycosylation site at N343 "structurally dispensable". This study emphasizes how glycosylation impacts both viral immune evasion and structural stability which may in turn impact receptor binding affinity and infectivity. Mutations that stabilize the antigen may relax the structural constraints on glycosylation opening up avenues for subsequent mutations that remove glycans and improve immune evasion. This interplay between immune evasion and receptor stability may support complex epistatic interactions which may in turn substantially expand the predicted mutational repertoire of the virus relative to expectations that do not take into account glycosylation.

    1. Reviewer #2 (Public Review):

      Summary:

      Using K562 (Leukemia) cells as an experimental model, Van Vracken et. al. use Thermal Proteome Profiling (TPP) to investigate changes in protein stability after exposing either live cells or crude cell lysates to a library of anti-cancer drugs. This was a large-scale and highly ambitious study, involving thousands of hours of mass spectrometry instrument time. The authors used an innovative combination of TPP together with Proteome Integral Solubility Alternation (PISA) assays to reduce the amount of instrument time needed, without compromising on the amount of data obtained.

      The paper is very well written, the relevance of this work is immediately apparent, and the results are well-explained and easy to follow even for a non-expert. The figures are well-presented. The methods appear to be explained in sufficient detail to allow others to reproduce the work.

      Strengths:

      Using CDK4/6 inhibitors, the authors observe strong changes in protein stability upon exposure to the drug. This is expected and shows their methodology is robust. Further, it adds confidence when the authors report changes in protein stability for drugs whose targets are not well-known. Many of the drugs used in this study - even those whose protein targets are already known - display numerous off-target effects. Although many of these are not rigorously followed up in this current study, the authors rightly highlight this point as a focus for future work.

      Weaknesses:

      While the off-target effects of several drugs could've been more rigorously investigated, it is clear the authors have already put a tremendous amount of time and effort into this study. The authors have made their entire dataset available to the scientific community - this will be a valuable resource to others working in the fields of cancer biology/drug discovery.

    1. Reviewer #2 (Public Review):

      Summary:

      This paper examines the recruitment of the inflammasome seeding pattern recognition receptor NLRP3 to the Golgi. Previously, electrostatic interactions between the polybasic region of NLRP3 and negatively charged lipids were implicated in membrane association. The current study reports that reversible S-acylation of the conserved Cys-130 residue, in conjunction with upstream hydrophobic residues plus the polybasic region, act together to promote Golgi localization of NLRP3, although additional parts of the protein are needed for full Golgi localization. Treatment with the bacterial ionophore nigericin inhibits membrane traffic and prevents Golgi-associated thioesterases from removing the acyl chain, causing NLRP3 to become immobilized at the Golgi. This mechanism is put forth as an explanation for how NLRP3 is activated in response to nigericin.

      Strengths:

      The experiments are generally well presented. It seems likely that Cys-130 does indeed play a previously unappreciated role in the membrane association of NLRP3.

      Weaknesses:

      The interpretations about the effects of nigericin are less convincing. Specific comments follow.

      (1) The experiments of Figure 4 bring into question whether Cys-130 is S-acylated. For Cys-130, S-acylation was seen only upon expression of a severely truncated piece of the protein in conjunction with overexpression of ZDHHC3. How do the authors reconcile this result with the rest of the story?

      (2) Nigericin seems to cause fragmentation and vesiculation of the Golgi. That effect complicates the interpretations. For example, the FRAP experiment of Figure 5 is problematic because the authors neglected to show that the FRAP recovery kinetics of non-acylated resident Golgi proteins are unaffected by nigericin. Similarly, the colocalization analysis in Figure 6 is less than persuasive when considering that nigericin significantly alters Golgi structure and could indirectly affect colocalization.

    1. Reviewer #2 (Public Review):

      Summary:

      Extensive previous research has shown that cell confinement, e.g., vertical compression of cells to a height smaller than the height of the unconfined cells, results in the unfolding of nuclear membrane invaginations, calcium and membrane tension mediated recruitment of cPLA2 to the nuclear membrane (which triggers increased cortical myosin accumulation and activity, among other effects), nuclear blebbing, and DNA damage. However, the long-term effects of confinement, and how cells adapt to such confined conditions, have remained largely unexplored.

      In this work, the authors use custom-built cell confinement devices that enable precise control of confinement for prolonged periods of time (up to several days), along with live cell and fixed cell imaging to compare short-term (2 hours) and long-term (24+ hours) effects of confinement on nuclear structure. The authors report that while vertical confinement results in a short-term increase in nuclear cross-sectional area, associated with an increase in nuclear surface area due to unfolding of nuclear envelope invaginations while maintaining nuclear volume, long-term confinement results in a decrease in nuclear volume, reduced cross-sectional area, and re-appearance of nuclear envelope invaginations. Using time-lapse imaging, the authors demonstrate that these effects are associated with a reduction in nuclear volume upon completion of the first mitosis under confinement. Pharmacological inhibition experiments indicate a requirement of cPLA2, calcium signaling, and actomyosin contractility in this process. Although it is not surprising that nuclear blebs disappear following mitosis, as the nuclear envelope breaks down at the onset of mitosis and subsequently reforms as the chromatin decondenses, the observed change in nuclear volume upon prolonged confinement is intriguing. Notably, the nuclear adaptation following prolonged confinement was also associated with a reduction in DNA damage when comparing cells at 2h and 24h of confinements, measured by the presence of gamma-H2AX foci in the nucleus. By fitting their experimental data of nuclear surface area measurements, the authors arrive at the conclusion that cells have an intrinsic nuclear envelope tension set-point and that completing mitosis enables cells to reset nuclear envelope tension to this set-point.

      Strengths:

      The use of an agarose confinement system with precise control over vertical confinement enables the authors to apply long-term confinement without depriving cells of nutrients while performing live cell imaging or immunofluorescence analysis following fixation. The live cell imaging is a powerful tool to assess the effect of confinement not only on nuclear morphology, but also on cell cycle progression (using the FUCCI fluorescent reporter) and to compare nuclear volume between mother and daughter cells. The data presented by the authors to demonstrate changes in nuclear volume and surface area are convincing and supported by several independent measurements. The model comparing total and apparent nuclear surface area nicely complements the experimental measurements and helps to make the point that cells have a nuclear envelope tension set-point, even though the authors were unable to directly measure nuclear envelope tension. The inhibitor experiments targeting cPLA2 (using AACOCF3), intracellular calcium (using BAPTA-Amand 2APB), and myosin contractility (using blebbistatin) identify key players in the underlying cellular mechanism.

      Weaknesses:

      Although the findings by the authors will be of interest to a broad community, several weaknesses limit the mechanistic insights gained from this study. One major limitation is that all experiments are performed in a single cell line, H-29 human colorectal cancer cells, which has an unusual nuclear envelope composition as it has no lamin B2, low lamin B1 levels, and contains a p53 mutation. Because lamins B1 and B2 play important functions in protecting the nuclear envelope from blebs and confinement-induced rupture, and p53 is crucial in the cellular DNA damage response, it remains unclear whether other cell lines exhibit similar adaptation behavior.

      Furthermore, although the time-lapse experiments suggest that reduction in nuclear volume occurs primarily during mitosis, the authors do not address whether prolonged confinement, even in the absence of apoptosis, could also result in cells adjusting their nuclear volume, or alternatively normalizing nuclear envelope tension by recruiting additional membrane from the endoplasmic reticulum, which is continuous with the nuclear membranes.

      Additionally, the molecular mechanisms underlying the observed loss in nuclear volume and the regulation of this process remain to be identified. The pharmacological studies implicate cPLA2, intracellular calcium, and actomyosin contractility in this process, but do not include validation to confirm the efficiency of the drug treatment or to rule out off-target effects. Regarding the proposed role of cPLA2, previous studies have shown that cPLA2 recruitment to the nuclear membrane, which is essential to mediate its nuclear mechanotransduction function, requires both an increase in nuclear membrane tension and intracellular calcium. However, the current study does not include any data showing the recruitment of cPLA2 to the nuclear membrane upon confinement, or the disappearance of nuclear membrane-associated cPLA2 during prolonged confinement, leaving unclear the precise function and dynamics of cPLA2 in the process.

      Lastly, it remains unclear (1) whether the reduction in nuclear volume is caused by a reduction in nuclear water content, by chromatin compaction, e.g. associated with an increase in heterochromatin, or through other mechanisms, (2) whether the change in nuclear volume is reversible, and if so, how quickly, and (3) what functional consequences the substantial reduction in nuclear volume has on nuclear function, as one would expect that this reduction would be associated with a substantial increase in nuclear crowding, affecting numerous nuclear processes.

    1. Reviewer #2 (Public Review):

      Summary:

      This work provides a new framework, "GPsite" to predict DNA, RNA, peptide, protein, ATP, HEM, and metal ions binding sites on proteins. This framework comes with a webserver and a database of annotations. The core of the model is a Geometric featurizer neural network that predicts the binding sites of a protein. One major contribution of the authors is the fact that they feed this neural network with predicted structure from ESMFold for training and prediction (instead of native structure in similar works) and a high-quality protein Language Model representation. The other major contribution is that it provides the public with a new light framework to predict protein-ligand interactions for a broad range of ligands. It is a convincing outcome of previous efforts to Geometric Deep Learning approaches to model protein-ligand interactions. The authors have demonstrated the interest of their framework with comprehensive ablation studies and benchmarks.

      Strengths:

      - The performance of this framework as well as the provided dataset and web server make it useful to conduct studies.<br /> - The ablations of some core elements of the method, such as the protein Language Model part, the use of multiple ligands in the same model, the input structure, or the use of predicted structure to complement native structure are very insightful. They can help convince the reader that every part of the framework is necessary. This could also guide further developments in the field. As such, the presentation of this part of the work holds a critical place in this work.

      Weaknesses:

      - The authors made an important effort to compare their work to other similar frameworks. Yet, the lack of homogeneity of training methods and data from one work to the other makes the comparison slightly unconvincing, as the authors pointed out. Ablations performed by the authors were able to compensate for this general weakness, as well as the focus on several example structures.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors tried to understand the mechanism on how a drug candidate, VLZ, works on a receptor, 5-HTR1A, by activating the SRC/MAPK pathway to promote the formation of platelets.

      Strengths:

      The authors used both computational and experimental methods. This definitely saves time and funds to find a useful drug candidate and its therapeutic marker in the subfield of platelets reduction in cancer patients. The authors achieved the aim to explain the mechanism of VLZ on improving thrombocytopenia by using two cell lines and two animal models.

      Weaknesses:

      Only two cell lines, HEL and Meg-01 cells, were evaluated in this study. However, using more cell lines is really depending on the work flow and the grant situations of the current research team.

    1. Reviewer #2 (Public Review):

      The study conducted by Benita et al studied the gut and nasopharyngeal microbiome in covid-19 severity. There are a lot of studies on this topic, and this study therefore cannot stand out from a pool of such similar studies. Beyond that, I have a number of major concerns:

      (1) The sample size is limited. There were 3 cohorts, but only ~100 subjects in total. This indicates that there were only a small number of subjects in each cohort (the authors did not list this information), and beyond that, there was a lack of healthy individuals as controls. A cohort-specific effect should usually exist, I believe with such a small number of patients (they were further divided into 3 groups), the authors cannot find reproducible data between cohorts.

      (2) The study did not meet the study goal. The authors say "Many factors have been described to be correlated with its severity but no specific determinants of infection outcome have been identified yet". However, numerous studies have shown the relationship between microbiome and covid. The present study only again showed a correlation between microbiome and covid severity and did not provide further insights, nor did they find specific determinants.

      (3) This study only studied 16s-seq for microbiome profiling, which made this study lack depth and resolution. Many peer papers have used metagenomics sequencing for in-depth interrogation.

      (4) Since there are fecal and nasopharyngeal microbiome data, the authors only listed their respective associations with covid severity yet did not provide further insights into whether and how these two microbiome types are linked to covid, or into whether there is a microbiome priority, resistance or transmission.

      (5) The abstract is amiss where each sentence lacks a key message - I don't understand each of the sentences or the underlying meanings. One example of an unclear expression is "this ratio" - what ratio?

      (6) The figures are all unclear and need significant improvement

    1. Depuis la révision constitutionnelle de 2003, la péréquation est un objectif de valeur constitutionnelle. L’article 72-2 de la Constitution dispose que : La loi prévoit des dispositifs de péréquation destinés à favoriser l'égalité entre les collectivités territoriales.
    1. Reviewer #2 (Public Review):

      The authors developed an original knock-in reporter mice line expressing ZSGreen under the control of endogenous FSHR promoter. The existence of FSHR in various extra-gonadal tissues and the physio-pathological consequences indeed remains a debated question and could potentially have an important impact on many high-incidence diseases occurring in menopausal women. Unfortunately, the provided data set lacks crucial controls and therefore does not provide a robust/convincing answer to the above-mentioned question.

      Summary:<br /> The authors investigated the expression pattern of the FSHR in the gonads, where its expression has been demonstrated for decades, but also in many extra-gonadal tissues. The question is important since the expression of FSHR outside of the gonads has been increasingly reported and associated with the dramatic increase of circulating FSH after menopause, and has been suggested to play an important role in the advent of multiple diseases occurring with high incidence in post-menopausal women. However, the reality of such extra-gonadal expression of FSHR remains debated, mainly because this receptor is expressed at a low level and because the specificity/affinity of the available anti-FSHR antibodies is questionable.

      Strengths:<br /> The development of reporter mice expressing ZsGreen fluorescent protein under the control of endogenous FSHR promoter is an original and potentially powerful approach to tackle the problem.

      Weaknesses:<br /> The data provided are provocative since the FSHR seems to be expressed in all tested tissues. In the testis, for instance, the authors report very high levels of FSHR in interstitial cells and germ cells. In the ovary, there seems to be no difference in FSHR expression between granulosa cells and the other cell types. These findings alone contradict all the knowledge on FSH expression patterns in the gonads that have been accumulated over decades by many independent labs. In view of such results, the validity of the reporter mice line should be questioned thoroughly:

      (1) Is the FSHR expression pattern affected by the knockin mice (no side-by-side comparison between wt and GSGreen mice, using in situ hybridization and ddRTPCR, at least in the gonads, is provided)?

      (2) Is the splicing pattern of the FSHR affected in the knockin compared to wt mice, at least in the gonads?

      (3) Are there any additional off-target insertions of GSGreen in these mice?

      (4) Are similar results observed in separate founder mice?

      (5) How long is GSGreen half-life? Could a very long half-life be a major reason for the extremely large expression pattern observed?

      In the absence of answers to these questions, the data produced in extra-gonadal tissues using the same reporter mice, are not convincing and do not support the authors' claims.

    1. Reviewer #2 (Public Review):

      In their study, Podkowik et al. elucidate the protective role of the accessory gene regulator (agr) system in Staphylococcus aureus against hydrogen peroxide (H2O2) stress. Their findings demonstrate that agr safeguards the bacterium by controlling the accumulation of reactive oxygen species (ROS), independent of agr activation kinetics. This protection is facilitated through a regulatory interaction between RNAIII and Rot, impacting virulence factor production and metabolism, thereby influencing ROS levels. Notably, the study highlights the remarkable adaptive capabilities of S. aureus conferred by agr. The protective effects of agr extend beyond the peak of agr transcription at high cell density, persisting even during the early log-phase. This indicates the significance of agr-mediated protection throughout the infection process. The absence of agr has profound consequences, as observed by the upregulation of respiration and fermentation genes, leading to increased ROS generation and subsequent cellular demise. Interestingly, the study also reveals divergent effects of agr deficiency on susceptibility to hydrogen peroxide compared to ciprofloxacin. While agr deficiency heightens vulnerability to H2O2, it also upregulates the expression of bsaA, countering the endogenous ROS induced by ciprofloxacin. These findings underscore the complex and context-dependent nature of agr-mediated protection. Furthermore, in vivo investigations using murine models provide valuable insights into the importance of agr in promoting S. aureus fitness, particularly in the context of neutrophil-mediated clearance, with notable emphasis on the pulmonary milieu. Overall, this study significantly advances our understanding of agr-mediated protection in S. aureus and sheds light on the sophisticated adaptive mechanisms employed by the bacterium to fortify itself against oxidative stress encountered during infection.

      The conclusions drawn in this paper are generally well-supported by the data.

    1. Reviewer #2 (Public Review):

      Summary:

      This manuscript reports a novel and quite important study of chimerism among common marmosets. As the authors discuss, it has been known for years that marmosets display chimerism across a number of tissues. However, as the authors also recognize, the scope and details of this chimerism have been controversial. Some prior publications have suggested that the chimerism only involves cells derived from hematopoietic stem cells, while other publications have suggested more cell types can also be chimeric, including a wide range of cell types present in multiple organs. The present authors address this question and several other important issues by using snRNA-seq to track the expression of host and sibling-derived mRNAs across multiple tissues and cell types. The results are clear and provide strong evidence that all chimeric cells are derived from hematopoietic cell lineages.

      This work will have an impact on studies using marmosets to investigate various biological questions but will have the biggest impact on neuroscience and studies of cellular function within the brain. The demonstration that microglia and macrophages from different siblings from a single pregnancy, with different genomes expressing different transcriptomes, are commonly present within specific brain structures of a single individual opens a number of new opportunities to study microglia and macrophage function as well as interactions between microglia, macrophages, and other cell types.

      Strengths:

      The paper has a number of important strengths. This analysis employs the first unambiguous approach providing a clear answer to the question of whether sibling-derived chimeric cells arise only from hematopoietic lineages or from a wider array of embryonic sources. That is a long-standing open question and these snRNA-seq data seem to provide a clear answer, at least for the brain, liver, and kidney. In addition, the present authors investigate quantitative variation in chimeric cell proportions across several dimensions, comparing the proportion of chimeric cells across individual marmosets, across organs within an individual, and across brain regions within an individual. All these are significant questions, and the answers have important implications for multiple research areas. Marmosets are increasingly being used for a range of neuroscience studies, and a better understanding of the process that leads to the chimerism of microglia and macrophages in the marmoset brain is a valuable and timely contribution. But this work also has implications for other lines of study. Third, the snRNA-seq data will be made available through the Brain Initiative NeMO portal and the software used to quantify host vs. sibling cell proportions in different biosamples will be available through GitHub.

      Weaknesses:

      I find no major weaknesses, but several minor ones. First, the main text of the manuscript provides no information about the specific animals used in this study, other than sex. Some basic information about the sources of animals and their ages at the time of study would be useful within the main paper, even though more information will be available in the supplementary material. Second, it is not clear why only 14 pairs of animals were used for estimating the correlation of chimerism levels in microglia and macrophages. Is this lower than the total number of pairwise comparisons possible in order to avoid using non-independent samples? Some explanation would be helpful. Finally, I think more analysis of the consistency and variability of gene expression in microglia across different regions of the brain would be valuable. Are there genetic pathways expressed similarly in host and sibling microglia, regardless of region of the brain? Are there pathways that are consistently expressed differently in host vs sibling microglia regardless of brain region?

    1. Reviewer #2 (Public Review):

      In this study, Solyga and Keller use multimodal closed-loop paradigms in conjunction with multiphoton imaging of cortical responses to assess whether and how sensorimotor prediction errors in one modality influence the computation of prediction errors in another modality. Their work addresses an important open question pertaining to the relevance of non-hierarchical (lateral cortico-cortical) interactions in predictive processing within the neocortex.

      Specifically, they monitor GCaMP6f responses of layer 2/3 neurons in the auditory cortex of head-fixed mice engaged in VR paradigms where running is coupled to auditory, visual, or audio-visual sensory feedback. The authors find strong auditory and motor responses in the auditory cortex, as well as weak responses to visual stimuli. Further, in agreement with previous work, they find that the auditory cortex responds to audiomotor mismatches in a manner similar to that observed in visual cortex for visuomotor mismatches. Most importantly, while visuomotor mismatches by themselves do not trigger significant responses in the auditory cortex, simultaneous coupling of audio-visual inputs to movement non-linearly enhances mismatch responses in the auditory cortex.

      Their results thus suggest that prediction errors within a given sensory modality are non-trivially influenced by prediction errors from another modality. These findings are novel, interesting, and important, especially in the context of understanding the role of lateral cortico-cortical interactions and in outlining predictive processing as a general theory of cortical function.

      In its current form, the manuscript lacks sufficient description of methodological details pertaining to the closed-loop training and the overall experimental design. In several scenarios, while the results per se are convincing and interesting, their exact interpretation is challenging given the uncertainty about the actual experimental protocols (more on this below). Second, the authors are laser-focused on sensorimotor errors (mismatch responses) and focus almost exclusively on what happens when stimuli deviate from the animal's expectations.

      While the authors consistently report strong running-onset responses (during open-loop) in the auditory cortex in both auditory and visual versions of the task, they do not discuss their interpretation in the different task settings (see below), nor do they analyze how these responses change during closed-loop i.e. when predictions align with sensory evidence.

      However, I believe all my concerns can be easily addressed by additional analyses and incorporation of methodological details in the text.

      Major concerns:

      (1) Insufficient analysis of audiomotor mismatches in the auditory cortex:

      Lack of analysis of the dependence of audiomotor mismatches on the running speed: it would be helpful if the authors could clarify whether the observed audiomotor mismatch responses are just binary or scale with the degree of mismatch (i.e. running speed). Along the same lines, how should one interpret the lack of dependence of the playback halt responses on the running speed? Shouldn't we expect that during playback, the responses of mismatch neurons scale with the running speed?

      Slow temporal dynamics of audiomotor mismatches: despite the transient nature of the mismatches (1s), auditory mismatch responses last for several seconds. They appear significantly slower than previous reports for analogous visuomotor mismatches in V1 (by the same group, using the same methods) and even in comparison to the multimodal mismatches within this study (Figure 4C). What might explain this sustained activity? Is it due to a sustained change in the animal's running in response to the auditory mismatch?

      (2) Insufficient analysis and discussion of running onset responses during audiomotor sessions: The authors report strong running-onset responses during open-loop in identified mismatch neurons. They also highlight that these responses are in agreement with their model of subtractive prediction error, which relies on subtracting the bottom-up sensory evidence from top-down motor-related predictions. I agree, and, thus, assume that running-onset responses during the open loop in identified 'mismatch' neurons reflect the motor-related predictions of sensory input that the animal has learned to expect. If this is true, one would expect that such running-onset responses should dampen during closed-loop, when sensory evidence matches expectations and therefore cancels out this prediction. It would be nice if the authors test this explicitly by analyzing the running-related activity of the same neurons during closed-loop sessions.

      (3) Ambiguity in the interpretation of responses in visuomotor sessions.

      Unlike for auditory stimuli, the authors show that there are no obvious responses to visuomotor mismatches or playback halts in the auditory cortex. However, the interpretation of these results is somewhat complicated by the uncertainty related to the training history of these mice. Were these mice exclusively trained on the visuomotor version of the task or also on the auditory version? I could not find this info in the Methods. From the legend for Figure 4D, it appears that the same mice were trained on all versions of the task. Is this the case? If yes, what was the training sequence? Were the mice first trained on the auditory and then the visual version?

      The training history of the animals is important to outline the nature of the predictions and mismatch responses that one should expect to observe in the auditory cortex during visuomotor sessions. Depending on whether the mice in Figure 3 were trained on visual only or both visual and auditory tasks, the open-loop running onset responses may have different interpretations.

      a) If the mice were trained only on the visual task, how should one interpret the strong running onset responses in the auditory cortex? Are these sensorimotor predictions (presumably of visual stimuli) that are conveyed to the auditory cortex? If so, what may be their role?

      b) If the mice were also trained on the auditory version, then a potential explanation of the running-onset responses is that they are audiomotor predictions lingering from the previously learned sensorimotor coupling. In this case, one should expect that in the visual version of the task, these audiomotor predictions (within the auditory cortex) would not get canceled out even during the closed-loop periods. In other words, mismatch neurons should constantly be in an error state (more active) in the closed-loop visuomotor task. Is this the case?

      If so, how should one then interpret the lack of a 'visuomotor mismatch' aligned to the visual halts, over and above this background of continuous errors?<br /> As such, the manuscript would benefit from clearly stating in the main text the experimental conditions such as training history, and from discussing the relevant possible interpretations of the responses.

      (4) Ambiguity in the interpretation of responses in multimodal versus unimodal sessions.

      The authors show that multimodal (auditory + visual) mismatches trigger stronger responses than unimodal mismatches presented in isolation (auditory only or visual only). Further, they find that even though visual mismatches by themselves do not evoke a significant response, co-presentation of visual and auditory stimuli non-linearly augments the mismatch responses suggesting the presence of non-hierarchical interactions between various predictive processing streams.

      In my opinion, this is an important result, but its interpretation is nuanced given insufficient details about the experimental design. It appears that responses to unimodal mismatches are obtained from sessions in which only one stimulus is presented (unimodal closed-loop sessions). Is this actually the case? An alternative and perhaps cleaner experimental design would be to create unimodal mismatches within a multimodal closed-loop session while keeping the other stimulus still coupled to the movement.

      Given the current experiment design (if my assumption is correct), it is unclear if the multimodal potentiation of mismatch responses is a consequence of nonlinear interactions between prediction/error signals exchanged across visual and auditory modalities. Alternatively, could this result from providing visual stimuli (coupled or uncoupled to movement) on top of the auditory stimuli? If it is the latter, would the observed results still be evidence of non-hierarchical interactions between various predictive processing streams?

      Along the same lines, it would be interesting to analyze how the coupling of visual as well as auditory stimuli to movement influences responses in the auditory cortex in close-loop in comparison to auditory-only sessions. Also, do running onset responses change in open-loop in multimodal vs. unimodal playback sessions?

      Minor concerns and comments:

      (1) Rapid learning of audiomotor mismatches: It is interesting that auditory mismatches are present even on day 1 and do not appear to get stronger with learning (same on day 2). The authors comment that this could be because the coupling is learned rapidly (line 110). How does this compare to the rate at which visuomotor coupling is learned? Is this rapid learning also observable in the animal's behavior i.e. is there a change in running speed in response to the mismatch?

      (2) The authors should clarify whether the sound and running onset responses of the auditory mismatch neurons in Figure 2E were acquired during open-loop. This is most likely the case, but explicitly stating it would be helpful.

      (3) In lines 87-88, the authors state 'Visual responses also appeared overall similar but with a small increase in strength during running ...'. This statement would benefit from clarification. From Figure S1 it appears that when the animal is sitting there are no visual responses in the auditory cortex. But when the animal is moving, small positive responses are present. Are these actually 'visual' responses - perhaps a visual prediction sent from the visual cortex to the auditory cortex that is gated by movement? If so, are they modulated by features of visual stimuli eg. contrast, intensity? Or, do these responses simply reflect motor-related activity (running)? Would they be present to the same extent in the same neurons even in the dark?

      (4) The authors comment in the text (lines 106-107) about cessation of sound amplitude during audiomotor mismatches as being analogous to halting of visual flow in visuomotor mismatches. However, sound amplitude versus visual flow are quite different in nature. In the visuomotor paradigm, the amount of visual stimulation (photons per unit time) does not necessarily change systematically with running speed. Whereas, in the audiomotor paradigm, the SNR of the stimulus itself changes with running speed which may impact the accuracy of predictions. On a broader note, under natural settings, while the visual flow is coupled to movement, sound amplitude may vary more idiosyncratically with movement.

      Perhaps such differences might explain why unlike in the case of visual cortex experiments, running speed does not affect the strength of playback responses in the auditory cortex.

    1. Reviewer #3 (Public Review):

      These studies reveal an S-phase requirement for the PARG dePARylation enzyme in removing ADP-ribosylation from PAR-modified proteins whose PARylation is promoted by the presence of unligated Okazaki fragments. The excessive protein ADP-ribosylation observed in S-phase of PARG-depleted human cells leads to trapping of the PARP1 ADP-ribosylation enzyme on chromatin. The findings would be strengthened by identification of the relevant ADP-ribosylation substrates of PARG whose dePARylation is needed for progression through S-phase.

      Comments on revised version:

      In the revised version the authors have addressed some of the reviewers' concerns, but, despite the new explanatory paragraph on page 16, the paper remains confusing because as shown in Figure 7 at the end of the Results the PARG KO 293A cells that were analyzed at the beginning of the Results are not true PARG knockouts. The authors stated that they did not rewrite the Results because they wanted to describe the experiments in the order in which they were carried out, but there is no imperative for the experiments to be described in the order in which they were done, and it would be much easier for the uninitiated reader to appreciate the significance of these studies if the true PARG KO cell data were presented at the beginning, as all three of the original reviewers proposed.

      While the authors have to some extent clarified the nature of the PARG KO alleles, they have not been able to identify the source of the residual PARG activity in the PARG KO cells, in part because different commercial PARG antibodies give different and conflicting immunoblotting results. Additional sequence characterization of PARG mRNAs expressed in the PARG cKO cells, and also in-depth proteomic analysis of the different PARG bands could provide further insight into the origins and molecular identities of the various PARG proteins expressed from the different KO PARG alleles, and determine which of them might retain catalytic activity.

      The authors have made no progress in identifying which are the key PARG substrates required for S phase progression, although they suggest that PARP1 itself may be an important target.

    1. Reviewer #2 (Public Review):

      The authors aimed to understand how epistasis influences the genetic architecture of the DNA-binding domain (DBD) of steroid hormone receptor. An ordinal regression model was developed in this study to analyze a published deep mutational scanning dataset that consists of all combinatorial amino acid variants across four positions (i.e. 160,000 variants). This published dataset measured the binding of each variant to the estrogen receptor response element (ERE, sequence: AGGTCA) as well as the steroid receptor response element (SRE, sequence: AGAACA). This model has major strengths of being reference free and able to account for global nonlinearity in the genotype-phenotype relationship. Thorough analyses of the modelling results have performed, which provided convincing results to support the importance of epistasis in promoting evolution of protein functions. This conclusion is impactful because many previous studies have shown that epistasis constrains evolution. The novelty this study will likely stimulate new ideas in the field. The model will also likely be utilized by other groups in the community.

    1. Reviewer #2 (Public Review):

      Summary:

      In this manuscript, the authors revealed that genetic deficiencies of ACK1 and BRK are associated with human SLE. First, the authors found that compound heterozygous deleterious variants in the kinase domains of the non-receptor tyrosine kinases (NRTK) TNK2/ACK1 in one multiplex family and PTK6/BRK in another family. Then, by an experimental blockade of ACK1 or BRK in a mouse SLE model, they found an increase in glomerular IgG deposits and circulating autoantibodies. Furthermore, they reported that ACK and BRK variants from the SLE patients impaired the MERTK-mediated anti-inflammatory response to apoptotic cells in human induced pluripotent stem cells (hiPSC)-derived macrophages. This work identified new SLE-associated ACK and BRK variants and a role for the NRTK TNK2/ACK1 and PTK6/BRK in efferocytosis, providing a new molecular and cellular mechanism of SLE pathogenesis.

      Strengths:

      This work identified new SLE-associated ACK and BRK variants and a role for the NRTK TNK2/ACK1 and PTK6/BRK in efferocytosis, providing a new molecular and cellular mechanism of SLE pathogenesis.

      Weaknesses:

      Although the manuscript is well-organized and clearly stated, there are some points below that should be considered:

      * In this study, the authors used forward genetic analyses to identify novel gene mutations that may cause SLE, combined with GWAS studies of SLE. To further explore the importance of these variants, haplotype analysis of two candidate genes could be performed, to observe the evolution and selection relationship of candidate genes in the population (UK 1000 biobank, for example).

      * Although the authors focused on SLE and macrophage efferocytosis in their studies, direct evidence of how macrophage efferocytosis significantly affects SLE is lacking. This point should at least be explicitly introduced and discussed by citing appropriate literature.

      * It is still not clear how the target molecules identified in this paper may influence macrophage efferocytosis. More direct evidence should be established.

      * For some transcriptional repressors mentioned in their studies, the authors should check whether there is clear experimental evidence. If not, it is recommended to supplement the experimental verifications for clarity.

      * In Figures 4C and 4D, it is seen that the usage of inhibitors causes cytoskeletal changes, however this reviewer would not have expected such large change. Did the authors check whether the cells die after heavy treatment by the inhibitors?

    1. Reviewer #2 (Public Review):

      Summary:

      mRNA translation regulation permits cells to rapidly adapt to diverse stimuli by fine-tuning gene expression. Specifically, the 13-subunit eukaryotic initiation factor 3 (eIF3) complex is critical for translation initiation as it aids in 48S PIC assembly to allow for ribosome scanning. In addition, eIF3 has been shown to drive transcript-specific translation by binding mRNA 5' cap structures through the eIF3d subunit. Dysregulation of eIF3 has been implicated in oncogenesis, however the precise eIF3 subunit contributions are unclear. Here, Herrmannová et al. aim to investigate how eIF3 subcomplexes, generated by knockdown (KD) of either eIF3e, eIF3d, or eIF3h, affect the global translatome. Using Ribo-seq and RNA-seq, the authors identified a large number of genes that exhibit altered translation efficiency upon eIF3d/e KD, while translation defects upon eIF3h KD were mild. eIF3d/e KD share multiple dysregulated transcripts, perhaps due to both subcomplexes lacking eIF3d. Both eIF3d/e KD increase the translation efficiency (TE) of transcripts encoding lysosomal, ER, and ribosomal proteins. This suggests a role of eIF3 in ribosome biogenesis and protein quality control. Many transcripts encoding ribosomal proteins harbor a TOP motif, and eIF3d KD and eIF3e KD cells exhibit a striking induction of these TOP-modified transcripts. On the other hand, eIF3d KD and eIF3e KD lead to a reduction of MAPK/ERK pathway proteins. Despite this downregulation, eIF3d KD and eIF3e KD activate MAPK/ERK signaling as ERK1/2 and c-Jun phosphorylation were induced. Finally, in all three knockdowns, MDM2 and ATF4 protein levels are reduced. This is notable because MDM2 and ATF4 both contain short uORFs upstream of the start codon, and further support a role of eIF3 in reinitiation. Altogether, Herrmannová et al. have gained key insights into precise eIF3-mediated translational control as it relates to key signaling pathways implicated in cancer.

      Strengths:

      The authors have provided a comprehensive set of data to analyze RNA and ribosome footprinting upon perturbation of eIF3d, eIF3e, and eIF3h. As described above in the summary, these data present many interesting starting points for understanding additional roles of the eIF3 complex and specific subunits in translational control.

      Weaknesses:

      - The differences between eIF3e and eIF3d knockdown are difficult to reconcile, especially since eIF3e knockdown leads to a reduction in eIF3d levels.

      - The paper would be strengthened by experiments directly testing what RNA determinants allow for transcript-specific translation regulation by the eIF3 complex. This would allow the paper to be less descriptive.

      - The paper would have more biological relevance if eIF3 subunits were perturbed to mimic naturally occurring situations where eIF3 is dysregulated. For example, eIF3e is aberrantly upregulated in certain cancers, and therefore an overexpression and profiling experiment would have been more relevant than a knockdown experiment.

    1. Reviewer #2 (Public Review):

      In the manuscript, the authors aimed to elucidate the molecular mechanism that explains neurodegeneration caused by the depletion of axonal mitochondria. In Drosophila, starting with siRNA depletion of Milton and Miro, the authors attempted to demonstrate that the depletion of axonal mitochondria induces the defect in autophagy. From proteome analyses, the authors hypothesized that autophagy is impacted by the abundance of eIF2β and the phosphorylation of eIF2α. The authors followed up the proteome analyses by testing the effects of eIF2β overexpression and depletion on autophagy. With the results from those experiments, the authors proposed a novel role of eIF2β in proteostasis that underlies neurodegeneration derived from the depletion of axonal mitochondria.

      The manuscript has several weaknesses. The reader should take extra care while reading this manuscript and when acknowledging the findings and the model in this manuscript.

      The defect in autophagy by the depletion of axonal mitochondria is one of the main claims in the paper. The authors should work more on describing their results of LC3-II/LC3-I ratio, as there are multiple ways to interpret the LC3 blotting for the autophagy assessment. Lysosomal defects result in the accumulation of LC3-II thus the LC3-II/LC3-I ratio gets higher. On the other hand, the defect in the early steps of autophagosome formation could result in a lower LC3-II/LC3-I ratio. From the results of the actual blotting, the LC3-I abundance is the source of the major difference for all conditions (Milton RNAi and eIF2β overexpression and depletion). In the text, the authors simply state the observation of their LC3 blotting. The manuscript lacks an explanation of how to evaluate the LC3-II/LC3-I ratio. Also, the manuscript lacks an elaboration on what the results of the LC3 blotting indicate about the state of autophagy by the depletion of axonal mitochondria.

      Another main point of the paper is the up-regulation of eIF2β by depleting the axonal mitochondria leads to the proteostasis crisis. This claim is formed by the findings from the proteome analyses. The authors should have presented their proteomic data with much thorough presentation and explanation. As in the experiment scheme shown in Figure 4A, the author did two proteome analyses: one from the 7-day-old sample and the other from the 21-day-old sample. The manuscript only shows a plot of the result from the 7-day-old sample, but that of the result from the 21-day-old sample. For the 21-day-old sample, the authors only provided data in the supplemental table, in which the abundance ratio of eIF2β from the 21-day-old sample is 0.753, meaning eIF2β is depleted in the 21-day-old sample. The authors should have explained the impact of the eIF2β depletion in the 21-day-old sample, so the reader could fully understand the authors' interpretation of the role of eIF2β on proteostasis.

      The manuscript consists of several weaknesses in its data and explanation regarding translation.

      (1) The authors are likely misunderstanding the effect of phosphorylation of eIF2α on translation. The P-eIF2α is inhibitory for translation initiation. However, the authors seem to be mistaken that the down-regulation of P-eIF2α inhibits translation.

      (2) The result of polysome profiling in Figure 4H is implausible. By 10%-25% sucrose density gradient, polysomes are not expected to be observed. The authors should have used a gradient with much denser sucrose, such as 10-50%.

      (3) Also on the polysome profiling, as in the method section, the authors seemed to fractionate ultra-centrifuged samples from top to bottom and then measured A260 by a plate reader. In that case, the authors should have provided a line plot with individual data points, not the smoothly connected ones in the manuscript.

      (4) For both the results from polysome profiling and puromycin incorporation (Figure 4H and I), the difference between control siRNA and Milton siRNA are subtle, if not nonexistent. This might arise from the lack of spatial resolution in their experiment as the authors used head lysate for these data but the ratio of Phospho-eIF2α/eIF2α only changes in the axons, based on their results in Figure 4E-G. The authors could have attempted to capture the spatial resolution for the axonal translation to see the difference between control siRNA and Milton siRNA.

    1. Reviewer #2 (Public Review):

      Summary:

      The manuscript by Han et al and Cordes is a tour-de-force effort to distinguish between induced fit and conformational selection in glutamine binding protein (GlnBP). It is important to say that I don't agree that a decision needs to be made between these two limiting possibilities in the sense that whether a minor population can be observed depends on the experiment and the energy difference between the states. That said, the authors make an important distinction which is that it is not sufficient to observe both states in the ligand-free solution because it is likely that the ligand will not bind to the already closed state. The ligand binds to the open state and the question then is whether the ligand sufficiently changes the energy of the open state to effectively cause it to close. The authors point out that this question requires both a kinetic and a thermodynamic answer. Their "method" combines isothermal titration calorimetry, single-molecule FRET including key results from multi-parameter photon-by-photon hidden Markov modelling (mpH2MM), and SPR. The authors present this "method" of combination of experiments as an approach to definitively differentiate between induced fit and conformational selection. I applaud the rigor with which they perform all of the experiments and agree that others who want to understand the exact mechanism of protein conformational changes connected to ligand binding need to do such a multitude of different experiments to fully characterize the process. However, the situation of GlnBP is somewhat unique in the high affinity of the Gln (slow off-rate) as compared to many small molecule binding situations such as enzyme-substrate complexes. It is therefore not surprising that the kinetics result in an induced fit situation. In the case of the E-S complexes I am familiar with, the dissociation is much more rapid because the substrate binding affinity is in the micromolar range and therefore the re-equilibration of the apo state is much faster. In this case, the rate of closing and opening doesn't change much whether ligand is present or not. Here, of course, once the ligand is bound the re-equilibration is slow. Therefore, I am not sure if the conclusions based on this single protein are transferrable to most other protein-small molecule systems. I am also not sure if they are transferrable to protein-protein systems where both molecules the ligand and the receptor are expected to have multiscale dynamics that change upon binding.

      Strengths:

      The authors provide beautiful ITC data and smFRET data to explore the conformational changes that occur upon Gln binding. Figure 3D and Figure 4 (mpH2MM data) provide the really critical data. The multi-parameter photon-by-photon hidden Markov modelling (mpH2MM) data. In the presence of glutamine concentrations near the Kd, two FRET-active sub-populations are identified that appear to interconvert on timescales slower than 10 ms. They then do a whole bunch of control experiments to look for faster dynamics (Figure 5). They also do TIRF smFRET to try to compare their results to those of previous publications. Here, they find several artifacts are occurring including inactivation of ~50% of the proteins. They also perform SPR experiments to measure the association rate of Gln and obtain expectedly rapid association rates on the order of 10^8 M-1s-1.

      Weaknesses:

      Looking at the traces presented in the supplementary figures, one can see that several of the traces have more than one molecule present. The authors should make sure that they use only traces with a single photobleaching event for each fluorophore. One can see steps in some of the green traces that indicate two green fluorophors (likely from 2 different molecules) in the traces. This is one of the frequent problems with TIRF smFRET with proteins, that only some of the spots represent single molecules and the rest need to be filtered out of the analysis.

      The NMR experiments that the authors cite are not in disagreement with the work presented here. NMR is capable of detecting "invisible states" that occur in 1-5% of the population. SmFRET is not capable of detecting these very minor states. I am quite sure that if NMR spectroscopists could add very high concentrations of Gln they would also see a conversion to the closed population.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors have analyzed ethnogeographic differences in the comorbidity factors, such as diabetes and heart disease, for the incidences of stroke and whether it leads to mortality.

      Strengths:<br /> The idea is interesting and the data are compelling. The results are technically solid.

      The authors identify specific genetic loci that increase the risk of a stroke and how they differ by region.

      Weaknesses:

      The presentation is not focused. It would be better to include p-values and focus presentation on the main effects of the dataset analysis.

    1. Reviewer #2 (Public Review):

      Summary:

      The results from this study demonstrated a cell-specific role of mitochondrial enzyme arginase-II (Arg-II) in heart aging and revealed a non-cell-autonomous effect of Arg-II on cardiomyocytes, fibroblasts, and endothelial cells through the crosstalk with macrophages via inflammatory factors, such as by IL-1, as well as a cell-autonomous effect of Arg-II through mtROS in fibroblasts contributing to cardiac aging phenotype. These findings highlight the significance of non-cardiomyocytes in the heart and bring new insights into the understanding of pathologies of cardiac aging. It also provides new evidence for the development of therapeutic strategies, such as targeting the ArgII activation in macrophages.

      Strengths:

      This study targets an important clinical challenge, and the results are interesting and innovative. The experimental design is rigorous, the results are solid, and the representation is clear. The conclusion is logical and justified.

      Weaknesses:

      The discussion could be extended a little bit to improve the realm of the knowledge related to this study.

    1. Reviewer #2 (Public Review):

      Summary:

      Semenova et. al., performed a cross-sectional analysis of host immunophenotypes (using flow cytometry) and the peripheral CD4+ T cell HIV reservoir size (using the Intact Proviral DNA Assay, IPDA) from 115 people with HIV (PWH) on ART. The study mostly highlights the machine learning methods applied to these host and viral reservoir datasets but fails to interpret these complex analyses into (clinically, biologically) interpretable findings. For these reasons, the direct translational take-home message from this work is lost amidst a large list of findings (shown as clusters of associated markers) and sentences such as "this study highlights the utility of machine learning approaches to identify otherwise imperceptible global patterns" - lead to overinterpretation of their data.

      Strengths:

      Measurement of host immunophenotyping measures (multiparameter flow cytometry) and peripheral HIV reservoir size (IPDA) from 115 PWH on ART.

      Major Weaknesses:

      (1) Overall, there is little to no interpretability of their machine learning analyses; findings appear as a "laundry list" of parameters with no interpretation of the estimated effect size and directionality of the observed associations. For example, Figure 2 might actually give an interpretation of each X increase in immunophenotyping parameter, we saw a Y increase/decrease in HIV reservoir measure.

      (2) The correlations all appear to be relatively weak, with most Spearman R in the 0.30 range or so.

      (3) The Discussion needs further work to help guide the reader. The sentence: "The correlative results from this present study corroborate many of these studies, and provide additional insights" is broad. The authors should spend some time here to clearly describe the prior literature (e.g., describe the strength and direction of the association observed in prior work linking PD-1 and HIV reservoir size, as well as specify which type of HIV reservoir measures were analyzed in these earlier studies, etc.) and how the current findings add to or are in contrast to those prior findings.

      (4) The most interesting finding is buried on page 12 in the Discussion: "Uniquely, however, CD127 expression on CD4 T cells was significantly inversely associated with intact reservoir frequency." The authors should highlight this in the abstract, and title, and move this up in the Discussion. The paper describes a very high dimensional analysis and the key takeaways are not clear; the more the author can point the reader to the take-home points, the better their findings can have translatability to future follow-up mechanistic and/or validation studies.

      (5) The authors should avoid overinterpretation of these results. For example in the Discussion on page 13 "The existence of two distinct clusters of PWH with different immune features and reservoir characteristics could have important implications for HIV cure strategies - these two groups may respond differently to a given approach, and cluster membership may need to be considered to optimize a given strategy." It is highly unlikely that future studies will be performing the breadth of parameters resulting here and then use these directly for optimizing therapy.

      (6) There are only TWO limitations listed here: cross-sectional study design and the use of peripheral blood samples. (The subsequent paragraph notes an additional weakness which is misclassification of intact sequences by IPDA). This is a very limited discussion and highlights the need to more critically evaluate their study for potential weaknesses.

      (7) A major clinical predictor of HIV reservoir size and decay is the timing of ART initiation. The authors should include these (as well as other clinical covariate data - see #12 below) in their analyses and/or describe as limitations of their study.

    1. Reviewer #2 (Public Review):

      Summary:

      Zeng et al investigate in an observational population-based cohort study whether the use of proton pump inhibitors (PPIs) is associated with an increased risk of several respiratory infections among which are influenza, pneumonia, and COVID-19. They conclude that compared to non-users, people regularly taking PPIs have increased susceptibility to influenza, pneumonia, as well as COVID-19 severity and mortality. By performing several different statistical analyses, they try to reduce bias as much as possible, to end up with robust estimates of the association.

      Strengths:

      The study comprehensively adjusts for a variety of critical covariates and by using different statistical analyses, including propensity-score-matched analyses and quantitative bias analysis, the estimates of the associations can be considered robust.

      Weaknesses:

      As it is an observational cohort study there still might be bias. Information on the dose or duration of acid suppressant use was not available, but might be of influence on the results. The outcome of interest was obtained from primary care data, suggesting that only infections as diagnosed by a physician are taken into account. Due to the self-limiting nature of the outcome, differences in health-seeking behavior might affect the results.

    1. Reviewer #2 (Public Review):

      This manuscript focused on why aging leads to decreased beiging of white adipose tissue. The authors used an inducible lineage tracing system and provided in vivo evidence that de novo beige adipogenesis from Pdgfra+ adipocyte progenitor cells is blocked during early aging in subcutaneous fat. Single-cell RNA sequencing of adipocyte progenitor cells and in vitro assays showed that these cells have similar beige adipogenic capacities in vitro. Single-cell nucleus RNA sequencing of mature adipocytes indicated that aged mice have more Npr3 high-expressing adipocytes in the subcutaneous fat from aged mice. Meanwhile, adipocytes from aged mice have significantly lower expression of genes involved in de novo lipogenesis, which may contribute to the declined beige adipogenesis.

      The mechanism that leads to age-related impairment of white adipose tissue beiging is not very clear. The finding that Pdgfra+ adipocyte progenitor cells contribute to beige adipogenesis is novel and interesting. It is more intriguing that the aging process represses Pdgfra+ adipocyte progenitor cells from differentiating into beige adipocytes during cold stimulation. Mature adipocytes that have high de novo lipogenesis activity may support beige adipogenesis is also novel and worth further pursuing. The study was carried out with a nice experimental design, and the authors provided sufficient data to support the major conclusions. I only have a few comments that could potentially improve the manuscript.

      (1) It is interesting that after three days of cold exposure, aged mice also have much fewer beige adipocytes. Is de novo adipogenesis involved at this early stage? Or does the previous beige adipocyte that acquired white morphology have a better "reactivation" in young mice? It would be nice if the author could discuss the possibilities.

      (2) Is the absolute number of Pdgfra+ cells decreased in aged mice? It would be nice to include quantifications of the percentage of tomato+ beige adipocytes in total tomato+ cells to reflect the adipogenic rate.

    1. Reviewer #2 (Public Review):

      Summary:

      In this work, Hu and colleagues investigate telomerase-independent survival in Saccharomyces cerevisiae strains engineered to have different chromosome numbers. The authors describe the molecular patterns of survival that change with fewer chromosomes and that differ from the well-described canonical Type I and Type II, including chromosome circularization and other atypical outcomes. They then take advantage of the strain with 3 chromosomes to examine the effect of deleting all the subtelomeric elements, called X and Y'. For most of the tested phenotypes, they find no significant effect of the absence of X- and Y'-element, and show that they are not essential for survivor formation. They speculate that X- and Y'-elements are remnants of ancient telomere maintenance mechanisms.

      Strengths:

      This work advances our understanding of the telomerase-independent strategies available to the cell by altering the structure of the genome and of the subtelomeres, a feat that was enabled by the set of strains they engineered previously. By using strains with non-standard genome structures, several alternative survival mechanisms are uncovered, revealing the diversity and plasticity of telomere maintenance mechanisms. Overall, the conclusions are well supported by the data, with adequate sample sizes for investigating survivors. The assessment of the genetic requirements for survivors in strains with different chromosome numbers greatly improved the quality of this work. The molecular analyses based on Southern blots are also very well-conducted.

      Weaknesses:

      The authors discovered alternative telomerase-independent survival strategies beyond the well-described type I and II (including circularization, type X and atypical, as they called them) at play in the context of reduced number of chromosomes. Their work provides a molecular and a partial genetic characterization of these survival pathways. A more thorough analysis of the frequency of each type of survivors and their genetic requirements would have advanced our understanding or the diversity of survival strategies in the absence of telomerase. However, as noted by the authors, the quantification of the rate of emergence of survivors (and their subtypes) is very difficult to achieve. This comment is therefore not meant as a criticism but rather as a perspective on exciting future research avenues.

    1. Reviewer #2 (Public Review):

      Summary:

      The article by Waleed et al discusses the self organization of actin cytoskeleton using the theory of active nematics. Linear stability analysis of the governing equations and computer simulations show that the system is unstable to density fluctuations and self organized structures can emerge. While the context is interesting, I am not sure whether the physics is new. Hence I have reservations about recommending this article.

      Strengths:

      (i) Analytical calculations complemented with simulations (ii) Theory for cytoskeletal network

      Weaknesses:

      Not placed in the context or literature on active nematics.

    1. Reviewer #2 (Public Review):

      Summary:

      The investigators apply scRNA seq and bioinformatics to identify biomarkers associated with DNFB-induced contact dermatitis in mice. The bioinformatics component of the study appears reasonable and may provide new insights regarding TH1-driven immune reactions in ACD in mice. However, the IF data and images of tissue sections are not clear and should be improved to validate the model.

      Strengths:

      The bioinformatics analysis.

      Weaknesses:

      The IF data presented in 4H, 6H, 7E and 7F are not convincing and need to be correlated with routine staining on histology and different IF markers for PDGFR. Some of the IF staining data demonstrates a pattern inconsistent with its target.

    1. Reviewer #2 (Public Review):

      In the manuscript "Full-length direct RNA sequencing uncovers stress-granule dependent RNA decay upon cellular stress", Dar, Malla, and colleagues use direct RNA sequencing on nanopores to characterize the transcriptome after arsenite and oxidative stress. They observe a population of transcripts that are shortened during stress. The authors hypothesize that this shortening is mediated by the 5'-3' exonuclease XRN1, as XRN1 knockdown results in longer transcripts. Interestingly, the authors do not observe a polyA-tail shortening, which is typically thought to precede decapping and XRN1-mediated transcript decay. Finally, the authors use G3BP1 knockout cells to demonstrate that stress granule formation is required for the observed transcript shortening.

      The manuscript contains intriguing findings of interest to the mRNA decay community. That said, it appears that the authors at times overinterpret the data they get from a handful of direct RNA sequencing experiments. To bolster some of the statements additional experiments might be desirable.

      A selection of comments:

      (1) Considering that the authors compare the effects of stress, stress granule formation, and XRN1 loss on transcriptome profiles, it would be desirable to use a single-cell system (and validated in a few more). Most of the direct RNAseq is performed in HeLa cells, but the experiments showing that stress granule formation is required come from U2OS cells, while short RNAseq data showing loss of coverage on mRNA 5'ends is reanalyzed from HEK293 cells. It may be plausible that the same pathways operate in all those cells, but it is not rigorously demonstrated.

      (2) An interesting finding of the manuscript is that polyA tail shortening is not observed prior to transcript shortening. The authors would need to demonstrate that their approach is capable of detecting shortened polyA tails. Using polyA purified RNA to look at the status of polyA tail length may not be ideal (as avidity to oligodT beads may increase with polyA tail length and therefore the authors bias themselves to longer tails anyway). At the very least, the use of positive controls would be desirable; e.g. knockdown of CCR4/NOT.

      (3) The authors use a strategy of ligating an adapter to 5' phosphorylated RNA (presumably the breakdown fragments) to be able to distinguish true mRNA fragments from artifacts of abortive nanopore sequencing. This is a fantastic approach to curating a clean dataset. Unfortunately, the authors don't appear to go through with discarding fragments that are not adapter-ligated (presumably to increase the depth of analysis; they do offer Figure 1e that shows similar changes in transcript length for fragments with adapter, compared to Figure 1d). It would be good to know how many reads in total had the adapter. Furthermore, it would be good to know what percentage of reads without adapters are products of abortive sequencing. What percentage of reads had 5'OH ends (could be answered by ligating a different adapter to kinase-treated transcripts). More read curation would also be desirable when building the metagene analysis - why do the authors include every 3'end of sequenced reads (their RNA purification scheme requires a polyA tail, so non-polyadenylated fragments are recovered in a non-quantitative manner and should be discarded).

      (4) The authors should come to a clear conclusion about what "transcript shortening" means. Is it exonucleolytic shortening from the 5'end? They cannot say much about the 3'ends anyway (see above). Or are we talking about endonucleolytic cuts leaving 5'P that then can be attached by XRN1 (again, what is the ratio of 5'P and 5'OH fragments; also, what is the ratio of shortened to full-length RNA)?

      (5) The authors should clearly explain how they think the transcript shortening comes about. They claim it does not need polyA shortening, but then do not explain where the XRN1 substrate comes from. Does their effect require decapping? Or endonucleolytic attacks?

      (6) XRN1 KD results in lengthened transcripts. That is not surprising as XRN1 is an exonuclease - and XRN1 does not merely rescue arsenite stress-mediated transcript shortening, but results in a dramatic transcript lengthening.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors set out to establish the role of the rice LEC1 homolog OsNF-YB7 in embryo development, especially as it pertains to the development of photosynthetic capacity, with chlorophyll production as a primary focus.

      Strengths:

      The results are well-supported and each approach used complements each other. There are no major questions left unanswered and the central hypothesis is addressed in every figure.

      Weaknesses:

      There are a handful of sections that could use clarifying for readers, but overall this is a solidly composed manuscript.

      The authors clearly achieved their aims; the results compellingly establish a disparity between how this system operates in rice and Arabidopsis. Conclusions are thoroughly supported by the provided data and interpretations. This work will force a reconsideration of the value of Arabidopsis as a model organism for embryo chlorophyll biosynthesis and possibly photosynthesis during embryo maturation more broadly, as rice is a major crop organism and it very clearly does not follow the Arabidopsis model. It will thus be useful to carry out similar tests in other organisms rather than relying on Arabidopsis and attempting to more fully establish the regulatory mechanism in rice.

    1. Reviewer #2 (Public Review):

      Summary:

      In this work, Song et al. propose a locus-based framework for performing GWAS and related downstream analyses including finemapping and polygenic risk score (PRS) estimation. GWAS are not sufficiently powered to detect phenotype associations with low-frequency variants. To overcome this limitation, the manuscript proposes a method to aggregate variant impacts on chromatin and transcription across a 4096 base pair (bp) loci in the form of a haplotype function score (HFS). At each locus, an association is computed between the HFS and trait. Computing associations at the level of imputed functional genomic scores enables integration of information across variants spanning the allele frequency spectrum and bolster the power of GWAS.

      The HFS for each locus is derived from a sequence-based predictive model - Sei. Sei predicts 21,907 chromatin and TF binding tracks, which can be projected onto 40 pre-defined sequence classes ( representing promoters, enhancers etc.). For each 4096 bp haplotype in their UKB cohort, the proposed method uses the Sei sequence class scores to derive the haplotype function score (HFS). The authors apply their method to 14 polygenic traits, identifying ~16,500 HFS-trait associations. They finemap these trait-associated loci with SuSie, as well perform target gene/pathway discovery and PRS estimation.

      Strengths:

      Sequence-based deep learning predictors of chromatin status and TF binding have become increasingly accurate over the past few years. Imputing aggregated variant impact using Sei, and then performing an HFS-trait association is therefore an interesting approach to bolster power in GWAS discovery. The manuscript demonstrates that region-level associations can be identified at the level of an aggregated functional score using sequence-based deep learning models. The finemapping and pathway identification analyses suggest that HFS-based associations identify relevant causal pathways and genes from an association study. Identifying associations at the level of functional genomics increases portability of PRSs across populations. Imputing functional genomic predictions using a sequence-based deep learning model does not suffer from the limitation of TWAS where gene expression is imputed from a limited size reference panel such as GTEx and is an interesting direction to bolster discovery power.

      However, a few limitations to this method in its current form are:

      (1) HFS-based association is going to miss coding variation as well as noncoding regulatory variants such as splicing variants/polyadenylation variants which are not modeled by Sei. This will lead to false negatives in the HFS-based association and additionally false negatives + associated false positives in the finemapping. Going forward, it'll therefore be important to characterize how this influences the genome-wide finemapping.

      (2) Sei predicts chromatin status / ChIP-seq peaks in the center of a 4kb region. It is thus not clear therefore whether the functional effects of variants not in the center of the 4kb region would be captured in a single Sei score. It also remains unclear how much the choice of window affects the association tests / finemapping.

      (3) There are going to be cases where there's an association driven by a variant that is correlated with a Sei prediction in a neighboring window. These would represent false positives for the method, it would be useful to identify or characterize these cases.

      Minor Concerns:<br /> (1) Sequence based deep learning model predictions can be miscalibrated for insertions and deletions (INDELs) as compared to SNPs. It'll be important to note that model INDEL scores may not be calibrated, which might also lead to false positives / false negatives in the finemapping.

    1. Reviewer #2 (Public Review):

      In this manuscript, Yao et al. present a series of experiments aiming at generating a cellular atlas of the human hippocampus across aging, and how it may be affected by injury, in particular, stroke. Although the aim of the study is interesting and relevant for a larger audience, due to the ongoing controversy around the existence of adult hippocampal neurogenesis in humans, a number or technical weaknesses result in a poor support for many of the conclusions made from the results of these experiments.<br /> In particular, a recent meta analysis of five previous studies applying similar techniques to human samples has identified different aspects of sample size as main determinants of the statistical power needed to make significant conclusions. Some of this aspects are the number of nuclei sequenced and subject stratification. These two aspects are of concern in Yao's study. First, the number of sequenced nuclei is lower than the calculated numbers of nuclei required for detecting rare cell types. However, Yao et al. report succeeding in detecting rare populations, including several types of neural stem cells in different proliferation states, which have been demonstrated to be extremely scarce by previous studies. It would be very interesting to read how the authors interpret these differences. Secondly, the number of donors included in some of the groups is extremely low (n=1) and the miscellaneous information provided about the donors is practically inexistent. As individual factors such as chronic conditions, medication, lifestyle parameters, etc... are considered determinant for the variability of adult hippocampal neurogenesis levels across individuals, this represents a series limitation of the current study. Overall, several technical weaknesses severely limit the relevance of this study and the ability of the authors to achieve their experimental aims.

      After a first review round, the manuscript is still lacking a clear discussion of its several technical limitations, which will help the audience to grasp the relevance of the findings. In particular, detailed information about individual patients health status and relevant lifestyle parameters that may have affected it is lacking. The authors make the point themselves that the discrepancies among studies might be caused by health state differences across hippocampi, which subsequently lead to different degrees of hippocampal neurogenesis." So, even in the authors own interpretation this is a serious limitation to the manuscript, that however out of the authors control, impacts on the quality of their findings.

    1. Reviewer #2 (Public Review):

      Summary:

      In this study, Ghafari et al. explored the correlation between hemispheric asymmetry in the volume of various subcortical regions and lateralization of posterior alpha band oscillations in a spatial attention task with varying cognitive demands. To this end, they combined structural MRI and task MEG to investigate the relationship between hemispheric differences in volume of basal ganglia, thalamus, hippocampus and amygdala and hemisphere-specific modulation of alpha-band power. The authors report that differences in the thalamus, caudate nucleus and globus pallidus volume are linked to the attention-related changes in alpha band oscillations with differential correlations for different regions in different conditions of the design (depending on the salience of the distractor and/or the target).

      The manuscript contributes to filling an important gap in current research on attention allocation which commonly focuses exclusively on cortical structures. Because it is not possible to reliably measure subcortical activity with non-invasive electrophysiological methods, they correlate volumetric measurements of the relevant subcortical regions with cortical measurements of alpha band power. Specifically, they build on their own previous finding showing a correlation between hemispheric asymmetry of basal ganglia volumes and alpha lateralization by assessing a task without an explicit reward component. Furthermore, the authors use differences in saliency and perceptual load to disentangle the individual contributions of the subcortical regions. These remain somewhat hard to interpret, given their post hoc nature, and the lack of statistical power to compare task demand effects directly, but the results raise interesting new hypotheses for future work.

    1. Reviewer #2 (Public Review):

      Summary:

      This study investigates the neural substrates of syntax variation in Bengalese finch song. Here, the authors tested the effects of bilateral lesions of mMAN, a brain area with inputs to HVC, a premotor area required for song production. Lesions in mMAN induce variability in syntactic elements of song specifically through increased transition entropy, variability within stereotyped song elements known as chunks and increases in the repeat number of individual syllables. These results suggest that mMAN projections to HVC contribute to multiple aspects of song syntax in the Bengalese finch. Overall the experiments are well-designed, the analysis excellent, and the results are of high interest.

      Strengths:

      The study identifies a novel role for mMAN, medial magnocellular nucleus of the anterior nidopallium, in the control of syntactic variation within adult Bengalese finch song. This is of particular interest as multiple studies previously demonstrated that mMAN lesions to do not effect song structure in zebra finches. The study undertakes a thorough analysis to characterise specific aspects of variability within the song of lesioned animals. The conclusions are well supported by the data.

    1. Reviewer #2 (Public Review):

      Summary:

      In this manuscript, L&S investigates the important general question of how humans achieve invariant behavior over stimuli belonging to one category given the widely varying input representation of those stimuli and more specifically, how they do that in arbitrary abstract domains. The authors start with the hypothesis that this is achieved by invariance transformations that observers use for interpreting different entries and furthermore, that these transformations in an arbitrary domain emerge with the help of the transformations (e. g. translation, rotation) within the spatial domain by using those as "scaffolding" during transformation learning. To provide the missing evidence for this hypothesis, L&S used behavioral category learning studies within and across the spatial, auditory and visual domains, where rotated and translated 4-element token sequences had to be learned to categorize and then the learned transformation had to applied in new feature dimensions within the given domain. Through single- and multiple-day supervised training and unsupervised tests, L&S demonstrated by standard computational analyses that in such setups, space and spatial transformations can, indeed, help with developing and using appropriate rotational mapping whereas the visual domain cannot fulfill such a scaffolding role.

      Strengths:

      The overall problem definition and the context of spatial mapping-driven solution to the problem is timely. The general design of testing the scaffolding effect across different domains is more advanced than any previous attempts clarifying the relevance of spatial coding to any other type of representational codes. Once the formulation of the general problem in a specific scientific framework is done, the following steps are clearly and logically defined and executed. The obtained results are well interpretable, and they could serve as a good steppingstone for deeper investigations. The analytical tools used for the interpretations are adequate. The paper is relatively clearly written.

      Weaknesses:

      Some additional effort to clarify the exact contribution of the paper, the link between analyses and the claims of the paper and its link to previous proposals would be necessary to better assess the significance of the results and the true nature of the proposed mechanism of abstract generalization.

      (1) Insufficient conceptual setup: The original theoretical proposal (the Tolman-Eichenbaum-Machine, Whittington et al., Cell 2020) that L&S relate their work proposes that just as in the case of memory for spatial navigation, humans and animal create their flexible relational memory system of any abstract representation by a conjunction code that combines on the one hand, sensory representation and on the other hand, a general structural representation or relational transformation. The TEM also suggest that the structural representation could contain any graph-interpretable spatial relations, albeit in their demonstration 2D neighbor relations were used. The goal of L&S's paper is to provide behavioral evidence for this suggestion by showing that humans use representational codes that are invariant to relational transformations of non-spatial abstract stimuli and moreover, that humans obtain these invariances by developing invariance transformers with the help of available spatial transformers. To obtain such evidence, L&S use the rotational transformation. However, the actual procedure they used actually solved an alternative task: instead of interrogating how humans develop generalizations in abstract spaces, they demonstrated that if one defines rotation in an abstract feature space embedded in visual or auditory modality that is similar to the 2D space (i.e. has two independent dimensions that are clearly segregable and continuous), humans cannot learn to apply rotation of 4-piece temporal sequences in those spaces while they can do it in 2D space, and with co-associating a one-to-one mapping between locations in those feature spaces with locations in the 2D space an appropriate shaping mapping training will lead to successful application of rotation in the given task (and in some other feature spaces in the given domain). While this is an interesting and challenging demonstration, it does not shed light on how humans learn and generalize only that humans CAN do learning and generalization in this, highly constrained scenario. This result is a demonstration of how a stepwise learning regiment can make use of one structure for mapping a complex input into a desired output. The results neither clarify how generalizations would develop in abstract spaces nor the question if this generalization uses transformations developed in the abstract space. The specific training procedure ensures success in the presented experiments but the availability and feasibility of an equivalent procedure in natural setting is a crucial part of validating the original claim and that has not been done in the paper.

      (2) Missing controls: The asymptotic performance in Exp 1 after training in the three tasks was quite different in the three tasks (intercepts 2.9, 1.9, 1.6 for spatial, visual and auditory, respectively; p. 5. para. 1, Fig 2BFJ). It seems that the statement "However, or main question was how participants would generalise learning to novel, rotated exemplars of the same concept." assumes that learning and generalization are independent. Wouldn't it be possible, though, that the level of generalization depends on the level of acquiring a good representation of the "concept" and after obtaining an adequate level of this knowledge, generalization would kick in without scaffolding? If so, a missing control is to equate the levels of asymptotic learning and see whether there is a significant difference in generalization. A related issue is that we have no information what kind of learning in the three different domains were performed, albeit we probably suspect that in space the 2D representation was dominant while in the auditory and visual domains not so much. Thus, a second missing piece of evidence is the model fitting results of the ⦰ condition that would show which way the original sequences were encoded (similar to Fig 2 CGK and DHL). If the reason for lower performance is not individual stimulus difficulty but the natural tendency to encode the given stimulus type by a combo of random + 1D strategy that would clarify that the result of the cross-training is, indeed, transferring the 2D-mapping strategy.

    1. Reviewer #2 (Public Review):

      In this manuscript, Hoops et al., using two different model systems, identified key developmental changes in Netrin-1 and UNC5C signaling that correspond to behavioral changes and are sensitive to environmental factors that affect the timing of development. They found that Netrin-1 expression is highest in regions of the striatum and cortex where TH+ axons are travelling, and that knocking down Netrin-1 reduces TH+ varicosities in mPFC and reduces impulsive behaviors in a Go-No-Go test. Further, they show that the onset of Unc5 expression is sexually dimorphic in mice, and that in Siberian hamsters, environmental effects on development are also sexually dimorophic. This study addresses an important question using approaches that link molecular, circuit and behavioral changes. Understanding developmental trajectories of adolescence, and how they can be impacted by environmental factors, is an understudied area of neuroscience that is highly relevant to understanding the onset of mental health disorders. I appreciated the inclusion of replication cohorts within the study.

    1. Reviewer #2 (Public Review):

      The authors succeed in generalizing the pre-alignment procedure for their cell identification method to allow it to work effectively on data with only small subsets of cells labeled. They convincingly show that their extension accurately identifies head angle, based on finding auto florescent tissue and looking for a symmetric l/r axis. Their demonstrated method works to allow the identification of a particular subset of neurons. Their approach should be a useful one for researchers wishing to identify subsets of head neurons in C. elegans, and the ideas might be useful elsewhere.

      The authors also assess the relative usefulness of several atlases for making identity predictions. They attempt to give some additional general insights on what makes a good atlas, and clearly demonstrate the value of more data. Some insights seem less clear as available data do not allow for experiments that cleanly decouple: 1) the number of examples in the atlas; 2) the completeness of the atlas; and 3) the match in strain and imaging modality discussed. In the presented experiments the custom atlas, besides the strain and imaging modality congruence discussed is also the only complete atlas with more than one example. The main neuroPAL atlas is an imperfect stand-in since a significant fraction of cells could not be identified in these data sets, making it a 60/40 mix of Openworm and a hypothetical perfect neuroPAL comparison. The alternate neuroPal atlases shown in supplemental figure 4 are complete but provide only one point cloud.

      It is striking that in the best available apples to apples match the single data set glr-1 atlas produces qualitatively better results than the single (complete) neuroPAL atlas. This is a clear performance advantage given the ground truth. This is as good an evaluation as is possible given current data however given the inexact nature of assigning ground truth identities I think it is difficult from results to tease out if this is due to strain, imaging conditions or systematically different identifications of cells from different sources.

      The experiments do usefully explore the volume of data needed. Though generalization to other arbitrary cell subsets remains to be shown the insight is useful for future atlas building that for the specific (small) set of cells labeled in the experiments 5-10 examples is sufficient to build an accurate atlas.

    1. Reviewer #3 (Public Review):

      This is a revision in response to the reviewer's comments. The authors provided new analyses and try to acknowledge limitations, overall doing a good job, but the interpretation still seems to me going above the available evidence, especially for the claim that it is episodic memory formation during sleep. I still believe the paper will be fairer in dropping this speculative part and omitting the word "episodic" from the title (like actually they did in the abstract). The argument of the authors is that they refer to a computational definition of episodic memory, which is to some extent valid, but I am afraid it is not the way it will be understood by most readers, and it will thus indirectly contribute to an erroneous (or at least, not substantiated) interpretation of the brain's sleeping capabilities.

      My main concern is that I have not seen any proposal for a control condition allowing to exclude the alternative, simpler hypothesis that mere perceptual associations between two elements (foreign word and translation) have been created and stored during sleep (which, I repeat, is already in itself an interesting finding). The authors argue that it seems to them not an efficient processing, but this an opinion, not a demonstration.

    1. Reviewer #2 (Public Review):

      The authors employ molecular dynamics simulations to understand the selectivity of FDA-approved inhibitors within dimeric and monomeric BRAF species. Through these comprehensive simulations, they shed light on the selectivity of BRAF inhibitors by delineating the main structural changes occurring during dimerization and inhibitor action. Notably, they identify the two pivotal elements in this process: the movement and conformational changes involving the alpha-C helix and the formation of a hydrogen bond involving the Glu-501 residue. These findings find support in the analyses of various structures crystallized from dimers and co-crystallized monomers in the presence of inhibitors. The elucidation of this mechanism holds significant potential for advancing our understanding of kinase signaling and the development of future BRAF inhibitor drugs.

      The authors employ a diverse array of computational techniques to characterize the binding sites and interactions between inhibitors and the active site of BRAF in both dimeric and monomeric forms. They combine traditional and advanced molecular dynamics simulation techniques such as CpHMD (all-atom continuous constant pH molecular dynamics) to provide mechanistic explanations. Additionally, the paper introduces methods for identifying and characterizing the formation of the hydrogen bond involving the Glu501 residue without the need for extensive molecular dynamics simulations. This approach facilitates the rapid identification of future BRAF inhibitor candidates.

      The use of molecular dynamics yields crucial structural insights and outlines a mechanism to elucidate dimer selectivity and cooperativity in these systems. However, the authors could consider the adoption of free energy methods to estimate the values of hydrogen bond energies and hydrophobic interactions, thereby enhancing the depth of their analysis.

    1. Reviewer #2 (Public Review):

      Most neurodegenerative diseases are characterized by the self-templated misfolding of a particular protein in a manner that enables progressive spread throughout the central nervous system. In diseases including Parkinson's disease (PD) and multiple system atrophy (MSA), the protein alpha-synuclein misfolds into unique shapes, or strains, which use this self-replicating mechanism to encode disease-specific information. Previous research suggests that a major contributor to the lack of successful clinical trials across neurodegenerative diseases is the lack of disease-relevant strains used in preclinical testing. While MSA patient samples are known to replicate efficiently in cell and mouse models of disease, Lewy body disease (LBD) patient samples do not. To overcome this obstacle, the seeding amplification assay (SAA) uses recombinant alpha-synuclein to amplify the misfolded protein structure present in a human patient sample. The resulting fibrils are then widely used by many laboratories as a model of PD. In this manuscript, Lee et al., set out to compare the strain properties of alpha-synuclein fibrils isolated from LBD and MSA patient samples with the resulting amplified fibrils following SAA. Using orthogonal biochemical and structural approaches to strengthen their analyses, the authors report that the SAA-amplified fibrils do not recapitulate the disease-relevant strains present in the patient samples. Moreover, their data suggest that regardless of which strain is used to seed the SAA reaction, the same strain is generated. These results clearly demonstrate that the SAA-amplified material is not disease-relevant. SAA fibrils are broadly used in academic and pharmaceutical laboratories. They are used in ongoing drug discovery efforts and recombinant fibrils broadly inform much of what is known about alpha-synuclein strain biology in LBD patients. The implications of the reported work are, therefore, expansive. These findings add to the growing ledger of reasons that the use of SAA fibrils in research should be halted until improved methods for amplification with high fidelity are developed.

    1. Reviewer #2 (Public Review):

      Summary:

      Regalado et al. studied how an extended motivational state, necessary for maintaining behavioural drive despite unrewarding experiences, could be encoded in the ACC and its potential causal implications for learning discriminatory behaviour and avoiding unrewarding stimuli. They designed a self-initiated learning task and identified bulk neural responses tuned specifically to reward delivery as well as trial initiation. Interestingly, in both cases, neural activity precedes behavioural onset, indicating the encoding of a motivational signal. To investigate the neural encoding of motivational signals during unrewarded, distracting stimuli presentation, they created a discrimination task by introducing 'no reward' cues, during which animals need to learn not to reduce running speed and not engage in licking. Interestingly, with mice learning to increase running speed and reduce licking rates after 'no reward' cues, the preceding ACC activity also gradually increased. Importantly, only the increase in running speed after 'no reward' cues was impaired upon optogenetic inhibition of ACC activity during early training, linking the extended motivational signal in ACC and learning to maximise rewards by actively avoiding distracting and unrewarded stimuli. Such motivational signals could also be observed in OFC-ACC projecting neurons. Especially the continuous ramping of activity upon repeated 'non-reward' cues, which could be exclusively observed in the 'fast learner' subgroup, provides an interesting concept of how an extended motivational signal necessary for learning avoidance of unrewarded stimuli could be implemented in ACC. The shift in the temporal activity of initially reward-responsive neurons towards the preceding 'no reward' cue, provides a potential mechanism linking extended motivation to reward maximisation. This mechanism seems to be particularly important in periods of persistent 'non-reward' cues, as demonstrated in the impairment of running speed increase after two consecutive 'non-reward' cues.

      Appraisal:

      The authors provide convincing experimental evidence to support their claims of an extended motivational signal encoded in the ACC that is implemented by OFC-ACC signalling and critically involved in learning avoidance of unrewarded stimuli. The newly designed task seems appropriate to identify correlates of relevant cognitive and behavioural variables (e.g. sustained motivation). The combination of recording Ca2+ transients (bulk as well as longitudinal single neuron recordings) to identify potential neural responses and subsequent evaluation of their causal role in establishing and maintaining this persistent motivational state using opto- and pharmacogenetic manipulations is generally accepted.

      Impact:

      The findings will be valuable for further research on the impact of motivational states on behaviour and cognition. The authors provided a promising concept of how persistent motivational states could be maintained, as well as established a novel, reproducible task assay. While experimental methods used are currently state-of-the-art, theoretical analysis seems to be incomplete/not extensive.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors present a very interesting collection of methods and results using brain ultrasound localization microscopy (ULM) in awake mice. They emphasize the effect of the level of anesthesia on the quantifiable elements assessable with this technique (i.e. vessel diameter, flow speed, in veins and arteries, area perfused, in capillaries) and demonstrate the possibility of achieving longitudinal cerebrovascular assessment in one animal during several weeks with their protocol.

      Strengths:

      Even if the methods elements considered separately are not new (brain ULM in rodents, setup for longitudinal awake imaging similar to those used in fUS imaging, quantification of vessel diameters/bubble flow/vessel area), when masterfully combined as it is done in this paper, they answer two questions that have been long-running in the community: what is the impact of anesthesia on the parameters measured by ULM (and indirectly in fUS and other techniques)? Is it possible to achieve ULM in awake rodents for longitudinal imaging? The authors answer quite exhaustively the first question. The manuscript is well-constructed and well-written, and the graphics are appealing.

      Weaknesses:

      The only major comment (calling for further work) I would like to make is the relative weakness of the manuscript regarding longitudinal imaging (mostly Figure 6), compared to the exhaustive review of the effect of isoflurane on the vasculature (3 rats, 3 imaging planes, quantification on a large number of vessels, in 9 different brain regions). The 6 cortical vessels evaluated in Figure 6 feel really disappointing. As longitudinal imaging is supposed to be the salient element of this manuscript (first word appearing in the title), it should be as good and trustworthy as the first part of the paper. Figure 6c. is of major importance, and should be supported by a more extensive vessel analysis, including various brain areas, and validated on several animals to validate the robustness of longitudinal positioning with several instances of the surgical procedure. Figure 6d estimates the reliability of flow measurements on 3 vessels only. Therefore I recommend showing something similar to what is done in Figures 4 and 5: 3 animals, and more extensive quantification in different brain regions.

    1. Reviewer #3 (Public Review):

      Eichler et al. set out to catalog the mechanosensory bristles of the fly head in an effort to understand the extent to which their organization is consistent with the parallel model of hierarchical suppression in the context of grooming behavior. They map the locations of the mechanosensory bristles on the fly head, examine the axonal morphology of the bristle mechanosensory neurons (BMNs) that innervate them, and match these to electron microscopy reconstructions of the same BMNs in a previously published EM volume of the female adult fly brain. They use BMN synaptic connectivity information to create clusters of BMNs that they show occupy different regions of the subesophageal zone brain region and use optogenetic activation of subsets of BMNs to evaluate the behaviors evoked by specific activation of BMN subpopulations innervating the head.

      The authors have beautifully cataloged the mechanosensory bristles and the projection paths and patterns of the corresponding BMN axons in the brain using detailed and painstaking methods. The result is a neuroanatomy resource that will be an important community resource. To match BMNs reconstructed in an electron microscopy volume of the adult fly brain, the authors matched clustered reconstructed BMNs with light-level BMN classes observed using precise dye-fills and stochastic labeling techniques. The authors then employ a variety of clustering methods to demonstrate that BMN populations that innervate different regions of the head project into the subesophageal zone and terminate in distinctive yet, in some cases, partially overlapping zones. By clustering BMNs on the basis of their synaptic partners, the authors find that BMNs from distant areas of the head have non-overlapping synaptic partners while those from neighbor areas have overlapping synaptic partners. This result calls into question the scale at which the parallel model of hierarchical suppression may be operating. Finally, the authors use tools that were generated during the light-level characterization of BMN projections to show that activating BMNs that innervate specific areas of the head leads to grooming of the innervated regions and neighboring regions, consistent with the observed overlap in downstream circuits between BMNs innervating neighboring regions of the head. This result suggests that while the parallel model could be operating on a broad scale, additional circuit mechanisms may be operating on a finer scale to produce grooming of the area surrounding the source of mechanosensory input.

      This work will have a positive impact on the field by contributing a complete accounting of the mechanosensory bristles of the fruit fly head, describing the brain projection patterns of the BMNs that innervate them, and linking them to BMN sensory projections in an electron microscopy volume of the adult fly brain. It will also have a positive impact on the field by providing genetic tools to help functionally subdivide the contributions of different BMN populations to circuit computations and behavior. This contribution will pave the way for further mechanistic study of central circuits that subserve grooming circuits.

    1. Reviewer #2 (Public Review):

      The authors address a question that is interesting and important to the sub-field of rsfMRI that examines electrophysiological correlates of rsfMRI. That is, while electrophysiology-produced correlation maps often appear similar to correlation maps produced from BOLD alone (as has been shown in many papers) is this actually coming from the same source of variance, or independent but spatially-correlated sources of variance? To address this, the authors recorded LFP signals in 2 areas (M1 and ACC) and compared the maps produced by correlating BOLD with them to maps produced by BOLD-BOLD correlations. They then attempt to remove various sources of variance and see the results.

      The basic concept of the research is sound, though primarily of interest to the subset of rsfMRI researchers who use simultaneous electrophysiology. However, there are major problems in the writing, and also a major methodological problem.

      Major problems with writing:

      (1) There is substantial literature on rats on site-specific LFP recording compared to rsfMRI, and much of it already examined removing part of the LFP and examining rsfMRI, or vice versa. The authors do not cover it and consider their work on signal removal more novel than it is.

      (2) The conclusion of the existence of an "electrophysiology-invisible signal" is far too broad considering the limited scope of this study. There are many factors that can be extracted from LFP that are not used in this study (envelope, phase, infraslow frequencies under 0.1Hz, estimated MUA, etc.) and there are many ways of comparing it to the rsfMRI data that are not done in this study (rank correlation, transformation prior to comparison, clustering prior to comparison, etc.). The one non-linear method used, mutual information, is low sensitivity and does not cover every possible nonlinear interaction. Mutual information is also dependent upon the number of bins selected in the data. Previous studies (see 1) have seen similar results where fMRI and LFP were not fully commensurate but did not need to draw such broad conclusions.

      (3) The writing refers to the spatial extent of correlation with the LFP signal as "spatial variance." However, LFP was recorded from a very limited point and the variance in the correlation map does not necessarily reflect underlying electrophysiological spatial distributions (e.g. Yu et al. Nat Commun. 2023 Mar 24;14(1):1651.)

      Major method problem:

      (4) Correlating LFP to fMRI is correlating two biological signals, with unknown but presumably not uniform distributions. However, correlating CC results from correlation maps is comparing uniform distributions. This is not a fair comparison, especially considering that the noise added is also uniform as it was created with the rand() function in MATLAB.

    1. Reviewer #2 (Public Review):

      Summary:

      Cuevas et al. investigate the involvement of DMS and DLS direct and indirect pathways in locomotion and action selection using optogenetic manipulation techniques. They show that optical excitation of dSPNs in both DMS and DLS induces place preference, with optical inhibition resulting in the opposite effect. Interestingly, and somewhat not coming as a surprise given many previous data on this, optical excitation of iSPNs in both regions resulted in place aversion - in line with the classical view of functional opposition.

      Then, the authors performed a two-choice task in which animals would have to choose between pressing in a lever alone or in a lever+stim to obtain a food reward. Again, and not surprisingly, they show that optical activation of dSPNs results in selection from pressing in the lever+stim with the opposite being observed for iSPN, in both DMS and DLS. What was concerting was the increase in lever pressing when inhibiting dSPNs in the DMS, since before authors show that it should cause aversion. When looking at locomotor effects, the authors report an increase in spontaneous displacement when exciting dSPNs in DMS, and the opposite in DLS. Contrary, the excitation of iSPNs either in DMS or DLS increased spontaneous displacement. In reward-seeking, displacement excitation of either dSPNs or iSPNs in both regions resulted in decreased locomotion.

      Strengths:

      Overall this manuscript brings a new light to the involvement of DLS SPNs in both locomotion and behavioral preference.

      Weaknesses:

      Some of the main claims would benefit from further discussion or new data on the effect of optogenetic manipulation on the activity of SPNs. This could allow for the creation of a clearer picture of the involvement of iSPNs and dSPNs of DMS and DLS for behavior.

    1. Reviewer #2 (Public Review):

      Summary

      The authors proposed a toolset Photo-SynthSeg to the software FreeSurfer which performs 3D reconstruction and high-resolution 3D segmentation on a stack of coronal dissection photographs of brain tissues. To prove the performance of the toolset, three experiments were conducted, including volumetric comparison of brain tissues on AD and HC groups from MADRC, quantitative evaluation of segmentation on UW-ADRC and quantitative evaluation of 3D reconstruction on HCP digitally sliced MRI data.

      Strengths

      To guarantee the successful workflow of the toolset, the authors clearly mentioned the prerequisites of dissection photograph acquisition, such as fiducials or rulers in the photos and tissue placement of brain slices with more than one connected component. The quantitative evaluation of segmentation and reconstruction on synthetic and real data demonstrates the accuracy of the methodology. Also, the successful application of this toolset on two brain banks with different slice thicknesses, tissue processing and photograph settings demonstrates its robustness. By working with tools of the SynthSeg pipeline, Photo-SynthSeg could further support volumetric cortex parcellation. The toolset also benefits from its adaptability of different 3D references, such as surface scan, ex vivo MRI and even probabilistic atlas, suiting the needs for different brain banks.

      Weaknesses

      Certain weaknesses are already covered in the manuscript. Cortical tissue segmentation could be further improved. The quantitative evaluation of 3D reconstruction is quite optimistic due to random affine transformations. Manual edits of slice segmentation task are still required and take a couple of minutes per photograph. Finally, the current toolset only accepts coronal brain slices and should adapt to axial or sagittal slices in future work.

    1. Reviewer #2 (Public Review):

      Summary:

      Zhou et al report development of a new method, Rec-Seq, that allows rigorous quantitation of the efficiency of 48S ribosomal pre-initiation complex (PIC) formation on messenger RNAs at transcriptome scale in vitro. With a next-generation deep-sequencing approach, Rec-Seq allows precisely targeted dissection of the roles of translation initiation factors in PIC assembly. This level of molecular precision is important to understanding mechanisms of translational control, making Rec-Seq a significant methodological advance. The authors leverage Rec-Seq to investigate the relative roles of two key helicase enzymes, Ded1p and eIF4A. While past work has pointed to differing roles for Ded1p and eIF4A helicase activity in PIC assembly, unambiguous interpretation of prior in-vivo data has been hindered by technical requirements for performing the experiments in cells. Rec-Seq circumvents these challenges, providing robust mechanistic insights. The authors find that Ded1p stimulates PIC formation selectively on mRNAs with long, structured leaders in the Rec-Seq system, while eIF4A provides much more general stimulation across mRNAs. The findings substantiate the past in-vivo results, along with adding new insights. They contrast with evidence that Ded1p promotes translation by suppressing inhibitory upstream initiation through structural remodeling, or through formation of intracellular, phase-separated granules. The conclusions of the study are well-supported by the data, and are likely to be of broad interest.

      Strengths:

      The quantitative nature of Rec-Seq, which uses an internal standard to measure absolute recruitment efficiencies, is an important strength.

      The methodology decisively overcomes past experimental limitations, allowing the authors to make clear conclusions with regard to the relative roles of Ded1p and eIF4A in PIC formation. An important and useful addition to the toolbox for studying translation and translational control mechanisms, Rec-Seq substantially expands the throughput and scope of mechanistic analyses for translation initiation.

      One significant finding to emerge is that the in-vitro reconstituted system used here recapitulates effects of in-vivo perturbations of translation initiation. Despite the lack of a cellular environment and its components, PIC formation appears to operate much as it does in the cell. Importantly, this highlights an inherent "modularity" to the system that is especially of interest in the context of how regulatory machinery beyond the PIC may control translation.

      Weaknesses:

      The study finds that Ded1p stimulates accumulation of PICs at internal AUG codons, i.e., within mRNA coding sequences, at an incidence of up to ~50% - thus, bypassing "canonical" translation start sites. Understanding the physiological significance of this activity will require further study. The authors address this in the text.

      A limitation of the methodology is that, as an endpoint assay, Rec-Seq does not readily decouple effects of Ded1p on PIC-mRNA loading from those on the subsequent scanning step where the PIC locates the start codon. Considering that Ded1p activity may influence each of these initiation steps through distinct mechanisms - i.e., binding to the mRNA cap-recognition factor eIF4F, or direct mRNA interaction outside eIF4F - additional studies will be needed to gain deeper mechanistic insights. The authors discuss this in the text.

      Comments on revised version:

      In revising their manuscript, the authors have responded very thoughtfully and insightfully to the initial review. The final manuscript is an important contribution to the field, and I am sure it will be of broad interest.

    1. Reviewer #2 (Public Review):

      How the chromosomal passenger complex (CPC) and its subunit Aurora B kinase regulate kinetochore-microtubule attachment, and how the CPC relocates from kinetochores to the spindle midzone as a cell transitions from metaphase to anaphase are questions of great interest. In this study, Ballmer and Akiyoshi take a deep dive into the CPC in T. brucei, a kinetoplastid parasite with a kinetochore composition that varies greatly from other organisms.

      Using a combination of approaches, most importantly in silico protein predictions using alphafold multimer and light microscopy in dividing T. brucei, the authors convincingly present and analyse the composition of the T. brucei CPC. This includes the identification of KIN-A and KIN-B, proteins of the kinesin family. This is a clear advancement over earlier work, for example by Li and colleagues in 2008. The involvement of KIN-A and KIN-B is of particular interest, as it provides a clue for the (re)localization of the CPC during the cell cycle. The evolutionary perspective makes the paper potentially interesting for a wide audience of cell biologists, a point that the authors bring across properly in the title, the abstract, and their discussion.

      The evolutionary twist of the paper would be strengthened 'experimentally' by predictions of the structure of the CPC beyond T. brucei. Depending on how far the authors can extend their in-silico analysis, it would be of interest to discuss a) available/predicted CPC structures in well-studied organisms and b) structural predictions in other euglenozoa. What are the general structural properties of the CPC (e.g. flexible linkers, overall dimensions, structural differences when subunits are missing etc.)? How common is the involvement of kinesin-like proteins?

    1. Reviewer #2 (Public Review):

      The hard work of the authors is much appreciated. With overexpression of a-arrestin Txnip in RPE, cones and the combined respectively, the authors show a potential gene agnostic treatment that can be applied to retinitis pigmentosa. Furthermore, since Txnip is related to multiple intracellular signaling pathway, this study is of value for research in the mechanism of secondary cone dystrophy as well.

      There are a few areas in which the article may be improved through further analysis and application of the data, as well as some adjustments that should be made in to clarify specific points in the article.

      Strengths

      - The follow-up study builds on innovative ground by exploring the impact of TxnipC247S and its combination with HSP90AB1 knockdown on cone survival, offering novel therapeutic pathways.<br /> - Testing of different Txnip deletion mutants provides a nuanced understanding of its functional domains, contributing valuable insights into the mechanism of action in RP treatment.<br /> - The findings regarding GLUT1 clearance and the differential effects of Txnip mutants on cone and RPE cells lay the groundwork for targeted gene therapy in RP.

      Weaknesses

      - The focus on specific mutants and overexpression systems might overlook broader implications of Txnip interactions and its variants in the wider context of retinal degeneration.<br /> - The study's reliance on cell count and GLUT1 expression as primary outcomes misses an opportunity to include functional assessments of vision or retinal health, which would strengthen the clinical relevance.<br /> - The paper could benefit from a deeper exploration of why certain treatments (like Best1-146 Txnip.C247S) do not lead to cone rescue and the potential for these approaches to exacerbate disease phenotypes through glucose shortages.<br /> - Minor inconsistencies, such as the missing space in text references and the need for clarification on data representation (retinas vs. mice), should be addressed for clarity and accuracy.<br /> - The observation of promoter leakage and potential vector tropism issues raise questions about the specificity and efficiency of the gene delivery system, necessitating further discussion and validation.

    1. Reviewer #2 (Public Review):

      Summary:

      In this paper, Sang et al. set out to identify gustatory receptors involved in salt taste sensation in Drosophila melanogaster. In a two-choice assay screen of 30 Ir mutants, they identify that Ir60b is required for avoidance of high salt. In addition, they demonstrate that activation of Ir60b neurons is sufficient for gustatory avoidance using either optogenetics or TRPV1 to specifically activate Ir60b neurons. Then, using tip recordings of labellar gustatory sensory neurons and proboscis extension response behavioral assays in Ir60b mutants, the authors demonstrate that Ir60b is dispensable for labellar taste neuron responses to high salt and the suppression of proboscis extension by high salt. Since external gustatory receptor neurons (GRNs) are not implicated, they look at Poxn mutants, which lack external chemosensory sensilla but have intact pharyngeal GRNs. High salt avoidance was reduced in Poxn mutants but was still greater than Ir60b mutants, suggesting that pharyngeal gustatory sensory neurons alone are sufficient for high salt avoidance. The authors use a new behavioral assay to demonstrate that Ir60b mutants ingest a higher volume of sucrose mixed with high salt than control flies do, suggesting that the action of Ir60b is to limit high salt ingestion. Finally, they identify that Ir60b functions within a single pair of gustatory sensory neurons in the pharynx, and that these neurons respond to high salt but not bitter tastants.

      Strengths:

      A great strength of this paper is that it rigorously corroborates previously published studies that have implicated specific Irs in salt taste sensation. It further introduces a new role for Ir60b in limiting high salt ingestion, demonstrating that Ir60b is necessary and sufficient for high salt avoidance and convincingly tracing the action of Ir60b to a particular subset of gustatory receptor neurons. Overall the authors have achieved their aim by identifying a new gustatory receptor involved in limiting high salt ingestion. They use rigorous genetic, imaging, and behavioral studies to achieve this aim, often confirming a given conclusion with multiple experimental approaches. They have further done a great service to the field by replicating published studies and corroborating the roles of a number of other Irs in salt taste sensation.

    1. Reviewer #5 (Public Review):

      Summary:

      The manuscript by Walker et al., nicely demonstrated a role of TMEM127 in regulating membrane dynamics of RET, a receptor tyrosine kinase and oncogene for multiple cancers, particularly in pheochromocytoma (PCC). They provided compelling cellular and biochemical evidence on how TMEM127 deficiency reduces RET internalization and degradation in specific cancer cell lines, thus stabilizing cell surface RET and promoting its signaling related to cell proliferation. Moreover, TMEM127 may have a broad function beyond RET, and may affect other surface protein activity such as EGFR etc. These findings provided novel mechanisms and key insights to the field of cancer biology.

      Strengths:

      Very interesting findings that nicely explained the mechanistic link between TMEM127 and tumorigenesis by RET regulation...the biochemical analysis was quite thorough and impressive.... the general messages delivered by this study are considered as important to the field of TMEM127 biology and tumorigenesis.

      Weaknesses:

      As acknowledged by the authors, the role of TMEM127 can be conditional and beyond RET modulation, the authors may need to include more discussion that why the loss of TMEM127 is more linked to the development of PCC compared to other cancer types, and why TMEM127 can have such a broad effects in those membrane molecules...in addition, TMEM127 deficiency has been recently linked to enhanced MHC-I-mediated tumor immunity and tumor eradication, in some cancer types...it is then worthwhile to discuss the dual effects of TMEM127 in tumor control in the context of immunity...<br /> Moreover, the authors may need to tune down their "ligand independent" claim on the loss of TMEM127 in driving RET signaling, which should be more related to the level of RET expression/strength of clustering...

    1. Reviewer #3 (Public Review):

      Summary:

      DeHaro-Arbona and colleagues investigate the in vivo dynamics of Notch-dependent transcriptional activation with a focus on the role of the Mastermind (MAM) transcriptional co-activator. They use GFP and HALO-tagged versions of the CSL DNA-binding protein and MAM to visualize the complex, and Int/ParB to visualize the site of Notch-dependent E(Spl)-C transcription. They make several conclusions. First, MAM accumulates at E(Spl)-C when Notch signaling is active, just like CSL. Second, MAM recruits the CDK module of Mediator but does not initiate chromatin accessibility. Third, after signaling is turned off, MAM leaves the site quickly but CSL and chromatin accessibility are retained. Fourth, RNA pol II recruitment, Mediator recruitment and active transcription were similar and stochastic. Fifth, ecdysone enhance the probability of transcriptional initiation.

      Strengths:

      The conclusions are well supported by multiple lines of extensive data that is carefully executed and controlled. A major strength is the strategic combination of Drosophila genetics, imaging and quantitative analyses to conduct compelling and easily interpretable experiments. A second major strength is the focus on MAM to gain insights into dynamics of transcriptional activation specifically.

      Weaknesses:

      Weaknesses were minor. and have been addressed in the revised manuscript.

    1. Reviewer #2 (Public Review):

      Summary:

      The experiments and analysis appear to be carefully done. My concerns center on the impact of the work in its current form on the research community.

      The focal yeast cross here has been the subject of many previous publications (for smaller sets of recombinant progeny), by the last author and others, including phenotyping, genotyping, transcriptomics, and proteomics. This mini-literature has proven relevant to the community because it has empirically pinpointed exactly how many variants underlie a given trait, both molecular and cellular. That is, whereas in more complex organisms we try our best to estimate/infer the full genetic architecture of varying traits from the results of mapping of necessarily weaker power, the highly-powered yeast system can access a more comprehensive mapping of the dozens of loci impinging on a given trait and learn from it. The question is what exactly we learn from the current study?

      Strengths and weaknesses:

      Most of the figures center on methods development and validation for the authors' single-cell RNA-seq in the yeast cross, including generating the large raw data set; analysis pipelines for mapping and genotyping (Figure 1); and higher-level analyses that recapitulate previously reported trends in heritability (Figure 2) and eQTL mapping (Figure 3 and Figure 4B-C). One potential novelty of the study is the methods per se: that is, showing that scRNA-seq works for concomitant genotyping and gene expression profiling in the natural variation context. The authors' rigor and effort notwithstanding: in my view, this can be described as modest in terms of principles. That is, the authors did a good job putting the scRNA-seq idea into practice, but their success is perhaps not surprising or highly relevant for work outside of yeast (as the discussion says). The more substantive claim by the authors for the impact of the study is that they make new observations about the role of expression in phenotype (lines 333-335). The major display item of the manuscript on this theme is Figure 4A, reporting which loci that control growth phenotype (from an earlier paper) also control expression. This is solid but I regret to say that the results strike me as modest. The discussion makes some perhaps fairly big claims that the work has helped "bridge understanding of how genetic variation influences transcriptomic variation" and ultimately cellular phenotype. But with the data as they stand, the authors have missed an opportunity to crystallize exactly how a given variant affects expression (perhaps in waves of regulators affecting targets that affect more regulators) and then phenotype, except for the speculations in the text on lines 305-319. The field started down this road years ago with Bayesian causality inference methods applied to eQTL and phenotype mapping (via e.g. the work of Eric Schadt). The authors could now try Mendelian randomization-type fine-grained detailed models for more firepower toward the same end, and/or experimental tests of the genotype-to-expression-to-phenotype relationship. I would see these directions, motivated by fundamental questions that are relevant to the field at large, as leading to a major advance for this very crowded field. As it stands, I felt their absence in this manuscript especially if the authors are selling principles about linking expression and phenotype as their take-home. I also wonder whether the co-mapping of expression and growth traits in Figure 4A would have been possible with e.g. the bulk RNA-seq from Albert et al., 2018, and I recommend that the authors repeat the Figure 4A-type analyses with the latter to justify their statement that their massive scRNA data set would actually be necessary for them to bear fruit (lines 386-388).

      I also read the discussion of the manuscript as bringing to the fore some of the challenges a reader has in judging the current state of the results to be of actionable impact. The discussion, and the manuscript, will be improved if the authors can put the work in context, posing concrete questions from the field and stating how they are addressed here and what's left to do.

    1. Reviewer #2 (Public Review):

      Summary:<br /> The manuscript, "A microRNA that controls the emergence of embryonic movement" by Menzies, Chagas, and Alonso provides evidence that Drosophila miR-2b-1 is expressed in neurons and controls the expression of the predicted chloride channel CG3638, here named "Janus". Loss of the miRNA leads to movement phenotypes that can be rescued by downregulation of Janus; using specific drivers, the authors show that a larval movement phenotype (slower movement) can be rescued by knockdown of Janus in the chordotonal organs, suggesting that the increase in Janus found in the chordotonal organs is likely the root of the movement defects. Overall, I found the data presented in the manuscript of reasonable quality and are well enough supported by the presented data. That being said, I do have a few problems with the manuscript, mostly stemming from what I feel is an inflated presentation of the importance of the findings.

      Strengths:<br /> The genetic and phenotypic analysis seems to be correct. The nicest part of the manuscript is the connection between the loss of a miRNA and finding its likely target in generating a phenotype. The authors also develop some protocols for the analysis of the movement phenotypes which may be useful for others.

      Weaknesses:<br /> As I mentioned above, I felt the presentation was a bit overstated. The authors present their data in a way that focuses on movement, the emergence of movement, and how their miRNA of interest is at the center of this topic. I only point to the title and name that they wish to give the target of their miRNA to emphasize this point. "Janus" the god of movement and change. The results and discussion section starts with a paragraph saying, "Movement is the main output of the nervous system... how developing embryos manage to organise the necessary molecular, cellular, and physiological processes to initiate patterned movement is still unknown. Although it is clear that the genetic system plays a role, how genes control the formation, maturation and function of the cellular networks underlying the emergence of motor control remains poorly understood." While there is nothing inherently untrue about these statements, it is a question of levels of understanding. One can always argue that something in biology is still unknown at a certain level. However, one could also argue that much is known about the molecular nature of movement. Next, I am not sure how much this work impacts the area of study regarding the emergence of movement. The authors show that a reduction of a miRNA can affect something about certain neurons, that affects movement. The early movements, although slightly diminished, still emerge. Thus, their work only suggests that the function of some neurons, or perhaps the development of these neurons may impact the early movements. This is not new as it was known already from early work from the Bate lab.

      Later larval movements were also shown to be modified in the miRNA mutants and were traced to "janus" overexpression in the chordotonal organs. As neurons are quite sensitive to the levels of Cl- and Janus is thought to be a Cl- channel, this could lead to a slight dysfunction of the chordotonal neurons. So, based on this, the work suggests that dysfunction of the chordotonal organs could impact larval movement. This was, of course, already known. The novelty of this work is in the genes being studied (important or not). We now know that miR 2b-1 and Janus are expressed in the early neurons and larval chordotonal neurons and their removal is consistent with a role for these genes in the functioning of these neurons. This is not to trivialize these findings, simply to state that these results are not significantly changing our overall understanding of movement and the emergence of movement. I would call it a stretch to say that this miRNA 'controls' the emergence of movement, as in the title.

      Finally, the name Janus should be changed as it is already being used. A quick scan of flybase shows that there is a Janus A and B in flies (phosphatases) and I am surprised the authors did not check this. I was initially worried about the Janus kinase (JAK) when I performed the search. While I understand that none are only called Janus, studies of the jan A and B genes refer to the locus as the janus region, which could lead to confusion. The completely different molecular functions of the genes relative to CG3638 add to the confusion. Thus, I ask that the authors change the name of CG3638 to something else.

    1. Reviewer #2 (Public Review):

      Summary:

      Seiichi Koike et al. studied two fusion models, explosive fusion, and bridge fusion, utilizing yolk sac visceral endoderm cells. They elucidated these two fusion models in vivo by employing mathematical modeling and incorporating fluctuations derived from actin dynamics as a key regulator for rapid homotypic fusion between late endosomes.

      Strengths:

      This study uncovered the role of actin dynamics in regulating the transition of fusion models in homotypic fusion between late endosomes and introduced a method for observing the fusion of single vesicles with two different targets. The role of actin dynamics in vesicle fusion in other systems has been extensively studied. This study could offer useful insights for research on vesicle fusion.

      Weaknesses:<br /> The physiological significance of different fusion models is lacking.

    1. Reviewer #2 (Public Review):

      Summary:

      P2X receptors play pivotal roles in physiological processes such as neurotransmission and inflammation, making them promising drug targets. This study, through cryo-EM and functional experiments, reveals the structural basis of the competitive inhibition of the PPNDS and PPADS on mammalian P2X7 receptors. Key findings include the identification of the orthosteric site for these antagonists, the revelation of how PPADS/PPNDS binding impedes channel-activating conformational changes, and the pinpointing of specific residues in P2X1 and P2X3 subtypes that determine their heightened sensitivity to these antagonists. These insights present a comprehensive understanding that could guide the development of improved drugs targeting P2X receptors. This work will be a valuable addition to the field.

      Strengths:

      The combination of structural experiments and mutagenesis analyses offers a deeper understanding of the mechanism. While the inclusion of MD simulation is appreciated, providing more insights from the simulation might further strengthen this already compelling story.

    1. Reviewer #2 (Public Review):

      The authors describe the structure of the S. pneumoniae Nox protein (SpNOX). This is a first. The relevance of it to the structure and function of eukaryotic Noxes is discussed in depth.

      One of the strengths of this work is the effort put into preparing a pure and functionally active SpNOX preparation. The protein was expressed in E. coli and the purification and optimization of its thermostability and activity are described in detail, involving salt concentration, glycerol concentration, and pH.

      Comments on revised version:

      This reviewer would like to compliment the authors for the conscientious revision of the manuscript. Their response to the comments and the detailed explanations of the issues that did not appear clear enough to the reviewer are much appreciated. Their reaction to the review was not only superbly competent but also prominently good natured.

      The revised version is perfect and represents a major contribution to our understanding of the molecular details of Nox function. As for the questions not yet answered, I shall quote the authors: "Time will tell".

    1. Reviewer #2 (Public Review):

      Summary:

      In this paper, the authors set out to better understand the mechanism by which the FtsZ-associated protein ZapD crosslinks FtsZ filaments to assemble a large scale cytoskeletal assembly. For this aim, they use purified proteins in solution and a combination of biochemical, biophysical experiments and cryo-EM. The most significant finding of this study is the observation of FtsZ toroids that form at equimolar concentrations of the two proteins.

      Strengths:

      Many experiments in this paper confirm previous knowledge about ZapD. For example, it shows that ZapD promotes the assembly of FtsZ polymers, that ZapD bundles FtsZ filaments, that ZapD forms dimers and that it reduces FtsZ's GTPase activity.

      The most novel discovery is the observation of different assemblies as a function of ZapD:FtsZ ratio. In addition, using CryoEM to describe the structure of toroids and bundles, the papers provides some information about the orientation of ZapD in relation to FtsZ filaments. For example, they found that the organization of ZapD in relation to FtsZ filaments is "intrinsic heterogeneous" and that FtsZ filaments were crosslinked by ZapD dimers pointing in all directions. The authors conclude that it is this plasticity that allows for the formation of toroids and its stabilization. Unfortunately, a high-resolution structure of the protein organization was not possible.

      Weaknesses:

      While the data is convincing, their interpretation has some substantial weaknesses that the authors should address for the final version of this paper.

      For example, as the authors are the first to describe FtsZ-ZapD toroids, a discussion why this has not been observed in previous studies would be very interesting, i.e. is it due to buffer conditions, sample preparation?

      At parts of the manuscript, the authors try a bit too hard to argue for the physiological significance of these toroids. This, however, is at least very questionable, because:<br /> The typical diameter is in the range of 0.25-1.0 μm, which requires some flexibility of the filaments to be able to accommodate this. It's difficult to see how a FtsZ-ZapD toroid, which appears to be quite rigid with a narrow size distribution of 502 nm {plus minus} 55 nm could support cell division rather than stalling it at that cell diameter. which the authors say is similar to the E. coli cell.

      For cell division, FtsZ filaments are recruited to the membrane surface via an interaction of FtsA or ZipA the C-terminal peptide of FtsZ. As ZapD also binds to this peptide, the question arises who wins this competition or where is ZapD when FtsZ is recruited to the membrane surface? Can such a toroidal structure of FtsZ filaments form on the membrane surface? Additional experiments would be helpful, but a more detailed discussion on how the authors think ZapD could act on membrane-bound filaments would be essential.

      The authors conclude that the FtsZ filaments are dynamic, which is essential for cell division. But the evidence for dynamic FtsZ filaments within these toroids seems rather weak, as it is solely the partial reassembly after addition of GTP. As ZapD significantly slows down GTP hydrolysis, I am not sure it's obvious to make this conclusion.

      On a similar note, on page 5 the authors claim that ZapD would transiently interact with FtsZ filaments. What is the evidence for this? They also say that this transient interaction could have a "mechanistic role in the functionality of FtsZ macrostructures." Could they elaborate?

      The author should also improve in putting their findings into the context of existing knowledge. For example:

      The authors observe a straightening of filament bundles with increasing ZapD concentration. This seems consistent with what was found for ZapA, but this is not explicitly discussed (Caldas et al 2019)

      A paragraph summarizing what is known about the properties of ZapD in vivo would be essential: i.e. what has been found regarding its intracellular copy number, location and dynamics?

      In the introduction, the authors write that "GTP binding and hydrolysis induce a conformational change in each monomer that modifies its binding potential, enabling them to follow a treadmilling behavior". This seems inaccurate, as shown by Wagstaff et al. 2022, the conformational change of FtsZ is not associated with the nucleotide state. In addition, they write that FtsZ polymerization depends on the GTPase activity. It would be more accurate to write that polymerization depends on GTP, and disassembly on GTPase activity.

      On page 2 they also write that "the mechanism underlying bundling of FtsZ filaments is unknown". I would disagree, the underlying mechanism is very well known (see for example Schumacher, MA JBC 2017), but how this relates to the large-scale organization of FtsZ filaments was not clear.

      The authors describe the toroid as a dense 3D mesh, how would this be compatible with the Z-ring and its role for cell division? I don't think this corresponds to the current model of the Z-ring (McQuillen & Xiao, 2020). Apart from the fact it's a ring, I don't think the organization of FtsZ obviously similar to the current of the Z-ring in the bacterial cell, in particular because it's not obvious how FtsZ filaments can bind ZapD and membrane anchors simultaneously.

      The authors write that "most of these modulators" interact with FtsZ's CTP, but then later that ZapD is the only Zap protein that binds CTP. This seems to be inconsistent. Why not write that membrane anchors usually bind the CTP, most Zaps do not, but ZapD is the exception?

      I also have some comments regarding the experiments and their analysis:

      Regarding cryoET: the filaments appear like flat bands, even in the absence of ZapD, which further elongates these bands. Is this due to an anisotropic resolution? This distortion makes the conclusion that ZapD forms bi-spherical dimers unconvincing.

      The authors say that the cryoET visualization provides crucial information on the length of the filaments within this toroid. How long are they? Could the authors measure it?

      Regarding the dimerization mutant of ZapD: there is actually no direct confirmation that mZapD is monomeric. Did the authors try SEC MALS or AUC? Accordingly, the statement that dimerization is "essential" seems exaggerated (although likely true).

      What do the authors mean that toroid formation is compatible with robust persistence length? I.e. What does robust mean? It was recently shown that FtsZ filaments are actually surprisingly flexible, which matches well the fact that the diameter of the Z-ring must continuously decrease during cell division (Dunajova et al Nature Physics 2023).

      the authors claim that their observations suggest „that crosslinkers ... allows filament sliding in an organized fashion". As far as I know there is no evidence of filament sliding, as FtsZ monomers in living cells and in vitro are static.

      What is the „proto-ring FtsA protein"?

      The authors refer to „increasing evidence" for „alternative network remodling mechanisms that do not rely on chemical energy consumption as those in which entropic forces act through diffusible crosslinkers, similar to ZapD and FtsZ polymers." A reference should be given, I assume the authors refer to the study by Lansky et al 2015 of PRC on microtubules. However, I am not sure how the authors made the conclusion that this applies to FtsZ and ZapD, on which evidence is this assumption based?

      Some inconsistencies in supplementary figure 3: The normalized absorbances in panel a do not seem to agree with the absolute absorbance shown in panel e, i.e. compare maximum intensity for ZapD = 20 µM and 5 µM in both panels.

      It's not obvious to me why the structure formed by ZapD and FtsZ disassembles after some time even before GTP is exhausted, can the authors explain? As the structures disassemble, how is the "steady-state turbidity" defined? Do the structures also disassemble when they use a non-hydrolyzable analog of GTP?

      Conclusion:

      Despite some weaknesses in the interpretation of their findings, I think this paper will likely motivate other structural studies on large scale assemblies of FtsZ filaments and its associated proteins. A systematic comparison of the effects of ZapA, ZapC and ZapD and how their different modes of filament crosslinking can result in different filament networks will be very useful to understand their individual roles and possible synergistic behavior.

    1. Reviewer #2 (Public Review):

      This project is on the role of ROCK in skeletogenesis during sea urchin development. That skeleton is produced by a small number of cells in the embryo with signaling inputs from the ectoderm providing patterning cues. The skeleton is built from secretion of CaCO3 by the skeletogenic cells. The authors conclude that ROCK is involved in the regulation of skeletogenesis with a role both in regulating actomyosin in the process, and in the gene regulatory network (GRN) underlying the entire sequence of events.

      The strength of the paper is that they show in detail how perturbations of ROCK results in abnormal actomyosin activity in the skeletogenic cells, and they show alterations both in expression of transcription factors of the GRN, and expression of genes involved in assembly of the skeletal matrix. Two different approaches lead to this conclusion: morpholino perturbations and the actions of a selective inhibitor of the kinase activity. Thus, they achieved their goal which was to test the hypothesis that ROCK is involved in the process of skeletogenesis. Those tests support the hypothesis with data that was quantitatively significant.

      The discussion was transparent regarding where the analysis ended and where the next phase of work should begin. While actomyosin involvement was altered when ROCK was perturbed, it isn't known how direct or indirect the role of ROCK might be. Also, while the regulatory input to spicule initiation and growth is affected when ROCK is inhibited, it isn't clear exactly where ROCK is involved.

    1. Reviewer #2 (Public Review):

      Summary:

      The aim of this manuscript is to use molecular dynamics (MD) simulations to describe the conformational changes of the neurotransmitter binding site of a nicotinic receptor. The study uses a simplified model including the alpha-delta subunit interface of the extracellular domain of the channel and describes the binding of four agonists to observe conformational changes during the weak to strong affinity transition.

      Strength:

      The 200 ns-long simulations of this model suggest that the agonist rotates about its centre in a 'flip' motion, while loop C 'flops' to restructure the site. The changes appear to reproduced across simulations and different ligands and are thus a strong point of the study.

      Weaknesses:

      After carrying out all-atom molecular dynamics, the authors revert to a model of binding using continuum Poisson-Boltzmann, surface area and vibrational entropy. The motivations for and limitations associated with this approximate model for the thermodynamics of binding, rather than using modern atomistic MD free energy methods (that would fully incorporate configurational sampling of the protein, ligand and solvent) could be provided. Despite this, the authors report correlation between their free energy estimates and those inferred from experiment. This did, however, reveal shortcomings for two of the agonists. The authors mention their trouble getting correlation to experiment for Ebt and Ebx and refer to up to 130% errors in free energy. But this is far worse than a simple proportional error, because -24 Vs -10 kcal/mol is a massive overestimation of free energy, as would be evident if it the authors were to instead to express results in terms of KD values (which would have error exceeding a billion fold). The MD analysis could be improved with better measures of convergence, as well as more careful discussion of free energy maps as function of identified principal components, as described below. Overall, however, the study has provided useful observations and interpretations of agonist binding that will help understand pentameric ligand-gated ion channel activation.

      Main points:

      Regarding the choice of model, some further justification of the reduced 2 subunit ECD-only model could be given. On page 5 the authors argue that, because binding free energies are independent of energy changes outside the binding pocket, they could remove the TMD and study only an ECD subunit dimer. While the assumption of distant interactions being small seems somewhat reasonable, provided conformational changes are limited and localised, how do we know the packing of TMD onto the ECD does not alter the ability of the alpha-delta interface to rearrange during weak or strong binding? They further write that "fluctuations observed at the base of the ECD were anticipated because the TMD that offers stability here was absent.". As the TMD-ECD interface is the "gating interface" that is reshaped by agonist binding, surely the TMD-ECD interface structure must affect binding. It seems a little dangerous to completely separate the agonist binding and gating infrastructure, based on some assumption of independence. Given the model was only the alpha and delta subunits and not the pentamer with TMD, I am surprised such a model was stable without some heavy restraints. The authors state that "as a further control we carried out MD simulation of a pentamer docked with ACh and found similar structural changes at the binding pocket compared to the dimer." Is this sufficient proof of the accuracy of the simplified model? How similar was the model itself with and without agonist in terms of overall RMSD and RMSD for the subunit interface and the agonist binding site, as well as the free energy of binding to each model to compare?

      Although the authors repeatedly state that they have good convergence with their MD, I believe the analysis could be improved to convince us. On page 8 the authors write that the RMSD of the system converged in under 200 ns of MD. However, I note that the graph is of the entire ECD dimer, not a measure for the local binding site region. An additional RMSD of local binding site would be much more telling. You could have a structural isomerisation in the site and not even notice it in the existing graph. On page 9 the authors write that the RMSF in Fig.S2 showed instability mainly in loops C and F around the pocket. Given this flexibility at the alpha-delta interface, this is why collecting those regions into one group for the calculation of RMSD convergence analysis would have been useful. They then state "the final MD configuration (with CCh) was well-aligned with the CCh-bound cryo-EM desensitized structure (7QL6)... further demonstrating that the simulation had converged." That may suggest a change occurred that is in common with the global minimum seen in cryo EM, which is good, but does not prove the MD has "converged". I would also rename Fig.S3 accordingly.

      The authors draw conclusions about the dominant states and pathways from their PCA component free energy projections that need clarification. It is important first to show data to demonstrate that the two PCA components chosen were dominant and accounted for most of the variance. Then when mapping free energy as a function of those two PCA components, to prove that those maps have sufficient convergence to be able to interpret them. Moreover, that if the free energies themselves cannot be used to measure state stability (as seems to be the case), that the limitations are carefully explained. First, was PCA done on all MD trajectories combined to find a common PC1 & PC2, or were they done separately on each simulation? If so, how similar are they? The authors write "the first two principal components (PC-1 and PC-2) that capture the most pronounced C. displacements". How much of the total variance did these two components capture? The authors write the changes mostly concern loop C and loop F, but which data proves this? e.g. A plot of PC1 and PC2 over residue number might help?

      The authors map the -kTln rho as a free energy for each simulation as function of PC1 & PC2. It is important to reveal how well that PC1-2 space was sampled, and how those maps converged over time. The shapes of the maps and the relative depths of the wells look very different for each agonist. If the maps were sampled well and converged, the free energies themselves would tell us the stabilities of each state. Instead, the authors do not even mention this and instead talk about "variance" being the indicator of stability, stating that m3 is most stable in all cases. While I can believe 200ns could not converge a PC1-2 map and that meaningful delta G values might not be obtained from them, the issue of lack of sampling must be dealt with. On page 12 they write "Although the bottom of the well for 3 energy minima from PCA represent the most stable overall conformation of the protein, they do not convey direct information regarding agonist stability or orientation". The reasons why not must be explained; as they should do just that if the two order parameters PC1 and PC2 captured the slowest degrees of freedom for binding and sampling was sufficient. The authors write that "For all agonists and trajectories, m3 had the least variance (was most stable), again supporting convergence by 200 ns." Again the issue of actual free energy values in the maps needs to be dealt with. The probabilities expressed as -kTln rho in kcal/mol might suggest that m2 is the most stable. Instead, the authors base stability only on variance (I guess breadth of the well?), where m3 may be more localised in the chosen PC space, despite apparently having less preference during the MD (not the lowest free energy in the maps).

      The motivations and justifications for use of approximate PBSA energetics instead of atomistic MD free energies should be dealt with in the manuscript, with limitations more clearly discussed. Rather than using modern all-atom MD free energy methods for relative or absolute binding free energies, the author select clusters from their identified states and do Poisson-Boltzmann estimates (electrostatic, vdW, surface area, vibrational entropy). I do believe the following sentence does not begin to deal with the limitations in that method: "there are limitations with regard to MM-PBSA accurately predicting absolute binding free energies (Genheden & Ryde, 2015; Hou et al., 2011) that depends on parameterization of the ligand (Oostenbrink et al., 2004)." What are the assumptions and limitations in taking a continuum electrostatics (presumably with parameters for dielectric constants and their assignments to regions after discarding solvent), surface area (with its assumptions and limitations) and of course assuming vibration of a normal mode can capture entropy. On page 30, regarding their vibrational entropy estimate, they write that the "entropy term provides insights into the disorder within the system, as well as how this disorder changes during the binding process". It is important that the extent of disorder captured by the vibrational estimate be discussed, as it is not obvious that it has captured entropy involving multiple minima on the system's true 3N-dimensional energy surface, and especially the contribution from solvent disorder in bound Vs dissociated states.

      As discussed above, errors in the free energy estimates need to be more faithfully represented, as fractional errors are not meaningful. On page 21 the authors write "The match improved when free energy ratios rather than absolute values were compared." But a ratio of free energies is not a typical or expected measure of error in delta G. They also write "For ACh and CCh, there is good agreement between.Gm1 and GLA and between.Gm3 and GHA. For these agonists, in silico values overestimated experimental ones only by ~8% and ~25%. The agreement was not as good for the other 2 agonists, as calculated values overestimated experimental ones by ~45%(Ebt) and ~130% (Ebt). However, the fractional overestimation was approximately the same for GLA and GHA." See above comment on how this may misrepresent the error. On page 21 they write, in relation to their large fractional errors, that they "do not know the origin of this factor but speculate that it could be caused by errors in ligand parameterization". But the estimates from the PBSA approach are, by design, only approximate. Both errors in parameterisation (and their likely origin) and the approximate model used, need discussion.

    1. Reviewer #2 (Public Review):

      Summary:

      Previous NMR and HDX-MS studies on full-length (FL) BTK showed that the covalent BTKi, ibrutinib, causes long-range effects on the conformation of BTK consistent with disruption of the autoinhibited conformation, based on HDX deuterium uptake patterns and NMR chemical shift perturbations. This study extends the analyses to four new covalent BTKi, acalabrutinib, zanubrutinib, tirabrutinib/ONO4059, and a noncovalent ATP competitive BTKi, pirtobrutinib/LOXO405.

      The results show distinct conformational changes that occur upon binding each BTKi. The findings show consistent NMR and HDX changes with covalent inhibitors, which move helix aC to an 'out' position and disrupt SH3-kinase interactions, in agreement with X-ray structures of the BTKi complexed with the BTK kinase domain. In contrast, the solution measurements show that pirtobrutinib maintains and even stabilizes the helix aC-in and autoinhibited conformation, even though the BTK:pritobrutinib crystallizes with helix aC-out. This and unexpected variations in NMR and HDX behavior between inhibitors highlight the need for solution measurements to understand drug interactions with the full-length BTK. Overall the findings present good evidence for allosteric effects by each BTKi that induce distal conformational changes which are sensitive to differences in inhibitor structure.

      The study goes on to examine BTK mutants T474I and L528W, which are known to confer resistance to pirtobrutinib, zanubritinib, and tirabrutinib. T474I reduces and L528W eliminates BTK autophosphorylation at pY551, while both FL-BTK-WT and FL-BTK-L528W increase HCK autophosphorylation and PLCg phosphorylation. These show that mutants partially or completely inactivate BTK and that inactive FL-BTK can activate HCK, potentially by direct BTK-HCK interactions. But they do not explain drug resistance. However, HDX and NMR show that each mutant alters the effects of BTKi binding compared to WT. In particular, T474I alters the effects of all three inhibitors around W395 and the activation loop, while L528W alters interactions around W395 with tirabrutinib and pirtobrutinib, and does not appear to bind zanubrutinib at all. The study concludes that the mutations might block drug efficacy by reducing affinity or altering binding mode.

      Strengths:

      The work presents convincing evidence that BTK inhibitors alter the conformation of regions distal to their binding sites, including those involved in the SH3-kinase interface, the activation loop, and a substrate binding surface between helix aF and helix aG. The findings add to the growing understanding of allosteric effects of kinase inhibitors, and their potential regulation of interactions between kinase and binding proteins.

      Weaknesses:

      The interpretation of HDX, NMR, and kinase assays is confusing in some places, due to ambiguity in quantifying how much kinase is bound to the inhibitor. It would be helpful to confirm binding occupancy, in order to clarify if mutants lower the amount of BTK complexed with BTKi as implied in certain places, or if they instead alter the binding mode. In addition, the interpretation of the mutant effects might benefit from a more detailed examination of how each inhibitor occupies the ATP pocket and how substitutions of T474 and L528 with Ile and Trp respectively might change the contacts with each inhibitor.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors identified that two of the placental CALHM orthologs, CALHM2 and CALHM4 can form heterooligomeric channels that are stable following detergent solubilization. By adding fiducial markers that specifically recognize either CALHM2 or CALHM4, the authors determine a cryo-EM density map of heterooligomeric CALHM2/CALHM4 from which they can determine how the channel is assembled. Surprisingly, the two orthologs segregate into two distinct segments of the channel. This segregation enables the interfacial subunits to ease the transition between the preferred conformations of each ortholog, which are similar to the confirmation that each ortholog adopts in homooligomeric channels.

      Strengths:

      Through the use of fiducial markers, the authors can clearly distinguish between the CALHM2 and CALHM4 promoters in the heterooligomeric channels, strengthening their assignment of most of the promoters. The authors take appropriate caution in identifying two subunits that are likely a mix of the two orthologs in the channel.

      Weaknesses:

      Despite the authors' efforts, no currents could be observed that corresponded to CALHM2/CALHM4 channels and thus the functional effect of their interaction is not known.

    1. Reviewer #2 (Public Review):

      Zhang et al investigated the biophysical mechanism of potassium-mediated chemotactic behavior in E coli. Previously, it was reported by Humphries et al that the potassium waves from oscillating B subtilis biofilm attract P aeruginosa through chemotactic behavior of motile P aeruginosa cells. It was proposed that K+ waves alter PMF of P aeruginosa. However, the mechanism was this behaviour was not elusive. In this study, Zhang et al demonstrated that motile E coli cells accumulate in regions of high potassium levels. They found that this behavior is likely resulting from the chemotaxis signalling pathway, mediated by an elevation of intracellular pH. Overall, a solid body of evidence is provided to support the claims. However, the impacts of pH on the fluorescence proteins need to be better evaluated. In its current form, the evidence is insufficient to say that the fluoresce intensity ratio results from FRET. It may well be an artefact of pH change.

      The authors now carefully evaluated the impact of pH on their FRET sensor by examining the YFP and CFP fluorescence with no-receptor mutant. The authors used this data to correct the impact of pH on their FRET sensor. This is an improvement, but the mathematical operation of this correction needs clarification. This is particularly important because, looking at the data, it is not fully convincing if the correction was done properly. For instance, 3mM KCl gives 0.98 FRET signal both in Fig3 and FigS4, but there is almost no difference between blue and red lines in Fig 3. FigS4 is very informative, but it does not address the concern raised by both reviewers that FRET reporter may not be a reliable tool here due to pH change.

      The authors show the FRET data with both KCl and K2SO4, concluding that the chemotactic response mainly resulted from potassium ions. However, this was only measured by FRET. It would be more convincing if the motility assay in Fig1 is also performed with K2SO4. The authors did not address this point. In light of complications associated with the use of the FRET sensor, this experiment is more important.

    1. Reviewer #2 (Public Review):

      Summary: In the manuscript, the authors have presented new mechanistic details to show how intracellular cAMP levels are maintained linked to the phosphodiesterase enzyme which in turn is controlled by PhoP. Later, they showed the physiological relevance linked to altered cAMP concentrations.

      Strengths: Well thought out experiments. The authors carefully planned the experiments well to uncover the molecular aspects of it diligently.

      Weaknesses: Some fresh queries were made based on the author's previous responses and hope to get satisfactory answers this time.

    1. Reviewer #2 (Public Review):

      The manuscript by Bohl et al. is an interesting and carefully done study on the biochemical properties and mode of action of potent autonomous AAA+ disaggregase ClpL from Listeria monocytogenes. ClpL is encoded on plasmids. It shows high thermal stability and provides Listeria monocytogenes food-pathogen substantial increase in resistance to heat. The authors show that ClpL interacts with aggregated proteins through the aromatic residues present in its N-terminal domain and subsequently unfolds proteins from aggregates translocating polypeptide chains through the central pore in its oligomeric ring structure. The structure of ClpL oligomers was also investigated in the manuscript. The results suggest that mono-ring structure and not dimer or tetramer of rings, observed in addition to mono-ring structures under EM, is an active specie of disaggregase. In the revised version additional data is presented suggesting that dimer or tetramer of ClpL rings play a protective role in cell by restricting ClpL activity.

      Presented experiments are conclusive and well controlled. I think the presentation and discussion of results are better in revised version.<br /> The study's strength lies in the direct comparison of ClpL biochemical properties with autonomous ClpG disaggregase present in selected Gram-negative bacteria and well-studied E. coli system consisting of ClpB disaggregase and DnaK and its cochaperones. This puts the results in a broader context.

    1. Reviewer #2 (Public Review):

      Summary:<br /> In the manuscript by Rincon-Torroella et al, the authors evaluated the therapeutic potential of ME3BP-7, a microencapsulated formulation of 3BP which specifically targets MCT-1 high tumor cells, in pancreatic cancer models. The authors showed that, compared to 3BP, ME3BP-7 exhibited much-enhanced stability in serum. In addition, the authors confirmed the specificity of ME3BP-7 toward MCT-1 high tumor cells and demonstrated the in vivo anti-tumor effect of ME3BP-7 in orthotopic xenograft of human PDAC cell line and PDAC PDX model.

      Strengths:<br /> (1) The study convincingly demonstrated the superior stability of ME3BP-7 in serum.<br /> (2) The specificity of ME3BP-7 and 3BP toward MCT-1 high PDAC cells was clearly demonstrated with CRISPR-mediated knockout experiments.

      Weaknesses:<br /> The advantage of ME3BP-7 over 3BP under an in vivo situation was not fully established.

    1. Reviewer #2 (Public Review):

      Summary:

      Gao et al. used single-molecule FRET and step-wise transcription methods to study the conformations of the recently reported guanidine-IV class of bacterial riboswitches that upregulate transcription in the presence of elevated guanidine. Using three riboswitch lengths, the authors analyzed the distributions and transitions between different conformers in response to different Mg2+ and guanidine concentrations. These data led to a three-state kinetic model for the structural switching of this novel class of riboswitches whose structures remain unavailable. Using the PLOR method that the authors previously invented, they further examined the conformations, ligand responses, and gene-regulatory outcomes at discrete transcript lengths along the path of vectorial transcription. These analyses uncover that the riboswitch exhibits differential sensitivity to ligand-induced conformational switching at different steps of transcription, and identify a short window where the regulatory outcome is most sensitive to ligand binding.

      Strengths:

      Dual internal labeling of long RNA transcripts remains technically very challenging but essential for smFRET analyses of RNA conformations. The authors should be commended for achieving very high quality and purity in their labelled RNA samples. The data are extensive, robust, thorough, and meticulously controlled. The interpretations are logical and conservative. The writing is reasonably clear and the illustrations are of high quality. The findings are significant because the paradigm uncovered here for this relatively simple riboswitch class is likely also employed in numerous other kinetically regulated riboswitches. The ability to quantitatively assess RNA conformations and ligand responses at multiple discrete points along the path towards the full transcript provides a rare and powerful glimpse into co-transcriptional RNA folding, ligand-binding, and conformational switching.

      Weaknesses:

      The use of T7 RNA polymerase instead of a near-cognate bacterial RNA polymerase in the termination/antitermination assays is a significant caveat. It is understandable as T7 RNA polymerase is much more robust than its bacterial counterparts, which probably will not survive the extensive washes required by the PLOR method. The major conclusions should still hold, as the RNA conformations are probed by smFRET at static, halted complexes instead of on the fly. However, potential effects of the cognate RNA polymerase cannot be discerned here, including transcriptional rates, pausing, and interactions between the nascent transcript and the RNA exit channel, if any. The authors should refrain from discussing potential effects from the DNA template or the T7 RNA polymerase, as these elements are not cognate with the riboswitch under study.

    1. Reviewer #2 (Public Review):

      In this report, Zeng and Staley have used an elegant combination of RNA imaging approaches (single molecule FISH), RNA co-immunoprecipitations, and translation reporters to characterize the factors and pathways involved in the nuclear export of splicing intermediates in budding yeast. Their study notably involves the use of specific reporter genes, which lead to the accumulation of pre-mRNA and lariat species, in a battery of mutants impacting mRNA export and quality control.

      The authors convincingly demonstrate that mRNA species expressed from such reporters are exported to the cytoplasm in a manner depending on the canonical mRNA export machinery (Mex67 and its adaptors) and the nuclear pore complex (NPC) basket (Mlp1). Interestingly, they provide evidence that the export of splicing intermediates requires docking and subsequent undocking at the nuclear basket, a step possibly more critical than for regular mRNAs.

      However, their assays do not always allow us to define whether the impacted mRNA species correspond to lariats and/or pre-mRNAs. This is all the more critical since their findings apparently contradict previous reports that supported a role for the nuclear basket in pre-mRNA quality control. These earlier studies, which were similarly based on the use of dedicated yet distinct reporters, had found that the nuclear basket subunit Mlp1, together with different cofactors, prevents the export of unspliced mRNA species. It would be important to clarify experimentally and discuss the possible reasons for these discrepancies.

    1. Reviewer #2 (Public Review):

      In this manuscript, Lee et al. assessed the role of Tead1 in mouse beta cells using three Cre-driver lines: Rip-Cre, Ins-Cre, and Mip-CreERT. The authors demonstrate that loss of TEAD1 during development and in mature beta cells leads to increased cell-autonomous beta cell proliferation and reduced insulin secretion. The phenotype of Tead1 knockout is not surprising, given that it is a key player in the Hippo pathway - a well-characterized pathway controlling cell proliferation. However, as the authors suggested, the phenotype observed in Tead1 might be through other non-Hippo pathway factors as well. The authors further convincingly established PDX1 and p16 as the target of Tead1 in controlling beta cell function and proliferation correspondingly. I have the following specific comments:

      (1) As the authors mentioned, there are concerns over the usage of some Cre transgenic lines. Another useful control would be the naive Cre line that is not bred to floxed mutant, in addition to the floxed mice used by the authors in the manuscript here.

      (2) The logic to rely on the deletion of Ezh2 to restore p16 in the Tead1 knockout mice is unclear. Ezh2 has so many more targets than p16. Why not a direct rescue experiment by overexpression of p16?

      (3) The observed correlation of PDX1 and TEAD1 in expression in human islets is intriguing. But does this correlation translate to beta cell proliferation and function? Does TEAD1 knockout in human islets elicit a similar proliferation versus function response?

      (4) The argument of Tead1 only controls maturation but not differentiation and that maturation function versus proliferation phenotype is independently controlled is weak. It appears that this conclusion is only based on that "many disallowed genes...were not altered in Tead1-deficient islets". Perhaps the authors can perform a formal comparison between the transcriptomic changes of Tead1 knockout and Myc overexpressing/Notch gain of function beta cells and show that these two processes are different. In addition, what are the signatures of genes that are upregulated in Tead1 knockout compared with controls?

    1. Reviewer #2 (Public Review):

      Summary:

      The manuscript by Bayanjargal et al. entitled "The DBD-alpha4 helix of EWS::FLI is required for GGAA microsatellite binding that underlies genome regulation in Ewing sarcoma" reports on the critical role of a small alpha helix in the DNA binding domain (DBD) of the FLI1 portion of EWS::FLI1 that is critical for binding to repetitive stretches of GGAA-motifs, i.e. GGAA microsatellites, which serve as potent neoenhancers in Ewing sarcoma.

      Strengths:

      The paper is generally well-written, and easy to follow and the data presented are of high quality, well-described and underpin the conclusions of the authors. The report sheds new light on how EWS::FLI1 mechanistically binds to and activates GGAA microsatellite enhancers, which is of importance to the field.

      Weaknesses:

      While there are no major weaknesses in this paper, there are a few minor issues that the authors may wish to address:

      (1) While the official protein symbol for the gene EWSR1 is indeed EWS, the protein symbol for the gene FLI1 is identical, i.e. FLI1. The authors nominate the fusion oncoprotein EWS::FLI1 (even in the title) but it appears more adequate to use EWS::FLI1.

      (2) The used cell lines should be spelled according to their official nomenclature (e.g. A-673 instead of A673).

      (3) It appears as if the vast majority of results were generated in a single Ewing sarcoma cell line (A-673) which is an atypical Ewing sarcoma cell line harboring an activating BRAF mutation and may be genomically quite unstable as compared to other Ewing sarcoma cell lines (Kasan et al. 2023 preprint at bioRxiv https://www.biorxiv.org/content/10.1101/2023.11.20.567802v1). Hence, it may be supportive for the paper to recapitulate/cross-validate a few key results in other Ewing sarcoma cell lines, e.g. by using EWS::ERG-positive cell lines. Perhaps the authors could make use of available published data.

      (4) Figure 6 and Supplementary Figure 5 are very interesting but focus on two selected target genes of the fusion (FCGRT and CCND1). It would be interesting to see whether these findings also extend to common EWS::ETS transcriptional signatures that have been reported. The authors could explore their data and map established consensus EWS::ETS signatures to investigate which other hubs might be affected at relevant target genes.

      (5) Table 1 is a bit hard to read. In my opinion, it is not necessary to display P-values with up to 8 decimal positions. The gene symbols should be displayed in italic font.

    1. Reviewer #2 (Public Review):

      Using proteogenomic analysis of human cancer datasets, Yu et al, found that EGFR protein levels negatively correlate with ZNFR3/RNF43 expression across multiple cancers. Interestingly, they found that CRC harbouring the frequent RNF43 G659Vfs*41 mutation exhibits higher levels of EGFR when compared to RNF43 wild-type tumors. This is highly interesting since this mutation is generally not thought to influence Frizzled levels and Wnt-bcatenin pathway activity. Using CRISPR knockouts and overexpression experiments, the authors show that EGFR levels are modulated by ZNRF3/RNF43. Supporting these findings, modulation of ZNRF3/RNF43 activity using Rspondin also leads to increased EGFR levels. Mechanistically, the authors, show that ZNRF3/RNF43 ubiquitinate EGFR and leads to degradation. Finally, the authors present functional evidence that loss of ZNRF3/RNF43 unleashes EGFR-mediated cell growth in 2D culture and organoids and promotes tumor growth in vivo.

      Overall, the conclusions of the manuscript are well supported by the data presented, but some aspects of the mechanism presented need to be reinforced to fully support the claims made by the authors. Additionally, the title of the paper suggests that ZNRF3 and RNF43 loss leads to the hyperactivity of EGFR and that its signalling activity contributes to cancer initiation/progression. I don't think the authors convincingly showed this in their study.

      Major points:

      (1) EGFR ubiquitination. All of the experiments supporting that ZNFR3/RNF43 mediates EGFR ubiquitination are performed under overexpression conditions. A major caveat is also that none of the ubiquitination experiments are performed under denaturing conditions. Therefore, it is impossible to claim that the ubiquitin immunoreactivity observed on the western blots presented in Figure 4 corresponds to ubiquitinated-EGFR species.

      Another issue is that in Figure 4A, the experiments suggest that the RNF43-dependent ubiquitination of EGFR is promoted by EGF. However, there is no control showing the ubiquitination of EGFR in the absence of EGF but under RNF43 overexpression. According to the other experiments presented in Figures 4B, 4C, and 4F, there seems to be a constitutive ubiquitination of EGFR upon overexpression. How do the authors reconcile the role of ZNRF3/RNF43 vs c-cbl ?

      (2) EGFR degradation vs internalization. In Figure 3C, the authors show experiments that demonstrate that RNF43 KO increases steady-state levels of EGFR and prevents its EGF-dependent proteolysis. Using flow cytometry they then present evidence that the reduction in cell surface levels of EGFR mediated by EGF is inhibited in the absence of RNF43. The authors conclude that this is due to inhibition of EGF-induced internalization of surface EGF. However, the experiments are not designed to study internalization and rather merely examine steady-state levels of surface EGFR pre and post-treatment. These changes are an integration of many things (retrograde and anterograde transport mechanisms presumable modulated by EGF). What process(es) is/are specifically affected by ZNFR3/RNF43 ? Are these processes differently regulated by c-cbl ? If the authors are specifically interested in internalization/recycling, the use of cell surface biotinylation experiments and time courses are needed to examine the effect of EGF in the presence or absence of the E3 ligases.

      (3) RNF43 G659fs*41. The authors make a point in Figure 1D that this mutant leads to elevated EGFR in cancers but do not present evidence that this mutant is ineffective in mediated ubiquitination and degradation of EGFR. As this mutant maintains its ability to promote Frizzled ubiquitination and degradation, it would be important to show side by side that it does not affect EGFR. This would perhaps imply differential mechanisms for these two substrates.

      (4) "Unleashing EGFR activity". The title of the paper implies that ZNRF3/RNF43 loss leads to increased EGFR expression and hence increased activity that underlies cancer. However, I could find only one direct evidence showing that increased proliferation of the HT29 cell line mutant for RNF43 could be inhibited by the EGFR inhibitor Erlotinib. All the other evidence presented that I could find is correlative or indirect (e.g. RPPA showing increased phosphorylation of pathway members upon RNF43 KO, increased proliferation of a cell line upon ZNRF3/ RNF43 KO, decreased proliferation of a cell line upon ZNRF3/RNF43 OE in vitro or in xeno...). Importantly, the authors claim that cancer initiation/ progression in ZNRF3/RNF43 mutants may in some contexts be independent of their regulation of Wnt-bcatenin signaling and relying on EGFR activity upregulation. However, this has not been tested directly. Could the authors leverage their znrf3/RNF43 prostate cancer model to test whether EGFR inhibition could lead to reduced cancer burden whereas a Frizzled or Wnt inhibitor does not?

      More broadly, if EGFR signaling were to be unleashed in cancer, then one prediction would be that these cells would be more sensitive to EGFR pathway inhibition. Could the authors provide evidence that this is the case? Perhaps using isogenic cell lines or a panel of patient-derived organoids (with known genotypes).

    1. Reviewer #2 (Public Review):

      Summary:

      Together with the known anatomical connectivity of C. elegans, a neurotransmitter atlas paves the way toward a functional connectivity map. This study refines the expression patterns of key genes for neurotransmission by analyzing the expression patterns from CRISPR-knocked-in GFP reporter strains using the color-coded Neuropal strain to identify neurons. Along with data from previous scRNA sequencing and other reporter strains, examining these expression patterns enhances our understanding of neurotransmitter identity for each neuron in hermaphrodites and the male nervous system. Beyond the known neurotransmitters (GABA, Acetylcholine, Glutamate, dopamine, serotonin, tyramine, octopamine), the atlas also identifies neurons likely using betaine and suggests sets of neurons employing new unknown monoaminergic transmission, or using exclusively peptidergic transmission.

      Strengths:

      The use of CRISPR reporter alleles and of the Neuropal strain to assign neurotransmitter usage to each neuron is much more rigorous than previous analysis and reveals intriguing differences between scRNA seq, fosmid reporter, and CRISPR knock-in approaches. Among other mechanisms, these differences between approaches could be attributed to 3'UTR regulatory mechanisms for scRNA vs. knockin or titration of rate-limited negative regulatory mechanisms for fosmid vs. knockin. It would be interesting to discuss this and highlight the occurrences of these potential phenomena for future studies.

      Weaknesses:

      For GABAergic transmission, one shortcoming arises from the lack of improved expression pattern by a knockin reporter strain for the GABA recapture symporter snf-11. In its absence, it is difficult to make a final conclusion on GABA recapture vs GABA clearance for all neurons expressing the vesicular GABA transporter neurons (unc-47+) but not expressing the GAD/UNC-25 gene e.g. SIA or R2A neurons. At minima, a comparison of the scRNA seq predictions versus the snf-11 fosmid reporter strain expression pattern would help to better judge the proposed role of each neuron in GABA clearance or recycling.

      Considering the complexities of different tagging approaches, like T2A-GFP and SL2-GFP cassettes, in capturing post-translational and 3'UTR regulation is important. The current formulation is simplistic. e.g. after SL2 trans-splicing the GFP RNA lacks the 5' regulatory elements, T2A-GFP self-cleavage has its own issues, and the his-44-GFP reporter protein does certainly have a different post-translational life than vesicular transporters or cytoplasmic enzymes.

      Do all splicing variants of neurotransmitter-related genes translate into functional proteins? The possibility that some neurons express a non-functional splice variant, leading to his-74-GFP reporter expression without functional neurotransmitter-related protein production is not addressed. Also, one tagged splice variant of unc-25 is expected to fail to produce a GFP reporter, can this cause trouble?

    1. Reviewer #2 (Public Review):

      Summary:

      In this paper, the authors assess the function of Rab10 in dense core vesicle (DCV) exocytosis using RNAi and cultured neurons. The author provides evidence that their knockdown (KD) is effective and provides evidence that DCV is compromised. They also perform proteomic analysis to identify potential pathways that are affected upon KD of Rab10 that may be involved in DCV release. Upon focusing on ER morphology and protein synthesis, the authors conclude that defects in protein synthesis and ER Ca2+ homeostasis contributes to the DVC release defect upon Rab10 KD. The authors claim that Rab10 is not involved in synaptic vesicle (SV) release and membrane homeostasis in mature neurons.

      Strengths:

      The data related to Rab10's role in DCV release seems to be strong and carried out with rigor. While the paper lacks in vivo evidence that this gene is indeed involved in DCV in a living mammalian organism, I feel the cellular studies have value. The identification of ER defect in Rab10 manipulation is not truly novel but it is a good conformation of studies performed in other systems. The finding that DCV release defect and protein synthesis defect seen upon Rab10 KD can be significantly suppressed by Leucine supplementation is also a strength of this work.

      Weaknesses:

      The data showing Rab10 is NOT involved in SV exocytosis seems a bit weak to me. Since the proteomic analysis revealed so many proteins that are involved in SV exo/encodytosis to be affected upon Rab10, it is a bit strange that they didn't see an obvious defect. Perhaps this could have been because of the protocol that the authors used to trigger SV release (I am not an E-phys expert but perhaps this could have been a 'sledge-hammer' manipulation that may mask any subtle defects)? Perhaps the authors can claim that DCV is more sensitive to Rab10 KD than SV, but I am not sure whether the authors should make a strong claim about Rab10 not being important for SV exocytosis.

      Also, the authors mention "Rab10 does not regulate membrane homeostasis in mature neurons" but I feel this is an overstatement. Since the authors only performed KD experiments, not knock-out (KO) experiments, I believe they should not make any conclusion about it not being required, especially since there is some level of Rab10 present in their cells. If they want to make these claims, I believe the authors will need to perform conditional KO experiments, which are not performed in this study.

      Finally, the authors show that protein synthesis and ER Ca2+ defects seem to contribute to the defect but they do not discuss the relationship between the two defects. If the authors treat the Rab10 KD cells with both ionomycin and Leucine, do they get a full rescue? Or is one defect upstream of the other (e.g. can they see rescue of ER morphology upon Leucine treatment)? While this is not critical for the conclusions of the paper, several additional experiments could be performed to clarify their model, especially considering there is no clear model that explains how Rab10, protein synthesis, ER homeostasis, and Ca2+ are related to DCV (but not SV) exocytosis.

    1. Reviewer #2 (Public Review):

      Summary:

      This study examines the pattern of responses produced by the combination of left-eye and right-eye signals in V1. For this, they used calcium imaging of neurons in V1 of awake, fixating monkeys. They take advantage of calcium imaging, which yields large populations of neurons in each field of view. With their data set, they observe how response magnitude relates to ocular dominance across the entire population. They analyze carefully how the relationship changed as the visual stimulus switched from contra-eye only, ipsi-eye only, and binocular. As expected, the contra-eye dominated neurons responded strongly with a contra-eye only stimulus. The ipsi-eye dominated neurons responded strongly with an ipsi-eye only stimulus. The surprise was responses to a binocular stimulus. The responses were similarly weak across the entire population, regardless of each neuron's ocular dominance. They conclude that this pattern of responses could be explained by interocular divisive normalization, followed by binocular summation.

      Strengths:

      A major strength of this work is that the model-fitting was done on a large population of simultaneously recorded neurons. This approach is an advancement over previous work, which did model-fitting on individual neurons. The fitted model in the manuscript represents the pattern observed across the large population in V1, and washes out any particular property of individual neurons. Given the large neuronal population from which the conclusion was drawn, the authors provide solid evidence supporting their conclusion. They also observed consistency across 5 field of views.

      The experiments were designed and executed appropriately to test their hypothesis. Their data support their conclusion.

      Weaknesses:

      The nonlinear interocular suppression found in this study, could potentially be partially exaggerated by the nonlinear properties of calcium signals. One of the authors of this study has previously reported that the particular GCaMP used in this study has a nice proportional relationship with firing rate of a neuron. So the concern of exaggeration probably does not apply to this particular study. The concern would apply to others who try similar measurements with other versions of GCaMP.

      The implication of their finding is that strong ocular dominance is the result of release from interocular suppression by a monocular stimulus, rather than the lack of binocular combination as many traditional studies have assumed. This could significantly advance our understanding of the binocular combination circuitry of V1. The entire population of neurons could be part of a binocular combination circuitry present in V1.

    1. Reviewer #2 (Public Review):

      Summary:

      The study investigates the mechanisms underlying chemotherapy-induced peripheral neuropathy (CIPN), a notable side effect of commonly used anticancer drugs like paclitaxel. It aims to comprehend the putative mechanisms through lipidomics analysis of plasma samples from cancer patients pre and post-paclitaxel treatment, drawing inspiration from preclinical studies highlighting the role of sphingolipids. While the use of patient plasma samples stands out as a major strength, shortcomings in the result presentation undermine the study's significance. The introduction lacks a robust rationale, failing to articulate the utility of machine learning methods over conventional lipidomics analysis and the relevance of broader neuropathy in the context of the study's goal of investigating peripheral neuropathy. The failure to robustly link neuropathy to paclitaxel treatment, with only around 50% of patients developing neuropathy, mostly at Grade 1, with no or mild symptoms that require no intervention, weakens the study's impact. The presentation of results lacks clarity on sphingolipid dysregulation, leaving uncertainty regarding downregulation or upregulation. Furthermore, no clarity in validation for the machine learning-based analysis with conventional methods and an overall weakness in result representation weaken the study, despite addressing an important question in the field.

      Strengths:

      The study leverages patient plasma samples before and after paclitaxel treatment, enhancing the translatability of findings to patient impact. The attempt to employ machine learning (ML) methods for analyzing biological samples and classifying patient groups is commendable, pushing the biomedical sciences towards ML applications for handling complex data. The chosen topic of investigating chemotherapy-induced peripheral neuropathy (CIPN) is clinically important, offering potential benefits for cancer patients undergoing chemotherapy treatment.

      Weaknesses:

      The article is poorly written, hindering a clear understanding of core results. While the study's goals are apparent, the interpretation of sphingolipids, particularly SA1P, as key mediators of paclitaxel-induced neuropathy lacks robust evidence. The introduction fails to establish the significance of general neuropathy or peripheral neuropathy in anticancer drug-treated patients, and crucial details, such as the percentage of patients developing general neuropathy or peripheral neuropathy, are omitted. This omission is particularly relevant given that only around 50% of patients developed neuropathy in this study, primarily of mild Grade 1 severity with negligible symptoms, contradicting the study's assertion of CIPN as a significant side effect. The lack of clarity in distinguishing results obtained by lipidomics using machine learning methods and conventional methods adds to the confusion. The poorly written results section fails to specify SA1P's downregulation or upregulation, and the process of narrowing down to sphingolipids and SA1P is inadequately explained. Integrating a significant portion of the discussion section into the results section could enhance clarity. An explanation of the utility of machine learning in classifying patient groups over conventional methods and the citation of original research articles, rather than relying on review articles, may also add clarity to the usefulness of the study.

    1. Reviewer #3 (Public Review):

      Summary

      The authors set out to formally contrast several theoretical models of working memory, being particularly interested in comparing the models regarding their ability to explain cueing effects at short cue durations. These benefits are traditionally attributed to the existence of a high capacity, rapidly decaying sensory storage which can be directly read out following short latency retro-cues. Based on the model fits, the authors alternatively suggest that cue-benefits arise from a freeing of working memory resources, which at short cue latencies can be utilized to encode additional sensory information into VWM.

      A dynamic neural population model consisting of separate sensory and VWM populations was used to explain temporal VWM fidelity of human behavioral data collected during several working memory tasks. VWM fidelity was probed at several timepoints during encoding, while sensory information was available and maintenance, when sensory information was no longer available. Furthermore, set size and exposure durations were manipulated to disentangle contributions of sensory and visual working memory.

      Overall, the model explained human memory fidelity well, accounting for set size, exposure time, retention time, error distributions and swap errors. Crucially the model suggests that recall at short delays is due to post-cue integration of sensory information into VWM as opposed to direct readout from sensory memory. The authors formally address several alternative theories, demonstrating that models with reduced sensory persistence, direct readout from sensory memory, no set-size dependent delays in cue processing and constant accumulation rate provide significantly worse fits to the data.

      I congratulate the authors for this rigorous scientific work. All my remarks were thoroughly addressed.

    1. Reviewer #2 (Public Review):

      Summary:

      The current work describes a set of behavioral tasks to explore individual differences in the preferred perceptual and motor rhythms. Results show a consistent individual preference for a given perceptual and motor frequency across tasks and, while these were correlated, the latter is slower than the former one. Additionally, the adaptation accuracy to rate changes is proportional to the amount of rate variation and, crucially, the amount of adaptation decreases with age.

      Strengths:

      Experiments are carefully designed to measure individual preferred motor and perceptual tempo. Furthermore, the experimental design is validated by testing the consistency across tasks and test-retest, what makes the introduced paradigm a useful tool for future research.<br /> The obtained data is rigorously analyzed using a diverse set of tools, each adapted to the specificities across the different research questions and tasks.<br /> This study identifies several relevant behavioral features: (i) each individual shows a preferred and reliable motor and perceptual tempo and, while both are related, the motor is consistently slower than the pure perceptual one; (ii) the presence of hysteresis in the adaptation to rate variations; and (iii) the decrement of this adaptation with age. All these observations are valuable for the auditory-motor integration field of research, and they could potentially inform existing biophysical models to increase their descriptive power.

      Weaknesses:

      To get a better understanding of the mechanisms underlying the behavioral observations, it would have been useful to compare the observed pattern of results with simulations done with existing biophysical models. However, this point is addressed if the current study is read along with this other publication of the same research group: Kaya, E., & Henry, M. J. (2024, February 5). Modeling rhythm perception and temporal adaptation: top-down influences on a gradually decaying oscillator. https://doi.org/10.31234/osf.io/q9uvr

    1. Reviewer #2 (Public Review):

      Summary:

      Tian et al. aimed to assess differences in biological motion (BM) perception between children with and without ADHD, as well as relationships to indices of social functioning and possible predictors of BM perception (including demographics, reasoning ability and inattention). In their study, children with ADHD showed poorer performance relative to typically developing children in three tasks measuring local, global, and general BM perception. The authors further observed that across the whole sample, performance in all three BM tasks was negatively correlated with scores on the social responsiveness scale (SRS), whereas within groups a significant relationship to SRS scores was only observed in the ADHD group and for the local BM task. Local and global BM perception showed a dissociation in that global BM processing was predicted by age, while local BM perception was not. Finally, general (local & global combined) BM processing was predicted by age and global BM processing, while reasoning ability mediated the effect of inattention on BM processing.

      Strengths:

      Overall, the manuscript is presented in a clear fashion and methods and materials are presented with sufficient detail so the study could be reproduced by independent researchers. The study uses an innovative, albeit not novel, paradigm to investigate two independent processes underlying BM perception. The results are novel and have the potential to have wide-reaching impact on multiple fields.

      Weaknesses:

      The manuscript has greatly improved in clarity and methodological considerations in response to the review. There are only a few minor points which deserve the authors' attention:

      When outlining the moviation for the current study, results from studies in ADHD and ASD are used too interchangeably. The authors use a lack of evidence for contributing (psychological/developmental) factors on BM processing in ASD to motivate the present study and refer to evidence for differences between typical and non-typical BM processing using studies in both ASD and ADHD. While there are certainly overlapping features between the two conditions/neurotypes, they are not to be considered identical and may have distinct etiologies, therefore the distinction between the two should be made clearer.

      In the first/main analysis, is unclear to me why in the revised manuscript the authors changed the statistical method from ANOVA/ANCOVA to independent samples t-tests (unless the latter were only used for post-hoc comparisons, then this needs to be stated). Furthermore, although p-values look robust, for this analysis too it should be indicated whether and how multiple comparison problems were accounted for.

    1. "Il résulte donc de ce qui précède, qu’en l’absence d’obstacle juridique, l’organe délibératif de l’EPLE est parfaitement libre d’adopter le principe d’une répartition de l’année scolaire en deux semestres, au lieu de trois trimestres. Une fois cette résolution arrêtée, il conviendra également de modifier en conséquence le règlement intérieur de l’établissement."

    1. She grades their results as if they haddone the writing entirely on their own.

      Surprising: This definitely surprised me seeing a professor going so far as to treat the result as if the students have done the writing entirely on their own. It definitely clashed with my previously held belief.

    2. “You will be expected to use AI generative tools in thisclass, following the instructor’s permissions and directions,”

      Interesting: I find this very interesting. This is the first time I have seen AI, when mostly prohibited or looked down upon in classroom setting is being used purposefully.

    3. Some, for example, require ascreenshot or link to the original text produced by the AI program, so they cansee how the student altered it.

      Troubling: It seems like this AI tool has become such a menace to both teachers and students in the acedemic realm and at this point I feel like it is doing more harm than good. Because students use it as a shortcut and professors are also worrying a lot more and requiring a lot more procedures just to grade an assignment such as:(screenshots, links, and even requirement them to submit notes and other artifacts of their work process) I feel like all this will only slow down the grading process and put more unecessary work for the ones in the teaching position.

    1. Reviewer #3 (Public Review):

      Summary:

      The manuscript by Huerlimann et al. entitled "The transcriptional landscape underlying metamorphosis in the Malabar grouper (Epinephelus malabaricus)." describes the transcriptional landscape of the Malabar grouper during selected metamorphic stages. The authors find evidence of dynamic regulation of HPT axis genes, TH signalling genes, and HPA and metabolic-related genes during post-natal development. Finally, the authors argue that the HPA is involved in grouper metamorphosis, given the related genes' dynamic expression during this developmental time.

      Strengths:

      The work is technically very good, and the methodology applied is solid.

      Weaknesses:

      However, the authors make substantial considerations that are not proven by experimental or functional data. In fact, this is a descriptive study that does not provide any functional evidence to support the claims made.

      The consideration that cortisol is involved in metamorphosis in teleosts has never been shown, and the only example cited by the authors (REF 20) clearly states that cortisol alone does not induce flatfish metamorphosis. In that work, the authors clearly state that in vivo cortisol treatment had no synergistic effect with TH in inducing metamorphosis. Moreover, in Senegalensis, the sole pre-otic CRH neuron number decreases during metamorphosis, further arguing that, at least in flatfish, cortisol is not involved in flatfish metamorphosis (PMID: 25575457). Furthermore, the authors need to recognise that the transcriptomic analysis is whole-body and that HPA axis genes are upregulated, which does not mean they are involved in regulating the HPT axis. The authors do not show that in thyrotrophs, any CRH receptor is expressed or in any other HPT axis-relevant cells and that changes in these genes correlate with changes in TSH expression. An in-situ hybridisation experiment showing co-expression on thyrotrophs of HPA genes and TSH could be a good start. However, the best scenario would be conducting cortisol treatment experiments to see if this hormone affects grouper metamorphosis.

      High TSH and Tg levels usually parallel whole-body TH levels during teleost metamorphosis. However, in this study, high Tg expression levels are only achieved at the juvenile stage, whereas high TSH is achieved at D32, and at the juvenile stage, they are already at their lowest levels.

      It is very difficult to conclude anything with the TH and cortisol levels measurements. The authors only measured up until D10, whereas they argue that metamorphosis occurs at D32. In this way, these measurements could be more helpful if they focus on the correct developmental time. The data is irrelevant to their hypothesis.

      Moreover, as stated in the previous review, a classical sign of teleost metamorphosis is the upregulation of TSHb and Tg, which does not occur at D32 therefore, it is very hard for me to accept that this is the metamorphic stage. With the lack of TH measurements, I cannot agree with the authors. I think this has to be toned down and made clear in the manuscript that D32 might be a putative metamorphic climax but that several aspects of biology work against it. Moreover, in D10, the authors show the highest cortisol level and lowest T4 and T3 levels. These observations are irreconcilable, with cortisol enhancing or participating in TH-driven metamorphosis.

      Given this, the authors should quantify whole-body TH levels throughout the entire developmental window considered to determine where the peak is observed and how it correlates with the other hormonal genes/systems in the analysis.

      Even though this is a solid technical paper and the data obtained is excellent, the conclusions drawn by the authors are not supported by their data, and at least hormonal levels should be present in parallel to the transcriptomic data. Furthermore, toning down some affirmations or even considering the different hypotheses available that are different from the ones suggested would be very positive.

    1. Reviewer #2 (Public Review):

      Summary and strengths:

      The article pertains to a topic of importance, specifically early life growth faltering, a marker of undernutrition, and how it influences brain functional connectivity and cognitive development. In addition, the data collection was laborious, and data preprocessing was quite rigorous to ensure data quality, utilizing cutting-edge preprocessing methods.

      Weaknesses:

      However, the subsequent analysis and explanations were not very thorough, which made some results and conclusions less convincing. For example, corrections for multiple tests need to be consistently maintained; if the results do not survive multiple corrections, they should not be discussed as significant results. Additionally, alternative plans for analysis strategies could be worth exploring, e.g., using ΔFC in addition to FC at a certain age. Lastly, some analysis plans lacked a strong theoretical foundation, such as the relationship between functional connectivity (FC) between certain ROIs and the development of cognitive flexibility.

      Thus, as much as I admire the advanced analysis of connectivity that was conducted and the uniqueness of longitudinal fNIRS data from these samples (even the sheer effort to collect fNIRS longitudinally in a low-income country at such a scale!), I have reservations about the importance of this paper's contribution to the field in its present form. Major revisions are needed, in my opinion, to enhance the paper's quality.

    1. Reviewer #2 (Public Review):

      Summary:

      The authors set out to test whether a TMS-induced reduction in excitability of the left Superior Frontal Sulcus influenced evidence integration in perceptual and value-based decisions. They directly compared behaviour - including fits to a computational decision process model - and fMRI pre and post-TMS in one of each type of decision-making task. Their goal was to test domain-specific theories of the prefrontal cortex by examining whether the proposed role of the SFS in evidence integration was selective for perceptual but not value-based evidence.

      Strengths:

      The paper presents multiple credible sources of evidence for the role of the left SFS in perceptual decision-making, finding similar mechanisms to prior literature and a nuanced discussion of where they diverge from prior findings. The value-based and perceptual decision-making tasks were carefully matched in terms of stimulus display and motor response, making their comparison credible.

      Weaknesses:<br /> More information on the task and details of the behavioural modelling would be helpful for interpreting the results. I had the following concerns:

      (1) The evidence for a choice and 'accuracy' of that choice in both tasks was determined by a rating task that was done in advance of the main testing blocks (twice for each stimulus). For the perceptual decisions, this involved asking participants to quantify a size metric for the stimuli, but the veracity of these ratings was not reported, nor was the consistency of the value-based ones. It is my understanding that the size ratings were used to define the amount of perceptual evidence in a trial, rather than the true size differences, and without seeing more data the reliability of this approach is unclear. More concerning was the effect of 'evidence level' on behaviour in the value-based task (Figure 3a). While the 'proportion correct' increases monotonically with the evidence level for the perceptual decisions, for the value-based task it increases from the lowest evidence level and then appears to plateau at just above 80%. This difference in behaviour between the two tasks brings into question the validity of the DDM which is used to fit the data, which assumes that the drift rate increases linearly in proportion to the level of evidence.

      (2) The paper provides very little information on the model fits (no parameter estimates, goodness of fit values or simulated behavioural predictions). The paper finds that TMS reduced the decision bound for perceptual decisions but only affected non-decision time for value-based decisions. It would aid the interpretation of this finding if the relative reliability of the fits for the two tasks was presented.

      (3) Behaviourally, the perceptual task produced decreased response times and accuracy post-TMS, consistent with a reduced bound and consistent with some prior literature. Based on the results of the computational modelling, the authors conclude that RT differences in the value-based task are due to task-related learning, while those in the perceptual task are 'decision relevant'. It is not fully clear why there would be such significantly greater task-related learning in the value-based task relative to the perceptual one. And if such learning is occurring, could it potentially also tend to increase the consistency of choices, thereby counteracting any possible TMS-induced reduction of consistency?

    1. Reviewer #2 (Public Review):

      In this study, the authors aim to understand how neurons in the anterior insular cortex (insula) modulate fear behaviors. They report that the activity of a subpopulation of insula neurons is positively correlated with freezing behaviors, while the activity of another subpopulation of neurons is negatively correlated to the same freezing episodes. They then used optogenetics and showed that activation of anterior insula excitatory neurons during tones predicting a footshock increases the amount of freezing outside the tone presentation, while optogenetic inhibition had no effect. Finally, they found that two neuronal projections of the anterior insula, one to the amygdala and another to the medial thalamus, are increasing and decreasing freezing behaviors respectively. While the study contains interesting and timely findings for our understanding of the mechanisms underlying fear, some points remain to be addressed.

    1. Reviewer #2 (Public Review):

      Summary:

      In Cheong et al., the authors analyze a new motor system (ventral nerve cord) connectome of Drosophila. Through proofreading, cross-referencing with another female VNC connectome, they define key features of VNC circuits with a focus on descending neurons (DNs), motor neurons (MNs), and local interneuron circuits. They define DN tracts, MNs for limb and wing control, and their nerves (although their sample suffers for a subset of MNs). They establish connectivity between DNs and MNs (minimal). They perform topological analysis of all VNC neurons including interneurons. They focus specifically on identifying core features of flight circuits (control of wings and halteres), leg control circuits with a focus on walking rather than other limbed behaviors (grooming, reaching, etc.), and intermediate circuits like those for escape (GF). They put these features in the context of what is known or has been posited about these various circuits.

      Strengths:

      Some strengths of the manuscript include the matching of new DN and MN types to light microscopy, including the serial homology of leg motor neurons. This is a valuable contribution that will certainly open up future lines of experimental work.

      Also, the analysis of conserved connectivity patterns within each leg neuromere and interconnecting connectivity patterns between neuromeres will be incredibly valuable. The standard leg connectome is very nice.

      Finally, the finding of different connectivity statistics (degrees of feedback) in different neuropils is quite interesting and will stimulate future work aimed at determining its functional significance.

      Weaknesses:

      First, it seems like quite a limitation that the neurotransmitter predictions were based on training data from a fairly small set of cells, none of which were DNs. It's wonderful that the authors did the experimental work to map DN neurotransmitter identity using FISH, and great that the predictions were overall decently accurate for both ACh and Glu, but unfortunate that they were not accurate for GABA. I hope there are plans to retrain the neurotransmitter predictions using all of this additional ground truth experimental data that the authors collected for DNs, in order to provide more accurate neurotransmitter type predictions across more cell types.

      Second, the degradation of many motor neurons is unfortunate. Figure 5 Supplement 1 shows that roughly 50% of the leg motor neurons have significantly compromised connectivity data, whereas, for non-leg motor neurons, few seem to be compromised. If that is the correct interpretation of this figure, perhaps a sentence like this that includes some percentages (~50% of leg MNs, ~5% of other MNs) could be added to the main text so that readers can get a sense of the impact more easily.

      As well, Figure 5 Supplement 1 caption says "Note that MN groups where all members of the group have reconstruction issues may not be flagged" - could the authors comment on how common they think this is based on manual inspection? If it changes the estimate of the percentage of affected leg motor neurons from 50% to 75% for example, this caveat in the current analysis would need to be addressed more directly. Comparing with FANC motor neurons could perhaps be an alternative/additional approach for estimating the number of motor neurons that are compromised.

      This analysis might benefit from some sort of control for true biological variability in the number of MN synapses between left and right or across segments. I assume the authors chose the threshold of 0.7 because it seemed to do a good job of separating degraded neurons from differences in counts that could just be due to biological variability or reconstruction imperfections, but perhaps there's some way to show this more explicitly. For example, perhaps show how much variability there is in synapse counts across all homologs for one or two specific MN types that are not degraded and are reconstructed extremely well, so any variability in input counts for those neurons is likely to be biologically real. Especially because the identification of serial homologs among motor neurons is a key new contribution of this paper, a more in-depth analysis of similarities and differences in homologous leg MNs across segments could be interesting to the field if the degradation doesn't preclude it.

      Fourth, the infomap communities don't seem to be so well controlled/justified. Community detection can be run on any graph - why should I believe that the VNC graph is actually composed of discrete communities? Perhaps this comes from a lack of familiarity with the infomap algorithm, but I imagine most readers will be similarly unfamiliar with it, so more work should be done to demonstrate the degree to which these communities are really communities that connect more within than across communities.

      I think the length of this manuscript reduces its potential for impact, as I suspect the reality is that many people won't read through all 140 pages and 21 main figures of (overall excellent) work and analysis.

    1. Reviewer #2 (Public Review):

      Summary:

      kTMP is a novel method of stimulating the brain using electromagnetic fields. It has potential benefits over existing technology because it is safe and easy. It explores a range of brain frequencies that have not been explored in depth before (2-5kHz) and thus offers new opportunities.

      Strengths:

      This work relied on standard methods and was carefully and conservatively performed.

      Weaknesses:

      The sham condition was prepared as well as could be done, but sham is always challenging in a treatment with sound and sensation and with knowledgeable operators. New technology, also, is very exciting to subjects and it is difficult to achieve a natural experiment. These difficulties are related to the technology, however, and not to the execution of these experiments.

    1. Reviewer #2 (Public Review):

      Summary:

      The manuscript by Isotani et al characterizes the hyperproliferation of intestinal stem cells (ISCs) induced by nicotine treatment in vivo. Employing a range of small molecule inhibitors, the authors systematically investigated potential receptors and downstream pathways associated with nicotine-induced phenotypes through in vitro organoid experiments. Notably, the study specifically highlights a signaling cascade involving α7-nAChR/PKC/YAP/TAZ/Notch as a key driver of nicotine-induced stem cell hyperproliferation. Utilizing a Lgr5CreER Apcfl/fl mouse model, the authors extend their findings to propose a potential role of nicotine in stem cell tumorgenesis. The study posits that Notch signaling is essential during this process.

      Strengths and Weaknesses:

      One noteworthy research highlight in this study is the indication, as shown in Figure 2 and S2, that the trophic effect of nicotine on ISC expansion is independent of Paneth cells. In the Discussion section, the authors propose that this independence may be attributed to distinct expression patterns of nAChRs in different cell types. To further substantiate these findings, it is suggested that the authors perform tissue staining of various nAChRs in the small intestine and colon. This additional analysis would provide more conclusive evidence regarding how stem cells uniquely respond to nicotine. It is also recommended to present the staining of α7-nAChR from different intestinal regions. This will provide insights into the primary target sites of nicotine in the gut tract. Additionally, it is recommended that the authors consider rephrasing the conclusion in this section (lines 123-124). The current statement implies that nicotine does not affect Paneth cells, which may be inaccurate based on the suggestion in line 275 that nicotine might influence Paneth cells through α2β4-nAChR. Providing a more nuanced conclusion would better reflect the complexity of nicotine's potential impact on Paneth cells.

      As shown in the same result section, the effect of nicotine on ISC organoid formation appears to be independent of CHIR99021, a Wnt activator. Despite this, the authors suggest a potential involvement of Wnt/β-catenin activation downstream of nicotine in Figure 4F. In the Lgr5CreER Apcfl/fl mouse model, it is known that APC loss results in a constitutive stabilization of β-catenin, thus the hyperproliferation of ISCs by nicotine treatment in this mouse model is likely beyond Wnt activation. Therefore, it is recommended that the authors reconsider the inclusion of Wnt/β-catenin as a crucial signaling pathway downstream of nicotine, given the experimental evidence provided in this study.

      In Figure 4, the authors investigate ISC organoid formation with a pan-PKC inhibitor, revealing that PKC inhibition blocks nicotine-induced ISC expansion. It's noteworthy that PKC inhibitors have historically been used successfully to isolate and maintain stem cells by promoting self-renewal. Therefore, it is surprising to observe no effect or reversal effect on ISCs in this context. A previous study demonstrated that the loss of PKCζ leads to increased ISC activity both in vivo and in vitro (DOI: 10.1016/j.celrep.2015.01.007). Additionally, to strengthen this aspect of the study, it would be beneficial for the authors to present more evidence, possibly using different PKC inhibitors, to reproduce the observed results with Gö 6983. This could help address potential concerns or discrepancies and contribute to a more comprehensive understanding of the role of PKC in nicotine-induced ISC expansion.

      An additional avenue that could enhance the clinical relevance of the study is the exploration of human datasets. Specifically, leveraging scRNA-seq datasets of the human intestinal epithelium (DOI: 10.1038/s41586-021-03852-1) could provide valuable insights. Analyzing the expression patterns of nAChRs across diverse regions and cell types in the human intestine may offer a potential clinical implication.

      In summary, the results generally support the authors' conclusions that nicotine directly influences ISC growth, potentially contributing to tumorgenesis. The identification of the α7-nAChR/PKC/YAP/TAZ/Notch pathway adds significant mechanistic insight. However, certain aspects of the experimental evidence, such as the receptor expression pattern, PKC inhibition response, and the involvement of Wnt/β-catenin activation, may require further clarification and exploration, especially considering previous literature suggesting potential discrepancies.

    1. Reviewer #2 (Public Review):

      Summary:

      The study provides strong evidence that leaf microbes mediate self-limitation at an early life stage. It highlights the importance of leaf microbes in population establishment and community dynamics.

      The authors conducted three experiments to test their hypothesis, elucidating the effects of leaf and soil microbial communities on the seedling growth of A. adenophora at different stages, screening potential microbial sources associated with seed germination and seedling performance, and identifying the fungus related to seedling mortality. The conclusions are justified by their results. Overall, the paper is well-structured, providing clear and comprehensive information.

    1. Reviewer #2 (Public Review):

      Summary:

      Dantzer and colleagues are investigating the pivotal role of ß-catenin, a gene that undergoes mutation in various cancer cells, and its influence on promoting the evasion of immune cells. In their initial experiments, the authors developed a HepG2 mutated ß-catenin KD model, conducting transcriptional and proteomic analyses. The results revealed that the silencing of mutated ß-catenin in HepG2 cells led to an up-regulation in the expression of exosome biogenesis genes.

      Furthermore, the researchers verified that these KD cells exhibited increased production of exosomes, with the mutant form of ß-catenin concurrently decreasing the expression of SDC4 and Rab27a. Intriguingly, applying a GSK inhibitor to the cells resulted in reduced expression of SDC4 and Rab27a. Subsequent findings indicated that mutated ß-catenin actively facilitates immune escape through exosomes, and silencing exosome biogenesis correlates with a decrease in immune cell infiltration.<br /> In a crucial clinical correlation, the study demonstrated that patients with ß-catenin mutations exhibited low levels of exosome biogenesis.

      Strengths:

      Overall, the data robustly supports the outlined conclusions, and the study is commendably designed and executed. However, there are a few suggestions for manuscript improvement.

      Weaknesses:<br /> No weaknesses were identified by this reviewer.

    1. Reviewer #2 (Public Review):

      Summary:

      In this work, Vivian Salgueiro et al. have comprehensively investigated the role of VirR in the vesicle production process in Mtb using state-of-the-art omics, imaging, and several biochemical assays. From the present study, authors have drawn a positive correlation between cell membrane permeability and vasculogenesis and implicated VirR in affecting membrane permeability, thereby impacting vasculogenesis.

      Strengths:

      The authors have discovered a critical factor (i.e. membrane permeability) that affects vesicle production and release in Mycobacteria, which can broadly be applied to other bacteria and may be of significant interest to other scientists in the field. Through omics and multiple targeted assays such as targeted metabolomics, PG isolation, analysis of Diaminopimelic acid and glycosyl composition of the cell wall, and, importantly, molecular interactions with PG-AG ligating canonical LCP proteins, the authors have established that VirR is a central scaffold at the cell envelope remodelling process which is critical for MEV production.

      Weaknesses:

      Throughout the study, the authors have utilized a CRISPR knockout of VirR. VirR is a non-essential gene for the growth of Mtb; a null mutant of VirR would have been a better choice for the study.

    1. Reviewer #2 (Public Review):

      Summary:

      The phytopathogenic bacterium Pseudomonas syringae is comprised of many pathovars with different host plant species and has been used as a model organism to study bacterial pathogenesis in plants. Transcriptional regulation is key to plant infection and adaptation to host environments by this bacterium. However, researchers have focused on a limited number of transcription factors (TFs) that regulate virulence-related pathways. Thus, a comprehensive, systems-level understanding of regulatory interactions between transcription factors in P. syringae has not been achieved.

      This study by Sun et al performed ChIP-seq analysis of 170 out of 301 TFs in P. syringae pv. syringae 1448A and used this unique dataset to infer transcriptional regulatory networks in this bacterium. The network analyses revealed hierarchical interactions between TFs, various network motifs, and co-regulation of target genes by TF pairs, which collectively mediate information flow. As discussed, the structure and properties of the P. syringae transcriptional regulatory networks are somewhat different from those identified in humans, yeast, and E. coli, highlighting the significance of this study. Further, the authors made use of the P. syringae transcriptional regulatory networks to find TFs of unknown functions to be involved in virulence-related pathways. For some of these TFs, their target specificity and biological functions, such as motility and biofilm formation, were experimentally validated. Of particular interest is the finding that despite conservation of TFs between P. syringae pv. syringae 1448A, P. syringae pv. tomato DC3000, P. syringae pv. syringae B728a, and P. syringae pv. actinidiae C48, some of the conserved TFs show different repertoires of target genes in these four P. syringae strains.

      Strengths:

      This study presents a systems-level analysis of transcriptional regulatory networks in relation to P. syringae virulence and metabolism, and highlights differences in transcriptional regulatory landscapes of conserved TFs between different P. syringae strains, and develops a user-friendly database for mining the ChIP-seq data generated in this study. These findings and resources will be valuable to researchers in the fields of systems biology, bacteriology, and plant-microbe interactions.

      Weaknesses:

      No major weaknesses were found, but some of the results may need to be interpreted with caution. ChIP-seq was performed with bacterial strains overexpressing TFs. This may cause artificial binding of TFs to promoters which may not occur when TFs are expressed at physiological levels. Another caution is applied to the interpretation of the biological functions of TFs. The biological roles of the tested TFs are based on in vitro experiments. Thus, functional relevance of the tested TFs during plant infection and/or survival under natural environmental conditions remains to be demonstrated.

    1. Reviewer #2 (Public Review):

      Summary:<br /> Schmidlin & Apodaca et al. aim to distinguish mutants that resist drugs via different mechanisms by examining fitness tradeoffs across hundreds of fluconazole-resistant yeast strains. They barcoded a collection of fluconazole-resistant isolates and evolved them in different environments with a view to having relevance for evolutionary theory, medicine, and genotype-phenotype mapping.

      Strengths:<br /> There are multiple strengths to this paper, the first of which is pointing out how much work has gone into it; the quality of the experiments (the thought process, the data, the figures) is excellent. Here, the authors seek to induce mutations in multiple environments, which is a really large-scale task. I particularly like the attention paid to isolates with are resistant to low concentrations of FLU. So often these are overlooked in favour of those conferring MIC values >64/128 etc. What was seen is different genotype and fitness profiles. I think there's a wealth of information here that will actually be of interest to more than just the fields mentioned (evolutionary medicine/theory).

      Weaknesses:<br /> Not picking up low fitness lineages - which the authors discuss and provide a rationale as to why. I can completely see how this has occurred during this research, and whilst it is a shame I do not think this takes away from the findings of this paper. Maybe in the next one!

      In the abstract the authors focus on 'tradeoffs' yet in the discussion they say the purpose of the study is to see how many different mechanisms of FLU resistance may exist (lines 679-680), followed up by "We distinguish mutants that likely act via different mechanisms by identifying those with different fitness tradeoffs across 12 environments". Whilst I do see their point, and this is entirely feasible, I would like a bit more explanation around this (perhaps in the intro) to help lay-readers make this jump. The remainder of my comments on 'weaknesses' are relatively fixable, I think:

      In the introduction I struggle to see how this body of research fits in with the current literature, as the literature cited is a hodge-podge of bacterial and fungal evolution studies, which are very different! So example, the authors state "previous work suggests that mutants with different fitness tradeoffs may affect fitness through different molecular mechanisms" (lines 129-131) and then cite three papers, only one of which is a fungal research output. However, the next sentence focuses solely on literature from fungal research. Citing bacterial work as a foundation is fine, but as you're using yeast for this I think tailoring the introduction more to what is and isn't known in fungi would be more appropriate. It would also be great to then circle back around and mention monotherapy vs combination drug therapy for fungal infections as a rationale for this study. The study seems to be focused on FLU-resistant mutants, which is the first-line drug of choice, but many (yeast) infections have acquired resistance to this and combination therapy is the norm.

      Methods: Line 769 - which yeast? I haven't even seen mention of which species is being used in this study; different yeast employ different mechanisms of adaptation for resistance, so could greatly impact the results seen. This could help with some background context if the species is mentioned (although I assume S. cerevisiae). In which case, should aneuploidy be considered as a mechanism? This is mentioned briefly on line 556, but with all the sequencing data acquired this could be checked quickly?

      I think the authors could be bolder and try and link this to other (pathogenic) yeasts. What are the implications of this work on say, Candida infections?

    1. Reviewer #2 (Public Review):

      Summary:

      Schwartzkopf et al characterized the meiotic recombination impact of highly heterozygous introgressed regions within the budding yeast Saccharomyces uvarum, a close relative of the canonical model Saccharomyces cerevisiae. To do so, they took advantage of the naturally occurring Saccharomyces bayanus introgressions specifically within fermentation isolates of S. uvarum and compared their behavior to the syntenic regions of a cross between natural isolates that do not contain such introgressions. Analysis of crossover (CO) and noncrossover (NCO) recombination events shows both a depletion in CO frequency within highly heterozygous introgressed regions and an increase in NCO frequency. These results strongly support the hypothesis that DNA sequence polymorphism inhibits CO formation, and has no or much weaker effects on NCO formation. Eventually, the authors show that the presence of introgressions negatively impacts "r", the parameter that reflects the probability that a randomly chosen pair of loci shuffles their alleles in a gamete.

      The authors chose a sound experimental setup that allowed them to directly compare recombination properties of orthologous syntenic regions in an otherwise intra-specific genetic background. The way the analyses have been performed looks right, although this reviewer is unable to judge the relevance of the statistical tests used. Eventually, most of their results which are elegant and of interest to the community are present in Figure 2.

      Strengths:

      Analysis of crossover (CO) and noncrossover (NCO) recombination events is compelling in showing both a depletion in CO frequency within highly heterozygous introgressed regions and an increase in NCO frequency.

      Weaknesses:

      The main weaknesses refer to a few text issues and a lack of discussion about the mechanistic implications of the present findings.

      - Introduction

      The introduction is rather long. I suggest specifically referring to "meiotic" recombination (line 71) and to "meiotic" DSBs (line 73) since recombination can occur outside of meiosis (ie somatic cells).

      From lines 79 to 87: the description of recombination is unnecessarily complex and confusing. I suggest the authors simply remind that DSB repair through homologous recombination is inherently associated with a gene conversion tract (primarily as a result of the repair of heteroduplex DNA by the mismatch repair (MMR) machinery) that can be associated or not to a crossover. The former recombination product is a crossover (CO), the latter product is a noncrossover (NCO) or gene conversion. Limited markers may prevent the detection of gene conversions, which erase NCO but do not affect CO detection.

      In addition, "resolution" in the recombination field refers to the processing of a double Holliday junction containing intermediates by structure-specific nucleases. To avoid any confusion, I suggest avoiding using "resolution" and simply sticking with "DSB repair" all along the text.

      Note that there are several studies about S. cerevisiae meiotic recombination landscapes using different hybrids that show different CO counts. In the introduction, the authors refer to Mancera et al 2008, a reference paper in the field. In this paper, the hybrid used showed ca. 90 CO per meiosis, while their reference to Liu et al 2018 in Figure 2 shows less than 80 COs per meiosis for S. cerevisiae. This shows that it is not easy to come up with a definitive CO count per meiosis in a given species. This needs to be taken into account for the result section line 315-321.

      In line 104, the authors refer to S. paradoxus and mention that its recombination rate is significantly different from that of S. cerevisiae. This is inaccurate since this paper claims that the CO landscape is even more conserved than the DSB landscape between these two species, and they even identify a strong role played by the subtelomeric regions. So, the discussion about this paper cannot stand as it is.

      Line 150, when the authors refer to the anti-recombinogenic activity of the MMR, I suggest referring to the published work from Martini et al 2011 rather than the not-yet-published work from Copper et al 2021, or both, if needed.

      Results

      The clear depletion in CO and the concomitant increase in NCO within the introgressed regions strongly suggest that DNA sequence polymorphism triggers CO inhibition but does not affect NCO or to a much lower extent. Because most CO likely arises from the ZMM pathway (CO interference pathway mainly relying on Zip1, 2, 3, 4, Spo16, Msh4, 5, and Mer3) in S. uvarum as in S. cerevisiae, and because the effect of sequence polymorphism is likely mediated by the MMR machinery, this would imply that MMR specifically inhibits the ZMM pathway at some point in S. uvarum.

      The weak effect or potential absence of the effect of sequence polymorphism on NCO formation suggests that heteroduplex DNA tracts, at least the way they form during NCO formation, escape the anti-recombinogenic effect of MMR in S. uvarum. A few comments about this could be added.

      The same applies to the fact that the CO number is lower in the natural cross compared to the fermentation cross, while the NCO number is the same. This suggests that under similar initiating Spo11-DSB numbers in both crosses, the decrease in CO is likely compensated by a similar increase in inter-sister recombination.

      Introgressions represent only 10% of the genome, while the decrease in CO is at least 20%. This is a bit surprising especially in light of CO regulation mechanisms such as CO homeostasis that tends to keep CO constant. Could the authors comment on that?

      Finally, the frequency of NCOs in introgressed regions is about twice the frequency of CO in non-introgressed regions. Both CO and NCO result from Spo11-initiating DSBs. This suggests that more Spo11-DSBs are formed within introgressed regions and that such DSBs specifically give rise to NCO. Could this be related to the lack of homolog engagement which in turn shuts down Spo11-DSB formation as observed in ZMM mutants by the Keeney lab? Could this simply result from better detection of NCO in introgressed regions related to the increased marker density, although the authors claim that NCO counts are corrected for marker resolution?

      What could be the explanation for chromosome 12 to have more shuffling in the natural cross compared to the fermentation cross which is deprived of the introgressed region?

      Technical points:

      - In line 248, the authors removed NCO with fewer than three associated markers.<br /> What is the rationale for this? Is the genotyping strategy not reliable enough to consider events with only one or two markers? NCO events can be rather small and even escape detection due to low local marker density.

      - Line 270: The way homology is calculated looks odd to this reviewer, especially the meaning of 0.5 homology. A site is either identical (1 homology) or not (0 homology).

      - Line 365: beware that the estimates are for mitotic mismatch repair (MMR). Meiotic MMR may work differently.

      - Figure 1: there is no mention of potential 4:0 segregations. Did the authors find no such pattern? If not, how did they consider them?

    1. Reviewer #2 (Public Review):

      Summary:

      In this manuscript, Liu et al. identified an important pathway regulating the nuclear translocation of the key transcriptional factor FOG1 during human hematopoiesis. The authors show that heat shock cognate B (HSCB) can interact with and promote the proteasomal degradation of TACC3, and this function is independent of its role in iron-sulfur cluster (ISC) biogenesis. TACC3 represses the activity of FOG1 by sequestering it in the cytoplasm. Therefore, HSCB can promote the nuclear translocation of FOG1 through down-regulating TACC3. The authors further show that the phosphorylation of HSCB by PI3K downstream of the EPO signaling pathway is important for its role in regulating the nuclear translocation of FOG1. The data are solid and the manuscript is overall well written. The findings of this manuscript provide new knowledge to the fields of hematopoiesis and cell biology.

      Strengths:

      This study uses a multi-pronged approach that combines techniques from a number of fields to convincingly demonstrate the pathway regulating the nuclear translocation of FOG1 during hematopoiesis.

      Weaknesses:

      This study only uses cell models. The significance of this work may be broadened by further studies using animal models.

    1. Reviewer #2 (Public Review):

      Summary:<br /> An analysis of images in the biology literature that are problematic for people with a color-vision deficiency (CVD) is presented, along with a machine learning-based model to identify such images and a web application that uses the model to flag problematic images. Their analysis reveals that about 13% of the images could be problematic for people with CVD and that the frequency of such images decreased over time. Their model yields 0.89 AUC score. It is proposed that their approach could help making biology literature accessible to diverse audiences.

      Strengths:<br /> The manuscript focuses on an important yet mostly overlooked problem, and makes contributions both in expanding our understanding of the extent of the problem and in developing solutions to mitigate the problem. The paper is generally well-written and clearly organized. Their CVD simulation combines five different metrics. The dataset has been assessed by two researchers and is likely to be of high-quality. Machine learning algorithm used (convolutional neural network, CNN) is an appropriate choice for the problem. The evaluation of various hyperparameters for the CNN model is extensive.

      Weaknesses:<br /> The focus seems to be on one type of CVD (deuteranopia) and it is unclear whether this would generalize to other types. The dataset consists of images from eLife articles. While this is a reasonable starting point, whether this can generalize to other biology/biomedical articles is not assessed. "Probably problematic" and "probably okay" classes are excluded from the analysis and classification, and the effect of this exclusion is not discussed. Machine learning aspects can be explained better, in a more standard way. The evaluation metrics used for validating the machine learning models seem lacking (e.g., precision, recall, F1 are not reported). The web application is not discussed in any depth.

    1. Reviewer #3 (Public Review):

      Summary:

      Bernou et al. propose the existence of a distinct neuroblast population with increased regenerative and differentiation potential. Their claims are based on the analysis of a sorted population identified as LeX-EGFR+CD24low, which they refer to as "immature NeuroBlasts, iNB". This population is defined by transcriptomics features that have been assessed through bulk microarray studies of sorted cells and single cell RNA sequencing of the whole SVZ- lineage. Analysis of these data sets leads to the identification of these iNBs as cycling cells with a specific expression pattern of RNA splicing machinery components. On these grounds, they propose that RNA splicing plays a key role in neuronal differentiation. Although the authors bring an innovative point to the table, their claims are not fully supported by their results.

      Strengths:

      Interesting Hypothesis

      Weaknesses:

      The comparison of their microarray data to published single-cell RNA sequencing datasets (scRNAseq) highlights the cycling nature of the iNB population. Moreover, their own cell cycle analysis on their scRNAseq data attributes G2M/S-phase stages to clusters classified as iNBs, while clusters identified as TAPs are assigned to a restricted G1/S-phase stage. However, it would be expected that TAPs, as cycling progenitors, would go through all cell cycle stages and not just the beginning of it. Thus, authors should consider the possibility that their iNB population entails a major fraction of transit amplifying progenitors (TAP) and a couple neuroblasts, as described in numerous previous studies.

      Authors regard the iNB population as neuroblasts due to the capacity of their sorted population to proliferate and differentiate into diverse neural cell types (neurons, oligodendrocytes and astrocytes) in vitro. It cannot be discarded that the sorted population (LeX-EGFR+CD24low) may not be pure and may be composed of a mixture of cells in different stages, including TAPs. Such a mixture of different cell types is unavoidable in sorted populations analyzed as bulk and is precisely one of the issues solved by single cell transcriptomics. Thus, the analysis of single cells resolves transition states at higher resolution and should be preferred over bulk analysis to prevent biases in analysis.

      To align the authors' findings with the existing body of literature and earlier characterizations of the SVZ niche, it is advisable to combine their single-cell RNA sequencing data with datasets that have already been published. Such integration will enable precise understanding of the identity of their iNB cells.

      On another note, the role of RNA splicing on neurogenesis lacks experimental validation. Unless manipulation of RNA splicing factors is conducted, the key role of this machinery in adult neurogenesis cannot be claimed.

    1. Reviewer #2 (Public Review):

      Summary:

      The manuscript by Salinas-Pena et. al examines the distribution of a subgroup of histone H1 variants primarily with the use of high-resolution microscopy. The authors find that while some H1s have a universal distribution pattern, some display a preference for discrete regions within the nuclear landscape namely, the periphery, the center, or the nucleolus. They also show using that the various H1s within a cell did not colocalize significantly with each other, rather, they occupy discrete 'nanodomains' throughout the nucleus which is visualized as a punctate signal.<br /> The authors present evidence towards a long-standing question in the field regarding the spatial distribution of the different H1 variants. Since reliable, specific antibodies toward the variants were unavailable, this question was unable to elicit a definitive answer. This study uses more recently available antibodies against endogenous H1s to put together a systematic and comprehensive view of a group of H1 variant distribution inside a nucleus and ties it with previously generated genome wide data to demonstrate localization and some functional heterogeneity.

      Strengths of the study.

      (1) First systematic, high-resolution view of H1 variants providing a significant advance towards the long hypothesized functional differences between H1 variants.

      (2) The use of endogenous antibodies allows the authors to bypass the need to use tagged proteins or overexpression strategies to study H1 distribution.

      (3) The availability of genome wide H1 distribution data for the variants using the endogenous H1 antibodies to strengthen the presented visual data.

      Weakness of the study.

      One of the major reasons for slow progress in deciphering variant specific function has been the dearth of quality, specific, antibodies. This study is heavily dependent on the antibody function and its ability to accurately report on the distribution. The authors have cited previous validations of the antibodies used using H1 knockdown, immunoblotting and ChIP-seq. For the scope of this study, the controls are adequate.

      Impact:

      This study sets the stage for an exciting avenue of H1 study where variant-specific cellular functions can be explored which has otherwise been severely understudied.

    1. Reviewer #2 (Public Review):

      Yang et al. recorded the activity of D1- and D2-MSNs in the dorsal striatum and analyzed their firing activity in relation to single-limb gait in normal and 6-OHDA lesioned mice. The authors provided evidence that the striatal D1- and D2-MSNs were phase-locked to the walking gait cycles of individual limbs, and dopamine lesions led to enhanced phase-locking between D2-MSN activity and walking gait cycles.

      Comments on revised version:

      The authors addressed my largest concern, which questioned if D1 and D2 MSNs phase-locked to single limbs better than the global gait cycles.

      As to my second major concern, which questioned the causal significance of single limb gait coding in D1 and D2 MSNs on gait control, they performed additional optogenetic experiments to establish evidence that D2 activity is causally relevant for gait pattern control. The additional experiments also closed the logic gap between dopamine lesion, D2 activity and gait control, supporting the hypothesis that dopamine affects gait control and global movement pattern via increasing D2 MSN activity.

    1. Reviewer #2 (Public Review):

      Summary:

      Nonalcoholic fatty liver disease (NASH), recently renamed as metabolic dysfunction-associated steatohepatitis (MASH) is a leading cause of liver-related death. Farnesoid X receptor (FXR) is a promising drug target for treating NASH and several drugs targeting FXR is under clinical investigation for its efficacy in treating NASH. The authors intended to address whether FXR mediates its hepatic protective effects through regulation of lncRNAs, which would provide novel insights into the pharmacological targeting of FXR for NASH treatment. The authors went from an unbiased transcriptomics profiling to identify a novel enhancer-derived lncRNA FincoR enriched in the liver and showed that the knockdown of FincoR in a murine NASH model attenuated part of the effect of tropifexor, an FXR agonist, namely inflammation and fibrosis, but not steatosis. This study provides a framework how one can investigate the role of noncoding genes in pharmacological intervention targeting a known protein coding genes. Given that many disease-associated genetic variants are located in the non-coding regions, this study, together with others, may provide useful information for improved and individualized treatment for metabolic disorders.

      Strengths:

      The study leverages both transcriptional profile and epigenetic signatures to identify the top candidate eRNA for further study. The subsequent biochemical characterization of FincoR using FXR-KO mice combined with Gro-seq and Luciferase reporter assays convincingly demonstrates this eRNA as a FXR transcriptional targets sensitive to FXR agonists. The use of in vitro culture cells and the in vivo mouse model of NASH provide multi-level evaluation of the context-dependent importance of the FincoR downstream of FXR in regulation of functions related to liver dysfunction.

      Weaknesses:

      Future work to dissect the detailed mechanisms by which FincoR facilitates action of FXR and its agonists is warranted. A more direct approach to alter eRNA levels, e.g., overexpression of FincoR in the liver would provide important data to interpret its functional regulation.

    1. Reviewer #4 (Public Review):

      Summary:

      In this work, the authors have used a mouse model of familial Amyotrophic lateral sclerosis (ALS) that carries a G93A mutation in the Sod1 gen to understand how the extraocular muscles (EOM) are preserved in ALS while other muscles undergo degeneration. Interestingly, the authors demonstrate that the integrity of neuromuscular junctions (NMJ) is affected by ALS in the limb and diaphragm muscles of G93A mice, while EOM is mostly preserved. The authors also further demonstrate that NaBu treatment partially restores the integrity of NMJ in the limb and diaphragm muscles of G93A mice. The results also indicate that chemokine Cxcl12 is expressed at higher levels in EOM myoblasts, and transduction with AAV encoding Cxcl12 improved the phenotypic characteristics of hindlimb-derived satellite cells.

      Strengths:

      The authors have used both in vivo and cell culture models. The findings have a translational potential.

      Weaknesses:

      The use of NaBu could be an issue as it has multiple effects and targets in ALS.

      The sample size of animal experiments still needs to be improved.

      The molecular mechanism of how Cxcl12 improved the phenotypic characteristics of hindlimb-derived satellite cells is still being determined.

    1. Reviewer #2 (Public Review):

      Summary:<br /> This is an interesting study that seeks to identify novel mosquito repellents that smell attractive to humans.

      Strengths:<br /> The combination of standard machine learning methods with mosquito behavioral tests is a strength.

      Weaknesses:<br /> The study would be strengthened by describing how other modern ML approaches (RF, decision trees) would classify and identify other potential repellents.

      A comparison in the repellent activity between DEET and the top ten hits identified in this new study indicates little change in repellent activity (~3%), suggesting that DEET remains the gold standard. Without additional toxicity tests, the study is arguably incremental. The study's novelty should be better clarified.

      The Methods in the repellency tests are sparse, and more information would be useful. Testing the top repellents at low doses (<<1%) and for long periods (2-12 h) would strengthen the manuscript. Without this information, the manuscript is lacking in depth.

      Testing human subjects on their olfactory perceptions of the repellents would also increase the depth and utility of the manuscript. Without additional experiments, the authors' conclusions lack support and have limited impact on the state-of-the-art.

      This manuscript is a mix of different approaches, which makes it lack cohesion. There is the ML method for classifying new repellents that smell good, but no testing of the repellents on human volunteers. The repellents are not tested at realistic concentrations and durations. And the calcium mobilization test is strange and makes little sense in the context of the other experiments and framing of the manuscript.

    1. Reviewer #2 (Public Review):

      Summary:

      Using a combination of in vivo studies with testosterone-inhibited and aged mice with lower testosterone levels, as well as isolated mouse and human seminal vesicle epithelial cells, the authors show that testosterone induces an increase in glucose uptake. They find that testosterone induces differential gene expression with a focus on metabolic enzymes. Specifically, they identify increased expression of enzymes that regulate cholesterol and fatty acid synthesis, leading to increased production of 18:1 oleic acid.

      Strength:

      Oleic acid is secreted by seminal vesicle epithelial cells and taken up by sperm, inducing an increase in mitochondrial respiration. The difference in sperm motility and in vivo fertilization in the presence of 18:1 oleic acid and the absence of testosterone is small but significant, suggesting that the authors have identified one of the fertilization-supporting factors in seminal plasma.

      Weaknesses:

      Further studies are required to investigate the effect of other seminal vesicle components on sperm capacitation to support the author's conclusions. The author's experiments focused on potential testosterone-induced changes in the rate of seminal vesicle epithelial cell glycolysis and oxphos, however, provide conflicting results and a potential correlation with seminal vesicle epithelial cell proliferation should be confirmed by additional experiments.

    1. Reviewer #3 (Public Review):

      This paper considers a challenging motor control task - the critical stability task (CST) - that can be performed equally well by humans and macaque monkeys. This task is of considerable interest since it is rich enough to potentially yield important novel insights into the neural basis of behavior in more complex tasks that point-to-point reaching. Yet it is also simple enough to allow parallel investigation in humans and monkeys, and is also easily amenable to computational modeling. The paper makes a compelling argument for the importance of this type of parallel investigation and the suitability of the CST for doing so.

      Behavior in monkeys and in human subjects suggests that behavior seems to include two qualitatively different kinds of behavior - in some cases, the cursor oscillates about the center of the screen, and in other cases, it drifts more slowly in one direction. The authors argue that these two behavioral regimes can be reliably induced by instructing human participants to either maintain the cursor in the center of the screen (position control objective), or keep the cursor still anywhere in the screen (velocity control objective) - as opposed to the usual 'instruction' to just not let the cursor leave the screen. A computational model based on optimal feedback control can reproduce the different behaviors under these two instructions.

      Overall, this is a creative study that leverages experiments in humans and computational modeling to gain insight into the nature of individual differences in behavior across monkeys (and people). The authors convincingly demonstrate that they can infer the control objectives from participants who were instructed how to perform the task to emphasize either position or velocity control, based on the RMS cursor position and RMS cursor velocity. The authors show that, while other behavioral metrics do contain similar information about the control objective, RMS position and velocity are sufficient, and their approach classifies control objectives for simulated data with high accuracy (~95%).

      The authors also convincingly show that the range of behaviors observed in the CST task cannot be explained as emerging from variations in effort cost, motor execution noise, or sensorimotor delays.

      One significant issue, however relates to framing the range of possible control objectives as a simple dichotomy between 'position' and 'velocity' objectives. The authors do clearly state that this is a deliberate choice made in order to simplify their first attempts at solving this challenging problem. However, I do think that the paper at times gives a false impression that this dichotomous view of the control objectives was something that emerged from the data, rather than resulting from a choice to simplify the modeling/inference problem. For instance, line 115: "An optimal control model was used to simulate different control objectives, through which we identified two different control objectives in the experimental data of humans and monkeys."

      In the no-instruction condition - which is the starting point and which the ultimate goal of the paper is to understand - there is a lot of variability in behavior across trials (even within an individual) and generally no clear correspondence to either the position or velocity objective. This variability is largely interpreted as the monkeys (and people) switching between control objectives on a trial-to-trial basis. If the behavior were truly a bimodal mixture of these two different behaviors, this might be a convincing interpretation. However, there are a lot of trials that fall in-between the patterns of behavior expected under the position and velocity control objectives. The authors do mention this issue in the discussion. However, it's not clearly examined whether these are simply fringe trials that are ambiguous (like some trials generated by the model are), or whether they reflect a substantial proportion of trials that require some other explanation (whether that is blended position/velocity control, or something else). The existence of these 'in-between' trials (which possibly amount to more than a third of all trials) makes the switching hypothesis a lot less plausible.

      Overall, while I think the paper introduces a promising approach and overall helps to improve our understanding of the behavior in this task, I'm not fully convinced that the core issue of explaining the variability in behavior in the no-instruction condition (in monkeys especially) has been resolved. The main explanation put forward is that the monkeys are switching between control objectives on a trial-by-trial basis, but there is no real evidence in the data for this, and I don't think there is yet a good explanation of what is occurring in the 'in-between' trials that aren't explained well by velocity or position objectives.

    1. Reviewer #3 (Public Review):

      This study presents a valuable exploration of CD4+ T cell response in a fixed TCRβ chain FoxP3-GFP mouse model across stimuli and tissues through the analysis of their TCRα repertoires. This is an insightful paper for the community as it suggests several future directions of exploration.

      The authors compare Treg and conventional CD4+ repertoires by looking at diversity measures and the relative overlap of shared clonotypes to characterize similarity across different tissues and antigen challenges. They find distinct yet convergent responses with occasional plasticity across subsets for some stimuli. The observed lack of a general behavior highlights the need for careful comparison of immune repertoires across cell subsets and tissues. Such comparisons are crucial in order to better understand the heterogeneity of the adaptive immune response. This mouse model demonstrates its utility for this task due to the reduced diversity of the TCRα repertoire and the ability to track a single chain.

      The revised manuscript has significantly improved in terms of clarity of explanations and presentations of the results.

    1. Reviewer #2 (Public Review):

      This manuscript explores the mechanism underlying the accumulation of phytosphingosine (PHS) and its role in initiating vacuole fission. The study posits the involvement of membrane contact sites (MCSs) in two key stages of this process. Firstly, MCSs tethered by tricalbin between the endoplasmic reticulum (ER) and the plasma membrane (PM) or Golgi regulate the intracellular levels of PHS. Secondly, the amassed PHS triggers vacuole fission, most likely through the nuclear-vacuolar junction (NVJ). The authors propose that MCSs play a regulatory role in vacuole morphology via sphingolipid metabolism.

      While some results in the manuscript are intriguing, certain broad conclusions occasionally surpass the available data. Despite the authors' efforts to enhance the manuscript, certain aspects remain unclear. It is still uncertain whether subtle changes in PHS levels could induce such effects on vacuolar fission. Additionally, it is regrettable that the lipid measurements are not comparable with previous studies by the authors. Future advancements in methods for determining intracellular lipid transport and levels are anticipated to shed light on the remaining uncertainties in this study.

    1. Reviewer #2 (Public Review):

      Summary:

      The goal of this study was to examine the role of FNDC5 in the response of the murine skeleton to either lactation or a calcium-deficient diet. The authors find that female FNDC5 KO mice are somewhat protected from the bone loss and osteocyte lacunar enlargement caused by either lactation or a calcium-deficient diet. In contrast, male FNDC5 KO mice lose more bone and have a greater enlargement of osteocyte lacunae than their wild type controls. Based on these results, the authors conclude that in males irisin protects bone from calcium deficiency but that in females it promotes calcium removal from bone for lactation.

      While some of the conclusions of this study are supported by the results, it is not clear that the modest effects of FNDC5 deletion have an impact on calcium homeostasis or milk production.

      Specific comments.

      (1) The authors sometimes refer to FNDC5 and other times to irisin when describing causes for a particular outcome. Because irisin was not measured in any of the experiments, the authors should not conclude that lack of irisin is responsible. Along these lines, is there any evidence that either lactation or a calcium-deficient diet increases production of irisin in mice?

      (2) The results of the irisin-rescue experiment shown in figure 2G cannot be appropriately interpreted without normal diet controls. In addition, some evidence that the AAV8-irisin virus actually increased irisin levels in the mice would strengthen the conclusion.

      (3) There is insufficient evidence to support the idea that the effect of FNDC5 on bone resorption and osteocytic osteolysis is important for the transfer of calcium from bone to milk. Previous studies by others have shown that bone resorption is not required to maintain milk or serum calcium when dietary calcium is sufficient but is critical if dietary calcium is low (Endo. 156:2762-73, 2015). To support the conclusions of the current study, it would be necessary to determine whether FNDC5 is required to maintain calcium levels when lactating mice lack sufficient dietary calcium.

      (4) The amount of cortical bone loss due to lactation is very similar in both WT and FNDC5 KO mice. The results of the statistical analysis of the data presented in figure 1B are surprising given the very similar effect size of lactation. The key result from the 2-way ANOVA is whether there is an effect of genotype on the effect size of lactation (genotype-lactation interaction). The interaction terms were not provided. Similar concerns are noted for the results shown in figure 1G and H.

      (5) It is not clear what justifies the term 'primed' or 'activated' for resorption. Is there evidence that a certain level of TRAP expression lowers the threshold for osteocytic osteolysis in response to a stimulus?

    1. Reviewer #2 (Public Review):

      In this manuscript, the authors propose a computational method based on deep convolutional neural networks (CNNs) to automatically detect cell divisions in two-dimensional fluorescence microscopy timelapse images. Three deep learning models are proposed to detect the timing of division, predict the division axis, and enhance cell boundary images to segment cells before and after division. Using this computational pipeline, the authors analyze the dynamics of cell divisions in the epithelium of the Drosophila pupal wing and find that a wound first induces a reduction in the frequency of division followed by a synchronised burst of cell divisions about 100 minutes after its induction.

      Comments on revised version:

      Regarding the Reviewer's 1 comment on the architecture details, I have now understood that the precise architecture (number/type of layers, activation functions, pooling operations, skip connections, upsampling choice...) might have remained relatively hidden to the authors themselves, as the U-net is built automatically by the fast.ai library from a given classical choice of encoder architecture (ResNet34 and ResNet101 here) to generate the decoder part and skip connections.

      Regarding the Major point 1, I raised the question of the generalisation potential of the method. I do not think, for instance, that the optimal number of frames to use, nor the optimal choice of their time-shift with respect to the division time (t-n, t+m) (not systematically studied here) may be generic hyperparameters that can be directly transferred to another setting. This implies that the method proposed will necessarily require re-labeling, re-training and re-optimizing the hyperparameters which directly influence the network architecture for each new dataset imaged differently. This limits the generalisation of the method to other datasets, and this may be seen as in contrast to other tools developed in the field for other tasks such as cellpose for segmentation, which has proven a true potential for generalisation on various data modalities. I was hoping that the authors would try themselves testing the robustness of their method by re-imaging the same tissue with slightly different acquisition rate for instance, to give more weight to their work.

      In this regard, and because the authors claimed to provide clear instructions on how to reuse their method or adapt it to a different context, I delved deeper into the code and, to my surprise, felt that we are far from the coding practice of what a well-documented and accessible tool should be.

      To start with, one has to be relatively accustomed with Napari to understand how the plugin must be installed, as the only thing given is a pip install command (that could be typed in any terminal without installing the plugin for Napari, but has to be typed inside the Napari terminal, which is mentioned nowhere). Surprisingly, the plugin was not uploaded on Napari hub, nor on PyPI by the authors, so it is not searchable/findable directly, one has to go to the Github repository and install it manually. In that regard, no description was provided in the copy-pasted templated files associated to the napari hub, so exporting it to the hub would actually leave it undocumented.

      Regarding now the python notebooks, one can fairly say that the "clear instructions" that were supposed to enlighten the code are really minimal. Only one notebook "trainingUNetCellDivision10.ipynb" has actually some comments, the other have (almost) none nor title to help the unskilled programmer delving into the script to guess what it should do. I doubt that a biologist who does not have a strong computational background will manage adapting the method to its own dataset (which seems to me unavoidable for the reasons mentioned above).

      Finally regarding the data, none is shared publicly along with this manuscript/code, such that if one doesn't have a similar type of dataset - that must be first annotated in a similar manner - one cannot even test the networks/plugin for its own information. A common and necessary practice in the field - and possibly a longer lasting contribution of this work - could have been to provide the complete and annotated dataset that was used to train and test the artificial neural network. The basic reason is that a more performant, or more generalisable deep-learning model may be developed very soon after this one and for its performance to be fairly compared, it requires to be compared on the same dataset. Benchmarking and comparison of methods performance is at the core of computer vision and deep-learning.