|
|
|
|
|
|
|
||||
| Home Help Feedback Subscriptions Archive Search Table of Contents | ||||
|
Fig. 1. Schematic representation of the MgntZ targeting
vector and recombination at the Mgn locus. (A) Restriction
map of the wild-type Mgn locus. Broken lines indicate regions of
homology in the targeting vector. (B) Restriction map of the
MgntZ targeting vector. (C) The predicted structure
of a mutated Mgn allele following homologous recombination. The
horizontal bars (5' and 3' external probe) indicate the DNA
fragment used for Southern blot analysis. (D) Targeted locus after
removing neomycin cassette (neo) by Cre-mediated excision at the loxP
sites. (E) Southern blot analysis of restriction enzyme-digested DNA
from targeted MgntZ (+/tZ) and wild-type (+/+)
animals with 5' and 3' external probes (the same strategy was used
to detect littermates from heterozygous intercrosses). wt and mt indicate the
position of the wild-type and the mutated allele, respectively. (F)
Southern blot containing genomic DNA upon SacII digestion and probed
with an internal probe, indicating proper excision of the neomycin gene
(
neo). (G) Heteroduplex PCR (primers for the mutant allele,
MM107 and tlacZ; primers for the wild-type allele, MM108 and MM109) used to
identify mutated embryos/mice. (H) RT-PCR with specific primers for the
bHLH domain of Mgn (MM111D and MM112R). The 250 bp band is missing in
the MgntZ/tZ mice.
|
