global analysis of gene expression in the developing brain of gtf2ird1 knockout mice全球的大脑发育的基因表达分析gtf2ird1基因敲除小鼠.pdfVIP

global analysis of gene expression in the developing brain of gtf2ird1 knockout mice全球的大脑发育的基因表达分析gtf2ird1基因敲除小鼠.pdf

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global analysis of gene expression in the developing brain of gtf2ird1 knockout mice全球的大脑发育的基因表达分析gtf2ird1基因敲除小鼠

Global Analysis of Gene Expression in the Developing Brain of Gtf2ird1 Knockout Mice 1 1,2 Jennifer O’Leary , Lucy R. Osborne * 1 Department of Molecular Genetics, University of Toronto, Toronto, Ontario, Canada, 2 Department of Medicine, University of Toronto, Toronto, Ontario, Canada Abstract Background: Williams-Beuren Syndrome (WBS) is a neurodevelopmental disorder caused by a hemizygous deletion of a 1.5 Mb region on chromosome 7q11.23 encompassing 26 genes. One of these genes, GTF2IRD1, codes for a putative transcription factor that is expressed throughout the brain during development. Genotype-phenotype studies in patients with atypical deletions of 7q11.23 implicate this gene in the neurological features of WBS, and Gtf2ird1 knockout mice show reduced innate fear and increased sociability, consistent with features of WBS. Multiple studies have identified in vitro target genes of GTF2IRD1, but we sought to identify in vivo targets in the mouse brain. Methodology/Principal Findings: We performed the first in vivo microarray screen for transcriptional targets of Gtf2ird1 in brain tissue from Gtf2ird1 knockout and wildtype mice at embryonic day 15.5 and at birth. Changes in gene expression in the mutant mice were moderate (0.5 to 2.5 fold) and of candidate genes with altered expression verified using real-time PCR, most were located on chromosome 5, within 10 Mb of Gtf2ird1. siRNA knock-down of Gtf2ird1 in two mouse neuronal cell lines failed to identify changes in expression of any of the genes identified from the microarray and subsequent analysis showed that differences in expression of genes on chromosome 5 were the result of retention of that chromosome region from the targeted embryonic stem cell line, and so were dependent upon strain rather than Gtf2ird1 genotype. In ad

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