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Figure 2


Fig. 2. Targeted replacement of wild-type Sox10 by mutant Sox10 sequences in mice. (A) Schematic showing, from top to bottom, the targeting construct for the Sox10 {Delta}K2 mutation, the Sox10 wild-type locus and the mutant locus before and after Cre recombination. The Sox10 exons (I-V) and the mutant Sox10 {Delta}K2 open reading frame (ORF) are shown as boxes, the 4.5 kb and 1.5 kb flanking regions as bars. Regions of homology between wild-type locus and targeting vector are depicted as thick black lines, introns III and IV as thin open boxes and surrounding genomic regions not contained in the targeting construct as dashed lines. Plasmid backbone sequences of the targeting construct are indicated by a thin line. Restriction sites for NcoI (N), BamHI (H) and ScaI (S) are shown, as are the locations of the 5' and 3' probes and the start codon of the Sox10 gene (ATG). The arrowheads indicate the locations of primers 1,2,3,4 used for quantitative RT-PCR. neo, neomycin resistance cassette; loxP, recognition sites for Cre recombinase; Tk, herpes simplex virus thymidine kinase gene cassette. (B) Schematic of the mutant locus for the Sox10 aa1 mutation. Recombination into the Sox10 genomic locus was as depicted for the Sox10 {Delta}K2 construct. (C) Southern blot analysis of DNA from wild-type (wt) and heterozygous (+/aa1 and +/{Delta}K2) ES cells digested with NcoI for use with the 5' probe, and with BamHI/ScaI for the 3' probe. The size of bands corresponding to the wild-type (6.6 kb for the 5' probe and 4.6 kb for the 3' probe) and the targeted alleles (10.9 and 5.9 kb, respectively, for the 5' probe; 10.2 and 10.4 kb, respectively, for the 3' probe) are indicated. (D) PCR genotyping of wild-type (wt), heterozygous (+/{Delta}K2 and +/aa1) and homozygous ({Delta}K2/{Delta}K2 and aa1/aa1) mouse embryos at 18.5 dpc. DNA fragments in the size marker (M) are 1.0 kb and 0.5 kb.





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