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Fig. 1. Bmpr1a function is not required for embryonic retinal development.
Control samples are from Bmpr1a+/fx;Cre mice and
mutants are from Bmpr1a-/fx;Cre mice. (A)
Hematoxylin and Eosin stained sections of the adult retina from 3-month-old
mice. Retinal lamination pattern and cell types are unaltered in the
Bmpr1a-/fx;Cre mutants (right), compared with
control littermates. (B) Anterograde tracing of retinal ganglion cell axons
into the superior colliculus of the midbrain of control (left) and mutant
(right). Fluorescent images of the left half of the midbrain of 9-day-old pups
that have received a focal injection of DiI into the right dorsal retina,
arrow indicates termination zone of dorsal axons. The axes in the left
superior colliculus are indicated; a, anterior; l, lateral; m, medial; p,
posterior. (C) Schematic representation of the Bmpr1a genomic locus
and various mutant alleles. (D) Genomic PCR to detect Bmpr1a alleles
using primers indicated in C. The genotypes of the sample DNAs are indicated
at the top. In the retina of adult mice carrying the Cre transgene, the
amplicon for the conditional allele (fx) is undetectable (arrowhead),
whereas in the tail the PCR product corresponding to the unrecombined
conditional allele is readily detected. Consistent with recombination of the
floxed allele occurring only in the retina, the dE2 amplicon, which
represents the recombined allele with exon 2 removed, is present only in the
retina of mice carrying the Cre transgene. gcl, ganglion cell layer; inl,
inner nuclear layer; onl, outer nuclear layer; rpe, retinal pigment
epithelium.
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