Adrenergic activation modulates the signal from the Reissner fiber to cerebrospinal fluid-contacting neurons during development

  1. Yasmine Cantaut-Belarif
  2. Adeline Orts Del'Immagine
  3. Margot Penru
  4. Guillaume Pézeron
  5. Claire Wyart  Is a corresponding author
  6. Pierre-Luc Bardet  Is a corresponding author
  1. Paris Brain Institute, ICM, Inserm U 1127, CNRS UMR 7225, Sorbonne Université, France
  2. Molecular Physiology and Adaptation (PhyMA - UMR 7221), Muséum National d’Histoire Naturelle, CNRS, France

Peer review process

This article was accepted for publication as part of eLife's original publishing model.

History

  1. Version of Record updated
  2. Version of Record published
  3. Accepted Manuscript published
  4. Accepted
  5. Received

Decision letter

  1. Michel Bagnat
    Reviewing Editor; Duke University, United States
  2. Didier YR Stainier
    Senior Editor; Max Planck Institute for Heart and Lung Research, Germany

In the interests of transparency, eLife publishes the most substantive revision requests and the accompanying author responses.

Acceptance summary:

In the manuscript by Cantaut-Belarif et al. the authors investigate how the Reissner fiber (RF) signals to the CSF neurons (CSFcNs). Using transcriptomics, state-of-the-art live imaging and in vivo electrophysiological analyses, they show that the RF elicits calcium signaling and controls the expression of urp2 via local adrenergic signaling. They also show that local adrenergic signaling can rescue RF defects. Thus, the authors show that monoamines are mediators of the RF- CSF pathway that controls axis wide patterning of the embryo.

This is an interesting, well developed and clearly written manuscript that presents research conducted in parallel and independently from another report recently published by Lu et al. (Lu et al., 2020). While both manuscripts report similar developmental phenotypes, Cantaut-Belarif et al. present an in-depth analysis of monoamine signaling and its effects in CSFcNs that provides new mechanistic insights into the RF- CSF pathway.

Decision letter after peer review:

Thank you for submitting your article "Adrenergic activation modulates the Reissner fiber signal to cerebrospinal fluid-contacting neurons during development" for consideration by eLife. Your article has been reviewed by two peer reviewers, and the evaluation has been overseen by a Reviewing Editor and Didier Stainier as the Senior Editor. The reviewers have opted to remain anonymous.

The reviewers have discussed the reviews with one another and the Reviewing Editor has drafted this decision to help you prepare a revised submission.

As the editors have judged that your manuscript is of interest, but as described below that additional experiments are required before it is published, we would like to draw your attention to changes in our revision policy that we have made in response to COVID-19 (https://elifesciences.org/articles/57162). First, because many researchers have temporarily lost access to the labs, we will give authors as much time as they need to submit revised manuscripts. We are also offering, if you choose, to post the manuscript to bioRxiv (if it is not already there) along with this decision letter and a formal designation that the manuscript is "in revision at eLife". Please let us know if you would like to pursue this option. (If your work is more suitable for medRxiv, you will need to post the preprint yourself, as the mechanisms for us to do so are still in development.)

This is an interesting and well written manuscript that investigates how the Reissner fiber (RF) signals to the CSF neurons (CSFcNs). The authors show that the RF elicits calcium signaling and controls the expression of urp2 likely via adrenergic signaling, which can rescue RF defects. Importantly, the authors show that monoamines are mediators of the RF-CSF pathway that controls axis wide patterning of the embryo. There are however several points that need to be addressed experimentally before the manuscript is ready for publication.

Essential revisions:

1) Hindbrain injection of monoamines. It is unclear what concentrations were used, how long the monoamines were thought to be bioactive and how this was assessed, and to what extent they diffused. The authors should provide controls and validate they assay. Clear and detailed protocols are needed as well.

2) Double immunostaining with anti-GFP and anti-norepinephrine, and anti-Adrb2 in pkd2l1:GCAMP fish.

3) Justify the use of relatively late stage embryos (i.e. 30 hpf vs. 24 hpf). Provide images of scospondin mutants at the 20-26 hpf window.

4) Detailed protocols are needed.

5) Editorial revision should include comments on similarities and differences with Lu et al.

https://doi.org/10.7554/eLife.59469.sa1

Author response

Essential revisions:

1) Hindbrain injection of monoamines. It is unclear what concentrations were used, how long the monoamines were thought to be bioactive and how this was assessed, and to what extent they diffused. The authors should provide controls and validate they assay. Clear and detailed protocols are needed as well.

We agree with the reviewers that this is a critical point for the validation of the calcium imaging assay after monoamine hindbrain ventricle (HBV) injection in 30 hpf embryos.

First, concentrations of epinephrine and norepinephrine were already described in the Materials and methods section (epinephrine and norepinephrine were diluted to 3 mM in aCSF before hindbrain ventricle injections, see subsection “In vivo calcium imaging”). The time post-injection at which embryos were imaged was not mentioned and is now described in the revised version of the manuscript (embryos were imaged from 20 to 60 minutes post injection, see the Results subsection “Epinephrine and norepinephrine restore the Reissner fiber-dependent calcium signaling in ventral CSF-cNs of scospondin mutants”and in the Materials and methods subsection “In vivo calcium imaging”).

Second, we assessed experimentally whether norepinephrine delivered through HBV injection accessed the central canal of the spinal cord, was stable and present in excess in the CSF to trigger long-range signaling along the antero-posterior axis of the embryos. To address these points, we perfomed immunostainings against norepinephrine (no antibody is available to detect epinephrine) 30 and 60 minutes post HBV injection of norepinephrine diluted to 3mM in aCSF or aCSF only (“control injection”). The results are now depicted in a Figure 5—figure supplement 1. Our assay shows that norepinephrine-positive signal is present in the central canal 30 and 60 minutes post-injection in excess compared to control injections. These observations further confirms that norepinephrine injected in the HBV can diffuse down the central canal and is stable in the conditions used for in vivo calcium imaging. These results are described in the subsection “Epinephrine and norepinephrine restore the Reissner fiber-dependent calcium signaling in ventral CSF-cNs of scospondin mutants”. Note that our observations are in line with former studies using tritiated norepinephrine (3H-NE) injected into cerebral ventricles of dogs (Maas and Landis, 1965), sheep (Forbes and Bail, 1974) and rats (Fuxe and Ungerstedt, 1966, Levitt, Kowalik and Barkai, 1983) showing that 3H-NE is depleted 5 to 6 hours after the initial injection (see subsection “Epinephrine and norepinephrine restore the Reissner fiber-dependent calcium signaling in ventral CSF-cNs of scospondin mutants”).

2) Double immunostaining with anti-GFP and anti-norepinephrine, and anti-Adrb2 in pkd2l1:GCAMP fish.

We thank the reviewers for requesting important precisions here.

First, we assessed whether norepinephrine can be associated with the Reissner fiber and/or Reissner fiber-positive material in vivo at 30 hpf in the central canal of the spinal cord. We performed double immunostainings against norepinephrine (NE) and GFP in Tg(scospondin-GFP) embryos. We have extended our initial observation to 16 other embryos as shown in the new Figure 6A. Our results show that in 10 out of 16 embryos newly analyzed, NE-positive spots are also detected on the fiber itself or associated with GFP-positive deposits in the central canal. Moreover, NE-positive signals were also detected in close apposition to the massa caudalis, the structure formed by the aggregation of Reissner-positive material at the caudal limit of the central canal. To highlight these different co-localization or apposition patterns, we now show merged images of both signals in the novel Figure 6A exemplified on several embryos and further describe this result in the subsection “Norepinephrine can be detected in the embryonic CSF and adrenergic receptors are expressed by spinal cells contacting the CSF”.

Second, we specified the localization of the Adrb2 signal relative to CSF-cNs. To answer this question, we performed double immunostainings against Adrb2 and GFP on Tg(pkd2l1:GCaMP5) 30 hpf embryos (Figure 6B). Our results show that Adrb2 is not expressed in CSF-cNs but rather in more medial cells, which – according to their cuboidal shape and medial localization in the ventral part of the neural tube – likely correspond to the medial floor plate (see novel Figure 6B). This confirms that an adrenergic signal can be received in the spinal central canal, and suggests that monoamines act indirectly on CSF-cNs. Importantly, this expression pattern is conserved in scospondin mutants, suggesting that the defect in calcium signaling observed in CSF-cNs is unlikely due to a defect in the receptor localization in the absence of the RF (see the aforementioned subsection).

3) Justify the use of relatively late stage embryos (i.e. 30 hpf vs. 24 hpf). Provide images of scospondin mutants at the 20-26 hpf window.

As stated in our previous publication (Cantaut-Belarif et al., 2018), the curled-down phenotype becomes obvious in scospondin mutants at 28-30 hpf. We had noticed that scospondin mutants could not be phenotypically recognized earlier than this stage. This is the reason why 28-30 hpf and 48 hpf embryos were solely used to identify scospondin mutants according to their specific curled phenotype. The 28-30 hpf stage corresponds to a developmental time where calcium variations are very important in the wild-type ventral CSF-cNs (Sternberg et al., 2018). This is stated in the revised manuscript to justify our choice (subsections “The Reissner fiber controls urp2 gene expression” and “The Reissner fiber is required for calcium signaling in urp2 expressing CSF-cNs”).

In addition, to better illustrate the evolution of the posterior axis geometry between 20 and 30 hpf, we imaged the evolution of the posterior axis geometry over time on animals generated from incrosses of adult scospondinicm15/* parents. We provide now images of a representative scospondinicm15/icm15 mutant and a control sibling at 20, 22, 24, 28 and 30 hpf in the revised version of the manuscript as Figure 1—figure supplement 1, which further confirms our previous observation regarding the onset of the curled down phenotype (Cantaut-Belarif et al., 2018).

4) Detailed protocols are needed.

We now detailed the protocols in the revised version of the manuscript, especially drug treatments, brain ventricle injections and immunohistochemistry procedures (see the Materials and methods section).

5) Editorial revision should include comments on similarities and differences with Lu et al.

We have now highlighted the similarities and differences with Lu et al. in the revised version of the manuscript.

Similarly to Lu et al., 2020: we found that in scospondin mutants epinephrine can compensate for the loss of the Reissner fiber on body axis curvature defects and urp neuropeptides expression. However, we add to this previous observation that norepinephrine can also act the same (see the Discussion subsection “Adrenergic activation restores the Reissner fiber-dependent signaling and axis straightening”).

Note that in contrast to Lu et al., we used here a quantitative approach to measure the effect of both monoamines on urp gene expression (using quantitative PCR on numerous independent samples instead of in situ hybridization) and body axis curvature (systematic ear-to-tail angle measurements on independent experimental groups).

In contrast to Lu et al., 2020: we report here a downregulation of urp2 gene expression only and not urp1 in scospondin mutants (subsection “urp2 expression in ventral CSF-cNs depends on the presence of the Reissner fiber and impacts on the curvature of embryonic axis”). Thus, we contradict the idea that the Reissner fiber is necessary for the expression of both neuropeptides and rather show that urp2 expression only is dependent on the Reissner fiber.

https://doi.org/10.7554/eLife.59469.sa2

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  1. Yasmine Cantaut-Belarif
  2. Adeline Orts Del'Immagine
  3. Margot Penru
  4. Guillaume Pézeron
  5. Claire Wyart
  6. Pierre-Luc Bardet
(2020)
Adrenergic activation modulates the signal from the Reissner fiber to cerebrospinal fluid-contacting neurons during development
eLife 9:e59469.
https://doi.org/10.7554/eLife.59469

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https://doi.org/10.7554/eLife.59469