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Fig. S2

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ZDB-IMAGE-191024-6
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Figures for Djannatian et al., 2019
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Fig. S2

Electron micrographs reperesent dorsal spinal cord cross-sections of 10 dpf wt and cntn1b-/-mag-/-zebrafish. Total numbers of myelinated axons in electron micrographs of 10 dpf wt and mutant dorsal spinal cord cross-sections. = 3 fish, one-way ANOVA: < 0.0001. Number of oligodendrocytes in 3 dpf anterior dorsal spinal cords of wt and mutant Tg(mbp:EGFP-CAAX) zebrafish larvae. = 8-10 fish, one-way ANOVA: < 0.0049. Myelin sheaths of single oligodendrocytes in 3 dpf wild-type (top) and cntn1b-/-mag-/- (bottom) fish. Number of myelin sheaths per oligodendrocyte in 3 dpf wt and mutant fish. Sheaths from 20 oligodendrocytes per genotype from 5-7 fish were quantified. One-way ANOVA: < 0.0001. Ensheathed cell bodies in 4 dpf caspr-/- (reproduced from Fig. 1a) and caspr-/-mag-/- fish. Ensheathed cell bodies per myelinated area at 4 dpf (= 8-10, one-way ANOVA: = 0.0001). Quantifications for wt and single mutants were reproduced from Fig. 1b. Representative wild type (wt) and mutant myelin sheaths of zebrafish commissural neurons at 4 dpf. Sheath length at 4 dpf (means of 30 sheaths per animal, = 3, one-way ANOVA, < 0.0001). j-m CNS myelination of 4 dpf nfascb-/-cntn1b-/- fish in comparison to nfascb-/-littermates. (j) Representative images of CNS myelin. (k) Ensheathed cell bodies per myelinated area (= 6, unpaired two-sided t test: = 0.0482). (l) Sheath length (means of 30 sheaths per animal, = 3, unpaired two-sided t test, < 0.2111). (m) Double sheaths (sheaths with fluorescence intensity steps combined with caliber changes, as depicted in Fig. 4a) normalized to myelinated area (= 6, unpaired two-sided t test, < 0.1877). Confocal images (d,f,h,j) are maximum intensity projections of Tg(mbp:EGFP-CAAX) zebrafish dorsal spinal cord. Bonferroni-corrected values, *0.05, **<0.01, ***<0.001. Data are presented as means ± s.d. Scale bars, 1 μm (a), 10 μm (d,f,h,j). Source data are provided as a Source Data file. 

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