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Fig. 9. Analysis of the sexual differentiation phenotype in mutants with somatic
cell-restricted loss of β-catenin. (A,B)
Whole-mount ISH with the indicated RNA probes was performed with XX E12.5
gonads from wild-type and
Sf1-Cre/β-catflox/flox (where
β-cat is Ctnnb1) mouse embryos (A) or with E13.5 XY
gonads from wild-type and XX
Sf1-Cre/β-catflox/flox embryos (B) to
examine the status of the female (A) and the male (B) pathway in XX gonads
upon β-catenin loss. (C) qRT-PCR analysis of gene expression in
the XX E12.5 wild-type and
Sf1-Cre/β-catflox/flox gonads. The data are
shown as the ratio of normalized expression (gene/Gapdh RNA copy
number) in wild-type over mutant samples. The combined
*Wnt4 level in the gonad-mesonephros block does not
change; see the corresponding panel in A for gonadal Wnt4 expression.
(D,E) Double immunofluorescent staining of E18.5 gonadal
sections for either 
H2AX (D; red) or SYN/COR (E; red) and PECAM1
(green). The wild-type E18.5 ovary contains numerous germ cells with
H2AX (D, top panel) or SYN1 (synapsin I) staining (E, top left). In the
XX Sf1-Cre/β-catflox/flox XX gonad, germ
cells are largely lost; no SYN1-positive cells are observed in the control or
Sf1-Cre/β-catflox/flox testis.
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