Iterative inhibition of commissural growth cone exploration, not post-crossing barrier, ensures forward midline navigation through SlitC-PlxnA1 signaling

Ducuing, Hugo; Gardette, Thibault; Pignata, Aurora; Kindbeiter, Karine; Bozon, Muriel; Thoumine, Olivier; Delloye-Bourgeois, Céline; Tauszig-Delamasure, Servane; Castellani,

doi:10.1101/2020.04.21.051359

Cited by 2 publications

(2 citation statements)

References 60 publications

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“…Basal feet appeared to be enlarged and oriented parallel to commissural growth cones (Figure 13(c)). This was in line with previous reports in the chicken and mouse embryos (Campbell & Peterson, 1993;Ducuing et al, 2020;Yaginuma et al, 1991;Yoshioka & Tanaka, 1989).…”

Section: Discussionsupporting

confidence: 93%

Axon guidance at the spinal cord midline—A live imaging perspective

2021

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During neural circuit formation, axons navigate several choice points to reach their final target. At each one of these intermediate targets, growth cones need to switch responsiveness from attraction to repulsion in order to move on. Molecular mechanisms that allow for the precise timing of surface expression of a new set of receptors that support the switch in responsiveness are difficult to study in vivo. Mostly, mechanisms are inferred from the observation of snapshots of many different growth cones analyzed in different preparations of tissue harvested at distinct time points. However, to really understand the behavior of growth cones at choice points, a single growth cone should be followed arriving at and leaving the intermediate target. Existing ex vivo preparations, like cultures of an “open‐book” preparation of the spinal cord have been successfully used to study floor plate entry and exit, but artifacts prevent the analysis of growth cone behavior at the floor plate exit site. Here, we describe a novel spinal cord preparation that allows for live imaging of individual axons during navigation in their intact environment. When comparing growth cone behavior in our ex vivo system with snapshots from in vivo navigation, we do not see any differences. The possibility to observe the dynamics of single growth cones navigating their intermediate target allows for measuring growth speed, changes in morphology, or aberrant behavior, like stalling and wrong turning. Moreover, observation of the intermediate target—the floor plate—revealed its active participation and interaction with commissural axons during midline crossing.

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Section: Discussionsupporting

confidence: 93%

Axon guidance at the spinal cord midline—A live imaging perspective

2021

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“…However, the work presented in this article demonstrates that Slit-FL and Slit-N have dramatically different activities in vivo . The key to these findings was the identification of Tok as the Slit protease, allowing in vivo genetic manipulation of Slit fragments to uncover the independent biological function of Slit-N. Our results complement the few studies in which Slit-FL and Slit-N have been observed to have distinct activities ( Gohrig et al, 2014 ; Nguyen Ba-Charvet et al, 2001 ; Wang et al, 1999 ) as well as those that have attributed activities to a specific Slit fragment ( Wright et al, 2012 ; Ducuing et al, 2020 preprint; Caipo et al, 2020 ). As Slit cleavage and Tok family proteases are evolutionarily conserved ( Brose et al, 1999 ; Hopkins et al, 2007 ), it seems highly likely that processing of Slits by BMP-1/Tolloid family proteases will diversify the biological output of Slit signaling in many different systems.…”

Section: Discussionsupporting

confidence: 64%

Proteolytic cleavage of Slit by the Tolkin protease converts an axon repulsion cue to an axon growth cue in vivo

et al. 2020

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Slit is a secreted protein that has a canonical function of repelling growing axons from the CNS midline. The full-length Slit (Slit-FL) is cleaved into Slit-N and Slit-C fragments, which have potentially distinct functions via different receptors. Here we report that the BMP-1/Tolloid family metalloprotease, Tolkin (Tok), is responsible for Slit proteolysis in vivo and in vitro. In tok mutants lacking Slit cleavage, midline repulsion of axons occurs normally, confirming that Slit-FL is sufficient to repel axons. However, longitudinal axon guidance is highly disrupted in tok mutants and can be rescued by midline expression of Slit-N, suggesting that Slit is the primary substrate for Tok in the embryonic CNS. Transgenic restoration of Slit-N or Slit-C does repel axons in Slit-null animals. Slit-FL and Slit-N are both biologically active cues with distinct axon guidance functions in vivo. Slit signaling is used in diverse biological processes, thus differentiating between Slit-FL and Slit fragments will be essential for evaluating Slit function in broader contexts.

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Iterative inhibition of commissural growth cone exploration, not post-crossing barrier, ensures forward midline navigation through SlitC-PlxnA1 signaling

Cited by 2 publications

References 60 publications

Axon guidance at the spinal cord midline—A live imaging perspective

Axon guidance at the spinal cord midline—A live imaging perspective

Proteolytic cleavage of Slit by the Tolkin protease converts an axon repulsion cue to an axon growth cue in vivo

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