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Genetic mapping of an insertional hydrocephalus-inducing mutation allelic to hy3
Authors:Michael L Robinson  Carl E Allen  Brian E Davy  William J Durfee  Frederick F Elder  Christopher S Elliott  Wilbur R Harrison
Institution:(1) Division of Molecular and Human Genetics, Dept. of Pediatrics, and Children's Research Institute, The Ohio State University, Children's Research Institute, 700 Children's Drive, Rm. W492, Columbus, Ohio 43205, USA, US;(2) Animal Resource Center, Case Western Reserve University, School of Medicine, Cleveland, Ohio, USA, US;(3) Dept. of Pathology, The University of Texas Southwestern Medical Center, Dallas, Texas, USA, US;(4) Dept. of Molecular and Cellular Biology, Baylor College of Medicine, Houston, Texas, USA, US
Abstract:The transgenic mouse line OVE459 carries a transgene-induced insertional mutation resulting in autosomal recessive congenital hydrocephalus. Homozygous transgenic animals experience ventricular dilation with perinatal onset and are noticeably smaller than hemizygous or non-transgenic littermates within a few days after birth. Fluorescence in situ hybridization (FISH) revealed that the transgene inserted in a single locus on mouse Chromosome (chr) 8, region D2-E1. Genetic crosses between hemizygous OVE459 mice and mice heterozygous for the spontaneous mutation hydrocephalus-3 (hy3) produced hydrocephalic offspring with a frequency of 22%, demonstrating that these two mutations are allelic. A genomic library was made by using DNA from homozygous OVE459 mice, and genomic DNA flanking the transgene insertion site was isolated and sequenced. A PCR polymorphism between C57BL/6 DNA and Mus spretus was used to map the location of the transgene insert to 1.06 cM ± 0.75 proximal to D8Mit152 by using the Jackson Laboratory Backcross DNA Panel Mapping Resource. Furthermore, sequence analysis from a mouse bacterial artificial chromosome (BAC) clone, positive for unique markers on both sides of the transgene insertion site, demonstrated that the genomic DNAs flanking each side of the transgene insertion are physically separated by approximately 51 kb on the wild-type mouse chromosome.
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