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Fig. 6. BMP4 signaling is required for the differentiation of the distal UB into
the ureter. (A) The Cre-flox system was used to conditionally
remove exons 3 and 4 of the Bmp4 gene. The presence of the
loxP sites flanking the Bmp4 allele and the occurrence of
the recombination event were confirmed through genotyping using specific PCR
primers. (B,C) In situ analysis of Bmp4 expression was
performed on rudiments isolated from E12.5 embryos and cultured for 4 days.
Expression of Bmp4 mRNA is detected in the
Bmp4flox/flox rudiments (B), whereas no Bmp4 is
detectable in Bmp4flox/flox;Cre-Esr1 mutant
rudiments (C). (D-K) Metanephric rudiments from E12.5
Bmp4flox/flox or
Bmp4flox/flox;Cre-Esr1 mutant embryos were
cultured for 4 days with 4-OH tamoxifen. Rudiments were analyzed as whole
mounts using E-cadherin expression to visualize the UB network (red) and
uroplakin (green, D-G) or SMA (green, H-K) to detect ureter differentiation.
Uroplakin expression can readily be detected in
Bmp4flox/flox cultures (D,F), but is difficult to detect
in the Bmp4flox/flox;Cre-Esr1 rudiments (E,G).
Bmp4flox/flox rudiments develop an SMA-positive coat (H,J)
that condenses around the distal domain of the UB. In the
Bmp4flox/flox;Cre-Esr1 rudiments, only a few unorganized
SMA-positive cells are detected (I,K).
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