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Fig. 1. Generation of Bmp4S2G mice. (A) Schematic
illustration of cleavage patterns of wild-type and S2G mutant forms of
proBMP4. (B) Wild-type or mutant forms of the BMP4 precursor were
expressed in HEK 293 cells and cleavage products analyzed by probing western
blots of cell lysates with anti-HA antibody which recognizes an epitope tag
present in the prodomain. Bands corresponding to uncleaved precursor, intact
prodomain following cleavage at the S1 site, and intact prodomain following
cleavage at the S2 site are indicated. Introduction of a point mutation
[BMP4(mS2G)] that prevents cleavage at the S2 site still allows for cleavage
at the S1 site whereas both sites are cleaved in native proBMP4. Mature BMP4
cleaved from either precursor migrates with an identical molecular mass (data
not shown). (C) Genomic organization of the wild-type Bmp4
allele, the targeting vector and the Bmp4S2Gneo allele.
The positions of the probes used for Southern analysis, and primers for PCR
genotyping (arrows) are indicated. (D) Southern blot analysis of
genomic DNA from targeted (H6, 2D8 and 2A10) or non-targeted (ES) ES cells.
Genomic DNA was digested as indicated and probed with the internal (probe 2)
or external (probe 3) genomic fragments shown in panel C. (E) PCR
genotyping of progeny generated by interbreeding Bmp4S2G/+
mice. The PCR product generated by the mutant allele is 293 bp and that
generated by the wild-type allele is 259 bp.
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