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Fig. 5. Inca is required for cranial NC specification and survival after
migration into the arches in Xenopus and zebrafish. Embryos were
co-injected into one cell at the two-cell stage with Inca MO,
together with lacZ RNA as a lineage tracer and assayed for gene
expression by whole-mount in situ hybridization at stage 14 (A-D,
injected sides are on the left) and stage 32 (E-H; E,G, injected sides)
with probes indicated in the panels. In no case was any change in gene
expression observed on the injected side [(A) Slug, n=83; (B) Sox9,
n=42; (C) Sox2, n=47; (D) AP2a, n=54; (E) Dlx2,
n=63; (G) Sox9, n=78]. At tadpole stage, cranial cartilage
was eliminated on the injected side (left side in I). Control MO
injection had no effect (J). (K-R) TUNEL staining of embryos
injected with control MO (K,M,O) or Inca MO (L,N,P-R), cultured to
stage 21 (K,L), stage 30 (M,N) or stage 45 (O-R). Q and R are dorsal and
ventral views, respectively, of the tadpole shown in P. Black arrowheads
indicate strong TUNEL signal in neurocranium (Q) and jaw cartilage (R).
(S-Z) Confocal images of sox10:egfp expression in cranial NC
cells of controls (S,U,W,Y) and inca1 morphants (T,V,X,Z). Lateral
views, anterior to the left. Stages are indicated in the panels. First and
second pharyngeal arches are indicated in S,T, and derived cartilage elements
by arrowheads in Y,Z. Asterisks indicate expression of sox10:eGFP in the otic
vesicle.
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