Enhanced Preprints

3D Reconstruction of Neuronal Allometry and Neuromuscular Projections in Asexual Planarians Using Expansion Tiling Light Sheet Microscopy

  1. Jing Lu
  2. Hao Xu
  3. Dongyue Wang
  4. Yanlu Chen
  5. Takeshi Inuoe
  6. Liang Gao author has email address
  7. Kai Lei author has email address
  1. College of Life Sciences, Zhejiang University, Hangzhou, Zhejiang, China
  2. Key Laboratory of Structural Biology of Zhejiang Province, School of Life Sciences, Westlake University, Hangzhou, Zhejiang, China
  3. Westlake Laboratory of Life Sciences and Biomedicine, Hangzhou, Zhejiang, China
  4. Key Laboratory of Growth Regulation and Translational Research of Zhejiang Province, School of Life Sciences, Westlake University, Hangzhou, Zhejiang, China
  5. Institute of Biology, Westlake Institute for Advanced Study, Hangzhou, Zhejiang, China
  6. Division of Adaptation Physiology, Faculty of Medicine, Tottori University, Yonago, Japan

Peer review process

Not revised: This Reviewed Preprint includes the authors’ original preprint (without revision), an eLife assessment, public reviews, and a provisional response from the authors.

Read more about eLife’s peer review process.

Editors

  • Reviewing Editor
    Frank Chan
    University of Groningen, Groningen, Netherlands
  • Senior Editor
    Christopher Huang
    University of Cambridge, Cambridge, United Kingdom

Reviewer #1 (Public review):

Summary:

The planarian flatworm Schmidtea mediterranea is widely used as a model system for regeneration because of its remarkable ability to regenerate its entire body plan from very small fragments of tissue, including the complete and rapid regeneration of the CNS. Prior to this study, analysis of CNS regeneration in planaria has mostly been performed on a gross anatomical level. Despite its simplicity compared to vertebrates, the CNS of many invertebrates, including planaria, is nonetheless complex, intricate, and densely packed. Some invertebrate models allow the visualization of individual cellular components of the CNS using transgenic techniques. Until transgenesis becomes commonplace in planaria, the visualization and analysis of detailed CNS anatomy must rely on alternate approaches in order to capitalize on the immense promise of this system as a model for CNS regeneration. Another challenge for the study of the CNS more broadly is how to perform imaging of a complete CNS on a reasonable timescale such that multiple individuals per experimental condition can be imaged.

Strengths:

In this report, Lu et al. describe a careful and detailed analysis of the planarian neuroanatomy and musculature in both the homeostatic and regenerating contexts. To improve the effective resolution of their imaging, the authors optimized a tissue expansion protocol for planaria. Imaging was performed by light sheet microscopy, and the resulting optical sections were tiled to reconstruct whole worms. Labelled tissues and cells were then segmented to allow quantification of neurons and muscle fibers, as well as all cells in individual worms using a DNA dye. The resulting workflow can produce highly detailed and quantifiable 3D reconstructions at a rate that is fast enough to allow the analysis of large numbers of animals.

Weaknesses:

Lu et al. use their workflow to visualize RNA expression of five enzymes that are each involved in the biosynthetic pathway of different neurotransmitters/modulators, namely chat (cholinergeric), gad (GABAergic), tbh (octopaminergic), th (dopaminergic), and tph (serotonergic). In this way, they generate an anatomical atlas of neurons that produce these molecules. Collectively these markers are referred to as the "neuronpool." They overstate when they write, "The combination of these five types of neurons constitutes a neuron pool that enables the labeling of all neurons throughout the entire body." This statement does not accurately represent the state of our knowledge about the diversity of neurons in S. mediterranea. There are several lines of evidence that support the presence of glutamatergic and glycinergic neurons, including the following. The glutamate receptor agonists NMDA and AMPA both produce seizure-like behaviors in S. mediterranea that are blocked by the application of glutamate receptor antagonists MK-801 and DNQX (which antagonize NMDA and AMPA glutamate receptors, respectively; Rawls et al., 2009). scRNA-Seq data indicates that neurons in S. mediterranea express a vesicular glutamate transporter, a kainite-type glutamate receptor, a glycine receptor, and a glycine transporter (Brunet Avalos and Sprecher, 2021; Wyss et al., 2022). Two AMPA glutamate receptors, GluR1 and GluR2, are known to be expressed in the CNS of another planarian species, D. japonica (Cebria et al., 2002). Likewise, there is abundant evidence for the presence of peptidergic neurons in S. mediterranea (Collins et al., 2010; Fraguas et al., 2012; Ong et al., 2016; Wyss et al., 2022; among others) and in D. japonica (Shimoyama et al., 2016). For these reasons, the authors should not assume that all neurons can be assayed using the five markers that they selected. The situation is made more complex by the fact that many neurons in S. mediterranea appear to produce more than one neurotransmitter/modulator/peptide (Brunet Avalos and Sprecher, 2021; Wyss et al., 2022), which is common among animals (Vaaga et al., 2014; Brunet Avalos and Sprecher, 2021). However the published literature indicates that there are substantial populations of glutamatergic, glycinergic, and peptidergic neurons in S. mediterranea that do not produce other classes of neurotransmission molecule (Brunet Avalos and Sprecher, 2021; Wyss et al., 2022). Thus it seems likely that the neuronpool will miss many neurons that only produce glutamate, glycine or a neuropeptide.

The authors use their technique to image the neural network of the CNS using antibodies raised vs. Arrestin, Synaptotagmin, and phospho-Ser/Thr. They document examples of both contralateral and ipsilateral projections from the eyes to the brain in the optic chiasma (Figure 1C-F). These data all seem to be drawn from a single animal in which there appears to be a greater than normal number of nerve fiber defasciculatations. It isn't clear how well their technique works for fibers that remain within a nerve tract or the brain. The markers used to image neural networks are broadly expressed, and it's possible that most nerve fibers are too densely packed (even after expansion) to allow for image segmentation. The authors also show a close association between estrella-positive glial cells and nerve fibers in the optic chiasma.

The authors count all cell types, neuron pool neurons, and neurons of each class assayed. They find that the cell number to body volume ratio remains stable during homeostasis (Figure S3C), and that the brain volume steadily increases with increasing body volume (Figure S3E). They also observe that the proportion of neurons to total body cells is higher in worms 2-6 mm in length than in worms 7-9 mm in length (Figure 2D, S3F). They find that the rate at which four classes of neurons (GABAergic, octopaminergic, dopaminergic, serotonergic) increase relative to the total body cell number is constant (Figure S3G-J). They write: "Since the pattern of cholinergic neurons is the major cell population in the brain, these results suggest that the above observation of the non-linear dynamics between neurons and cell numbers is likely from the cholinergic neurons." This conclusion should not be reached without first directly counting the number of cholinergic neurons and total body cells. Given that glutamatergic, glycinergic, and peptidergic neurons were not counted, it also remains possible that the non-linear dynamics are due (in part or in whole) to one or more of these populations.

The authors next assayed the production of different classes of neurons in regenerating post-pharyngeal tail fragments. At 14 dpa, they find significantly reduced proportions of octopaminergic, GABAergic, and dopaminergic neurons in these regenerated animals (Figure 3K). Given that these three neuron classes are primarily found in the brain region (Figure S2A), this suggests that the brains of these animals may not have finished regenerating by 14 dpa.

The authors next applied their imaging and segmentation technique to the musculature using the 6G10 antibody. They find that the body wall muscle fibers from the dorsal and ventral body walls integrate differently at the anterior end (to form a cobweb-like arrangement) compared to the posterior end (Figure 4I). They knock down β-catenin in regenerating head anterior fragments and find that the resulting double-headed worms produce a cobweb-like arrangement at both ends (Figure 4J).

RNAi knockdown of inr-1 is known to produce mobility defects and have elongated bodies relative to control animals (Lei et al., 2016; Figure S6A). To understand the nature of these defects, the authors image the muscle of inr-1 RNAi animals and find increased circular body wall muscle fibers on both dorsal and ventral sides, while β-catenin RNAi animals have increased longitudinal muscle fibers on the dorsal side (Figure 6C). The inr-1 RNAi animals also have reduced cholinergic neurons (Figure S6B), and ectopic expression of the GABAergic marker gad in the periphery (Figure S6B). Lastly the authors simultaneously image muscle and estrella-positive glia and find that these glia lack their typically elaborate stellate morphology in inr-1 RNAi animals (Figure 6E, S6E-K). The combination of this muscle, neuronal, and glial defects may account for the mobility defects observed in inr-1 RNAi worms.

Reviewer #2 (Public review):

Summary:

This manuscript builds on the authors' 2020 study by combining tissue expansion with light sheet microscopy to quantify the organism-wide spatial distribution of various cell types in the planarian.

Strengths:

(1) The quantification of cell types as a function of animal size and regeneration stages could be a useful resource for the planarian research community.

(2) The high-quality images can help clarify some anatomical structures within the planarian tissues.

Weaknesses:

(1) The proprietary nature of the microscope, protected by a patent, limits the technical details provided, making the method hard to reproduce in other labs.

(2) The resolution of the analyses is mostly limited to the cellular level, which does not fully leverage the advantages of expansion microscopy. Previous applications of expansion microscopy have revealed finer nanostructures in the planarian nervous system (see Fan et al. Methods in Cell Biology 2021; Wang et al. eLife 2021). It is unclear whether the current protocol can achieve a comparable resolution.

(3) The data largely corroborate past observations, while the novel claims are insufficiently substantiated.

A few major issues with the claims:

(4) Line 303-304: While 6G10 is a widely used antibody to label muscle fibers in the planarian, it doesn't uniformly mark all muscle types (Scimone at al. Nature 2017). For a more complete view of muscle fibers, it is important to use a combination of antibodies targeting different fiber types or a generic marker such as phalloidin. This raises fundamental concerns about all the conclusions drawn from Figures 4 and 6 about differences between various muscle types. Additionally, the authors should cite the original paper that developed the 6G10 antibody (Ross et al. BMC Developmental Biology 2015).

(5) Lines 371-379: The claim that DV muscles regenerate into longitudinal fibers lacks evidence. Furthermore, previous studies have shown that TFs specifying different muscle types (DV, circular, longitudinal, and intestinal) both during regeneration and homeostasis are completely different (Scimone et al., Nature 2017 and Scimone et al., Current Biology 2018). Single-cell RNAseq data further establishes the existence of divergent muscle progenitors giving rise to different muscle fibers. These observations directly contradict the authors' claim, which is only based on images of fixed samples at a coarse time resolution.

(6) Line 423: The manuscript lacks evidence to claim glia guide muscle fiber branching.

(7) Lines 432/478: The conclusion about neuronal and muscle guidance on glial projections is similarly speculative, lacking functional evidence. It is possible that the morphological defects of estrella+ cells after bcat1 RNAi are caused by Wnt signaling directly acting on estrella+ cells independent of muscles or neurons.

(8) Finally, several technical issues make the results difficult to interpret. For example, in line 125, cell boundaries appear to be determined using nucleus images; in line 136, the current resolution seems insufficient to reliably trace neural connections, at least based on the images presented.

Reviewer #3 (Public review):

Summary:

In this manuscript, the authors apply tissue expansion and tiling light sheet microscopy to study allometric growth and regeneration in planaria. They developed image analysis pipelines to help them quantify different neuronal subtypes and muscles in planaria of different sizes and during regeneration. Among the strengths of this work, the authors provide beautiful images that show the potential of the approaches they are taking and their ability to quantify specific cell types in relatively large numbers of whole animal samples. Many of their findings confirm previous results in the literature, which helps validate the techniques and pipelines they have applied here. Among their new observations, they find that the body wall muscles at the anterior and posterior poles of the worm are organized differently and show that the muscle pattern in the posterior head of beta-catenin RNAi worms resembles the anterior muscle pattern. They also show that glial cell processes appear to be altered in beta-catenin or insulin receptor-1 RNAi worms. Weaknesses include some over-interpretation of the data and lack of consideration or citation of relevant previous literature, as discussed below.

Strengths:

This method of tissue expansion will be useful for researchers interested in studying this experimental animal. The authors provide high-quality images that show the utility of this technique. Their analysis pipeline permits them to quantify cell types in relatively large numbers of whole animal samples.

The authors provide convincing data on changes in total neurons and neuronal sub-types in different-sized planaria. They report differences in body wall muscle pattern between the anterior and posterior poles of the planaria, and that these differences are lost when a posterior head forms in beta-catenin RNAi planaria. They also find that glial cell projections are reduced in insulin receptor-1 RNAi planaria.

Weaknesses:

The work would have been strengthened by a more careful consideration of previous literature. Many papers directly relevant to this work were not cited. Such omissions do the authors a disservice because in some cases, they fail to consider relevant information that impacts the choice of reagents they have used or the conclusions they are drawing.

For example, when describing the antibody they use to label muscles (monoclonal 6G10), they do not cite the paper that generated this reagent (Ross et al PMCID: PMC4307677), and instead, one of the papers they do cite (Cebria 2016) that does not mention this antibody. Ross et al reported that 6G10 does not label all body wall muscles equivalently, but rather "predominantly labels circular and diagonal fibers" (which is apparent in Figure S5A-D of the manuscript being reviewed here). For this reason, the authors of the paper showing different body wall muscle populations play different roles in body patterning (Scimone et al 2017, PMCID: PMC6263039, also not cited in this paper) used this monoclonal in combination with a polyclonal antibody to label all body wall muscle types. Because their "pan-muscle" reagent does not label all muscle types equivalently, it calls into question their quantification of the different body wall muscle populations throughout the manuscript. It does not help matters that their initial description of the body wall muscle types fails to mention the layer of thin (inner) longitudinal muscles between the circular and diagonal muscles (Cebria 2016 and citations therein).

Ipsilateral and contralateral projections of the visual axons were beautifully shown by dye-tracing experiments (Okamoto et al 2005, PMID: 15930826). This paper should be cited when the authors report that they are corroborating the existence of ipsilateral and contralateral projections.

The proportional decrease of neurons with growth in S. mediterranea was shown by counting different cell types in macerated planarians (Baguna and Romero, 1981; https://link.springer.com/article/10.1007/BF00026179) and earlier histological observations cited there. These results have also been validated by single-cell sequencing (Emili et al, bioRxiv 2023, https://www.biorxiv.org/content/10.1101/2023.11.01.565140v). Allometric growth of the planaria tail (the tail is proportionately longer in large vs small planaria) can explain this decrease in animal size. The authors never really discuss allometric growth in a way that would help readers unfamiliar with the system understand this.

In some cases, the authors draw stronger conclusions than their results warrant. The authors claim that they are showing glial-muscle interactions, however, they do not provide any images of triple-stained samples labeling muscle, neurons, and glia, so it is impossible for the reader to judge whether the glial cells are interacting directly with body wall muscles or instead with the well-described submuscular nerve plexus. Their conclusion that neurons are unaffected by beta-cat or inr-1 RNAi based on anti-phospho-Ser/Thr staining (Fig. 6E) is unconvincing. They claim that during regeneration "DV muscles initially regenerate into longitudinal fibers at the anterior tip" (line 373). They provide no evidence for such switching of muscle cell types, so it is unclear why they say this.

The authors show how their automated workflow compares to manual counts using PI-stained specimens (Figure S1T). I may have missed it, but I do not recall seeing a similar ground truth comparison for their muscle fiber counting workflow. I mention this because the segmented image of the posterior muscles in Figure 4I seems to be missing the vast majority of circular fibers visible to the naked eye in the original image.

It is unclear why the abstract says, "We found the rate of neuron cell proliferation tends to lag..." (line 25). The authors did not measure proliferation in this work and neurons do not proliferate in planaria.

It is unclear what readers are to make of the measurements of brain lobe angles. Why is this a useful measurement and what does it tell us?

The authors repeatedly say that this work lets them investigate planarians at the single-cell level, but they don't really make the case that they are seeing things that haven't already been described at the single-cell level using standard confocal microscopy.

Author response:

Reviewer #1 (Public review):

Lu et al. use their workflow to visualize RNA expression of five enzymes that are each involved in the biosynthetic pathway of different neurotransmitters/modulators, namely chat (cholinergeric), gad (GABAergic), tbh (octopaminergic), th (dopaminergic), and tph (serotonergic). In this way, they generate an anatomical atlas of neurons that produce these molecules. Collectively these markers are referred to as the "neuronpool." They overstate when they write, "The combination of these five types of neurons constitutes a neuron pool that enables the labeling of all neurons throughout the entire body." This statement does not accurately represent the state of our knowledge about the diversity of neurons in S. mediterranea. There are several lines of evidence that support the presence of glutamatergic and glycinergic neurons, including the following. The glutamate receptor agonists NMDA and AMPA both produce seizure-like behaviors in S. mediterranea that are blocked by the application of glutamate receptor antagonists MK-801 and DNQX (which antagonize NMDA and AMPA glutamate receptors, respectively; Rawls et al., 2009). scRNA-Seq data indicates that neurons in S. mediterranea express a vesicular glutamate transporter, a kainite-type glutamate receptor, a glycine receptor, and a glycine transporter (Brunet Avalos and Sprecher, 2021; Wyss et al., 2022). Two AMPA glutamate receptors, GluR1 and GluR2, are known to be expressed in the CNS of another planarian species, D. japonica (Cebria et al., 2002). Likewise, there is abundant evidence for the presence of peptidergic neurons in S. mediterranea (Collins et al., 2010; Fraguas et al., 2012; Ong et al., 2016; Wyss et al., 2022; among others) and in D. japonica (Shimoyama et al., 2016). For these reasons, the authors should not assume that all neurons can be assayed using the five markers that they selected. The situation is made more complex by the fact that many neurons in S. mediterranea appear to produce more than one neurotransmitter/modulator/peptide (Brunet Avalos and Sprecher, 2021; Wyss et al., 2022), which is common among animals (Vaaga et al., 2014; Brunet Avalos and Sprecher, 2021). However the published literature indicates that there are substantial populations of glutamatergic, glycinergic, and peptidergic neurons in S. mediterranea that do not produce other classes of neurotransmission molecule (Brunet Avalos and Sprecher, 2021; Wyss et al., 2022). Thus it seems likely that the neuronpool will miss many neurons that only produce glutamate, glycine or a neuropeptide.

In response to your comments, we agree that our initial statement regarding the "neuron pool" overstated the extent of neuronal coverage provided by the five selected markers. We have revised the sentence as “The combination of these five types of neurons constitutes a neuron pool that enables the labeling of most of the neurons throughout the entire body, including the eyes, brain, and pharynx”.

Furthermore, we chose the five neurotransmitter systems (cholinergic, GABAergic, octopaminergic, dopaminergic, and serotonergic) based on their well-characterized roles in planarian neurobiology and the availability of reliable markers. However, we acknowledge the limitations of this approach and recognize that it does not encompass all neuron types, particularly those involved in glutamatergic, glycinergic, and peptidergic signaling, which have been documented in S. mediterranea. We will also add the content about other neuron types in our revised manuscript “Additionally, there is considerable diversity among glutamatergic, glycinergic, and peptidergic neurons in planarians. Many neurons in S. mediterranea express more than one neurotransmitter or neuropeptide, which adds further complexity to the system.”

The authors use their technique to image the neural network of the CNS using antibodies raised vs. Arrestin, Synaptotagmin, and phospho-Ser/Thr. They document examples of both contralateral and ipsilateral projections from the eyes to the brain in the optic chiasma (Figure 1C-F). These data all seem to be drawn from a single animal in which there appears to be a greater than normal number of nerve fiber defasciculatations. It isn't clear how well their technique works for fibers that remain within a nerve tract or the brain. The markers used to image neural networks are broadly expressed, and it's possible that most nerve fibers are too densely packed (even after expansion) to allow for image segmentation. The authors also show a close association between estrella-positive glial cells and nerve fibers in the optic chiasma.

Thank you for your detailed feedback. While we did not perform segmentation of all neuron fibers, we were able to segment more isolated fibers that were not densely packed within the neural tracts. We use 120 nm resolution to segment neurons along the three axes. Our data show the presence of both contralateral and ipsilateral projections of visual neurons. Although Figure 1C-F shows data from one planarian, we imaged three independent specimens to confirm the consistency of these observations. In the revised manuscript, we will include a discussion on the limitations of TLSM in reconstructing neural networks, particularly when it comes to resolving fibers within densely packed regions of the nerve tracts.

The authors count all cell types, neuron pool neurons, and neurons of each class assayed. They find that the cell number to body volume ratio remains stable during homeostasis (Figure S3C), and that the brain volume steadily increases with increasing body volume (Figure S3E). They also observe that the proportion of neurons to total body cells is higher in worms 2-6 mm in length than in worms 7-9 mm in length (Figure 2D, S3F). They find that the rate at which four classes of neurons (GABAergic, octopaminergic, dopaminergic, serotonergic) increase relative to the total body cell number is constant (Figure S3G-J). They write: "Since the pattern of cholinergic neurons is the major cell population in the brain, these results suggest that the above observation of the non-linear dynamics between neurons and cell numbers is likely from the cholinergic neurons." This conclusion should not be reached without first directly counting the number of cholinergic neurons and total body cells. Given that glutamatergic, glycinergic, and peptidergic neurons were not counted, it also remains possible that the non-linear dynamics are due (in part or in whole) to one or more of these populations.

We have removed the statement "Since the pattern of cholinergic neurons is the major cell population in the brain, these results suggest that the above observation of the non-linear dynamics between neurons and cell numbers is likely from the cholinergic neurons." We changed this statement into “These results suggest that the above observation of the non-linear dynamics between neurons and cell numbers is not likely from the octopaminergic, GABAergic, dopaminergic and serotonergic neurons. Since our neuron pool may not include glutamatergic, glycinergic, and peptidergic neurons, we would like to add the possibility that the non-linear dynamics may be from cholinergic neurons or other neurons not included in our staining.”

Reviewer #2 (Public review):

Weaknesses:

(1) The proprietary nature of the microscope, protected by a patent, limits the technical details provided, making the method hard to reproduce in other labs.

Thank you for your comment. We understand the importance of reproducibility and transparency in scientific research. We would like to point out that the detailed design and technical specifications of the TLSM are publicly available in our published work: Chen et al., Cell Reports, 2020. Additionally, the protocol for C-MAP, including the specific experimental steps, is comprehensively described in the methods section of this paper. We believe that these resources should provide sufficient information for other labs to replicate the method.

(2) The resolution of the analyses is mostly limited to the cellular level, which does not fully leverage the advantages of expansion microscopy. Previous applications of expansion microscopy have revealed finer nanostructures in the planarian nervous system (see Fan et al. Methods in Cell Biology 2021; Wang et al. eLife 2021). It is unclear whether the current protocol can achieve a comparable resolution.

Thank you for raising this important point. The strength of our C-MAP protocol lies in its fluorescence-protective nature and user convenience. Notably, the sample can be expanded up to 4.5-fold linearly without the need for heating or proteinase digestion, which helps preserve fluorescence signals. In addition, the entire expansion process can be completed within 48 hours. While our current analysis focused on cellular-level structures, our method can achieve comparable or better resolution and we will add this information in the revised manuscript.

(3) The data largely corroborate past observations, while the novel claims are insufficiently substantiated.

A few major issues with the claims:

(4) Line 303-304: While 6G10 is a widely used antibody to label muscle fibers in the planarian, it doesn't uniformly mark all muscle types (Scimone at al. Nature 2017). For a more complete view of muscle fibers, it is important to use a combination of antibodies targeting different fiber types or a generic marker such as phalloidin. This raises fundamental concerns about all the conclusions drawn from Figures 4 and 6 about differences between various muscle types. Additionally, the authors should cite the original paper that developed the 6G10 antibody (Ross et al. BMC Developmental Biology 2015).

We appreciate the reviewer’s insightful comments and acknowledge that 6G10 does not uniformly label all muscle fiber types. We agree that this limitation should be recognized in the interpretation of our results. we will revise the manuscript to explicitly state the limitations of using 6G10 alone for muscle fiber labeling and highlight the need for additional markers. We would also clarify that the primary objective of our study was not to distinguish all muscle fiber types but rather to demonstrate the application of our 3D tissue reconstruction method in addressing traditional research questions. Nonetheless, we agree that expanding the labeling strategy in future studies would allow for a more thorough investigation of muscle fiber diversity. We will ensure all citations are properly revised and updated in our next version.

(5) Lines 371-379: The claim that DV muscles regenerate into longitudinal fibers lacks evidence. Furthermore, previous studies have shown that TFs specifying different muscle types (DV, circular, longitudinal, and intestinal) both during regeneration and homeostasis are completely different (Scimone et al., Nature 2017 and Scimone et al., Current Biology 2018). Single-cell RNAseq data further establishes the existence of divergent muscle progenitors giving rise to different muscle fibers. These observations directly contradict the authors' claim, which is only based on images of fixed samples at a coarse time resolution.

Thank you for your valuable feedback. Our intent was not to suggest that DV muscles regenerate into longitudinal fibers. Our observations focused on the wound site, where DV muscle fibers appear to reconnect, and longitudinal fibers, along with other muscle types, gradually regenerate to restore the structure of the injured area. We will revise the relevant sections of the manuscript to clarify this dynamic process more accurately.

(6) Line 423: The manuscript lacks evidence to claim glia guide muscle fiber branching.

We will remove this statement from the revised version. Instead, we will focus on describing our observations of the connections between glial cells and muscle fibers.

(7) Lines 432/478: The conclusion about neuronal and muscle guidance on glial projections is similarly speculative, lacking functional evidence. It is possible that the morphological defects of estrella+ cells after bcat1 RNAi are caused by Wnt signaling directly acting on estrella+ cells independent of muscles or neurons.

We understand that this approach is insufficient and we will revise the manuscript to more clearly state the limitations of our data. We will describe our observations as preliminary and suggest that further experiments are required.

(8) Finally, several technical issues make the results difficult to interpret. For example, in line 125, cell boundaries appear to be determined using nucleus images; in line 136, the current resolution seems insufficient to reliably trace neural connections, at least based on the images presented.

We use two setups for imaging cells and neuron projections. For cellular resolution imaging, we utilized a 1× air objective with a numerical aperture (NA) of 0.25 and a working distance of 60 mm (OLYMPUS MV PLAPO). The voxel size used was 0.8×0.8×2.5 µm3. This configuration resulted in a resolution of 2×2×5 µm3 and a spatial resolution of 0.5×0.5×1.25 µm3 with 4× isotropic expansion. Alternatively, for sub-cellular imaging, we employed a 10×0.6 SV MP water immersion objective with 0.8 NA and a working distance of 8 mm (OLYMPUS). The voxel size used in this configuration was 0.26×0.26×0.8 µm3. As a result of this configuration, we achieved a resolution of 0.5×0.5×1.6 µm3 and a spatial resolution of 0.12×0.12×0.4 µm3 with a 4.5× isotropic expansion. The higher resolution achieved with sub-cellular imaging allows us to observe finer structures and trace neural connections.

Regarding your question about cell boundaries, we will revise the manuscript to specify that the boundaries we identified are those of each nucleus, rather than entire cells. This distinction will be made clear in the revised version.

Reviewer #3 (Public review):

Weaknesses:

(1) The work would have been strengthened by a more careful consideration of previous literature. Many papers directly relevant to this work were not cited. Such omissions do the authors a disservice because in some cases, they fail to consider relevant information that impacts the choice of reagents they have used or the conclusions they are drawing.

For example, when describing the antibody they use to label muscles (monoclonal 6G10), they do not cite the paper that generated this reagent (Ross et al PMCID: PMC4307677), and instead, one of the papers they do cite (Cebria 2016) that does not mention this antibody. Ross et al reported that 6G10 does not label all body wall muscles equivalently, but rather "predominantly labels circular and diagonal fibers" (which is apparent in Figure S5A-D of the manuscript being reviewed here). For this reason, the authors of the paper showing different body wall muscle populations play different roles in body patterning (Scimone et al 2017, PMCID: PMC6263039, also not cited in this paper) used this monoclonal in combination with a polyclonal antibody to label all body wall muscle types. Because their "pan-muscle" reagent does not label all muscle types equivalently, it calls into question their quantification of the different body wall muscle populations throughout the manuscript. It does not help matters that their initial description of the body wall muscle types fails to mention the layer of thin (inner) longitudinal muscles between the circular and diagonal muscles (Cebria 2016 and citations therein).

Ipsilateral and contralateral projections of the visual axons were beautifully shown by dye-tracing experiments (Okamoto et al 2005, PMID: 15930826). This paper should be cited when the authors report that they are corroborating the existence of ipsilateral and contralateral projections.

Thank you for your feedback. We will incorporate these citations and clarifications into the revised manuscript. We acknowledge the limitations of this approach and recognize that it does not encompass all neuron types, particularly those involved in glutamatergic, glycinergic, and peptidergic signaling. We will also add the content about other neuron types in our revised version.

(2) The proportional decrease of neurons with growth in S. mediterranea was shown by counting different cell types in macerated planarians (Baguna and Romero, 1981; https://link.springer.com/article/10.1007/BF00026179) and earlier histological observations cited there. These results have also been validated by single-cell sequencing (Emili et al, bioRxiv 2023, https://www.biorxiv.org/content/10.1101/2023.11.01.565140v). Allometric growth of the planaria tail (the tail is proportionately longer in large vs small planaria) can explain this decrease in animal size. The authors never really discuss allometric growth in a way that would help readers unfamiliar with the system understand this.

Thank you for your feedback. We will incorporate these citations and clarifications into the revised manuscript.

(3) In some cases, the authors draw stronger conclusions than their results warrant. The authors claim that they are showing glial-muscle interactions, however, they do not provide any images of triple-stained samples labeling muscle, neurons, and glia, so it is impossible for the reader to judge whether the glial cells are interacting directly with body wall muscles or instead with the well-described submuscular nerve plexus. Their conclusion that neurons are unaffected by beta-cat or inr-1 RNAi based on anti-phospho-Ser/Thr staining (Fig. 6E) is unconvincing. They claim that during regeneration "DV muscles initially regenerate into longitudinal fibers at the anterior tip" (line 373). They provide no evidence for such switching of muscle cell types, so it is unclear why they say this.

We acknowledge that some of our conclusions were overclaimed given the current data, and we appreciate the opportunity to clarify and refine these claims in the revised manuscript. Regarding the statement that "DV muscles initially regenerate into longitudinal fibers at the anterior tip" (line 373), as addressed in our previous response, this phrasing was unclear. Our intent was not to imply that DV muscles switch into longitudinal fibers. Instead, we observed that muscle fibers reconnect at the wound site, with longitudinal fibers and other muscle types gradually restoring the structure. We will revise this section to better describe the dynamic changes observed during regeneration.

(4) The authors show how their automated workflow compares to manual counts using PI-stained specimens (Figure S1T). I may have missed it, but I do not recall seeing a similar ground truth comparison for their muscle fiber counting workflow. I mention this because the segmented image of the posterior muscles in Figure 4I seems to be missing the vast majority of circular fibers visible to the naked eye in the original image.

Thank you for raising this important point. We will include a ground truth comparison of our automated muscle fiber counting with manual counts in the supplementary figures. Regarding the observation of missing circular fibers in Figure 4I, we agree that the segmentation appears to have missed a significant number of circular fibers in this particular image. This may have been due to limitations in the current parameters of the segmentation algorithm, especially in distinguishing fibers in regions of varying intensity or overlap. We are revisiting the segmentation parameters to improve the accuracy of detecting circular fibers, and we will provide an updated version of Figure 4I in the revised manuscript.

(5) It is unclear why the abstract says, "We found the rate of neuron cell proliferation tends to lag..." (line 25). The authors did not measure proliferation in this work and neurons do not proliferate in planaria.

Thank you for bringing this to our attention. What we intended to convey was the increase in neuron number during homeostasis. We will revise the abstract to avoid this mistake in this context and instead describe it as the increase in neuron numbers due to progenitor cell differentiation during homeostasis.

(6) It is unclear what readers are to make of the measurements of brain lobe angles. Why is this a useful measurement and what does it tell us?

The measurement of brain lobe angles is intended to provide a quantitative assessment of the growth and morphological changes of the planarian brain during regeneration. Additionally, the relevance of brain lobe angles has been explored in previous studies, such as Arnold et al., Nature, 2016, further supporting its use as a meaningful parameter.

(7) The authors repeatedly say that this work lets them investigate planarians at the single-cell level, but they don't really make the case that they are seeing things that haven't already been described at the single-cell level using standard confocal microscopy.

Thank you for your comment. We agree that single-cell level imaging has been previously achieved in planarians using conventional confocal microscopy. However, our goal was to extend the application of expansion microscopy by combining C-MAP with tiling light sheet microscopy (TLSM), which allows for faster and high-resolution 3D imaging of whole-mount planarians. This combination offers several key advantages over traditional confocal microscopy. For example, it enables high-throughput imaging across entire organisms with a level of detail and speed that is not easily achieved using confocal methods. This approach allows us to investigate the planarian nervous system at multiple developmental and regenerative stages in a more comprehensive manner, capturing large-scale structures while preserving fine cellular details. The ability to rapidly image whole planarians in 3D with this resolution provides a more efficient workflow for studying complex biological processes. We believe this distinction is significant and represents an advance over previous methods. We will clarify this point in the manuscript to better distinguish our approach from standard techniques.

  1. Howard Hughes Medical Institute
  2. Wellcome Trust
  3. Max-Planck-Gesellschaft
  4. Knut and Alice Wallenberg Foundation