Fig. 5 Knockdown of ncam1a in ncam1b mutants phenocopies the ncam1b knockdown phenotype. (A–E) Lateral views of 48 hpf Tg(ClaudinB::lynGFP) (A) Wild type uninjected (WT uni) (B) n1b -/- Del uninjected, (C) n1b MO in WT, (D) ncam1a MO in WT and (E) ncam1a MO in n1b -/- Del. Embryos are oriented with rostral to the left and dorsal to the top. (A) At 48 hpf, primI (star) of WT reaches the tip of the tail and deposits 5 proneuromasts (L1–L5). The migration distance was measured from the otic vesicle (ov) to primI. (B) n1b -/- Del mutants show the same phenotype as WT, with primI reaching the tip of the tail and 5 deposited proneuromasts. (C) ncam1b MO injection leads to reduced migration of smaller primI and deposition of fewer proneuromasts. (D) Injection of the ncam1a MO in wild type zebrafish caused moderate defects in lateral line system development, but these effects did not reach statistical significance. (E) ncam1a MO injection in n1b -/- Del induce reduced migration of a smaller primI and fewer deposited neuromasts. (F-H) Quantification of migration distance, primI length and number of proneuromasts. Bars indicate mean values of the medians of each experiment, with error bars representing standard error. Differences between the five groups were analyzed using a one-way ANOVA followed by Scheffé post hoc tests. Differences were considered significant if the F-value exceeded the critical Scheffé value (p < 0.05). Groups that share the same letter do not differ significantly. Groups with different letters show significant differences in their means. Scale bar 200 µm. Abbreviations: WT: Wild type; n1b -/- Del: ncam1b deletion mutant; MO: Morpholino; uni: uninjected; primI: primordium; pnm: proneuromast; ov: otic vesicle.
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Full text @ Eur. J. Cell Biol.