Abnormal primordium patterning leads to loss of terminal neuromasts in the lef1nl2 mutant. (A,B) eya1 expression in the pLL of wild-type sibling and lef1nl2 mutant embryos at 2 dpf. The lef1nl2 mutant lacks a tc. (A′,B′) Distal limit of eya1 expression in wild-type and lef1nl2 mutant (arrow) embryos. (C) Average number of NMs (excluding tc) in lef1nl2 mutant and wild-type sibs (mean±s.d.) are not significantly different at 2 dpf (n=28 wild type, 11 lef1nl2, P=0.49, Student′s t-test). (D) Axial positions of L1-L5 in lef1nl2 and wild-type siblings at 2 dpf (mean±s.d.). The axial level of stalled primordium (prim) in lef1nl2 mutants is indicated by the pink bar. Position of L1-L5 is significantly shifted anteriorly in lef1nl2 mutants (n=18, P<0.001, two-way ANOVA with replication). (E-F′′) Stills from time-lapse movies of primordium migration in wild-type sibling and lef1nl2 mutant embryos that express the Tg(–8.0cldnb:lynGFP) transgene. Wild-type and lef1nl2 embryos were imaged beginning at 34 hpf for 780 minutes and 840 minutes, respectively (see Movies 1 and 2 in the supplementary material). (E-E′′) Over the course of 780 minutes, the primordium in the wild-type embryo migrated out of frame, deposited three NMs (red, blue and yellow asterisks) and generated two new rosettes (green and pink asterisks). (F-F′′′) Over the course of 840 minutes, the primordium in the lef1nl2 mutant has slowed and became elongated (pink asterisk), having deposited four NMs (red, blue, yellow and green asterisks). Scale bars: 20 μm.
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