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Fig. 3. Hair cells are dramatically increased in Dll1/Jag2 double mutant
cochleae, whereas supporting cells are only modestly reduced. (A-D) Myosin
VIIa (red), p27kip1 (green) and DAPI (blue nuclear stain)
immunostained sections from E18.5
Dll1hyp/-Jag2-/- mutant and control cochleae.
Supporting cells are clearly still present in
Dll1hyp/-Jag2-/- mutant cochleae, as shown by
the p27kip1-stained cells. However, some p27kip1-stained
cells (presumably Deiter's cells) appeared to be missing in some sections
(C,D, arrows). (E-H) E18.5 cochleae processed for in situ hybridization using
the indicated probes. Expression of 
-tectorin or ß-tectorin in the
various supporting cell populations did not appear to differ between controls
and mutants, with the exception of ß-tectorin expression in Deiter's
cells (H), which appears to be disorganized and reduced. (I) Hair and
supporting cell counts from sections, as shown in A-D. Sections from three
ears were counted for each group, either control or
Dll1hyp/-Jag2-/-. Controls were either wild
type, or Dll1 or Jag2 single heterozygotes. Counts of both
hair cells and supporting cells were significantly different between
Dll1hyp/-Jag2-/- mutant and control cochleae
(*P<0.001, Student's t-test). However, the
increase in hair cells did not equal the supporting cell losses
(P<0.0001; one-way ANOVA). d, Deiter's cells; h, Hensen's cells;
Ko, Koelliker's organ; iPh, inner phalangeal cells; p, pillar cells. Scale
bars: in D, 50 µm for A-D; in H, 50 µm for E-H.
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