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同源结构域蛋白BARX2新型结合元件及基因靶点的鉴定

Identification of novel binding elements and gene targets for the homeodomain protein BARX2.

作者信息

Stevens Tracy A, Iacovoni Jason S, Edelman David B, Meech Robyn

机构信息

Department of Neurobiology, The Scripps Research Institute, La Jolla, California 92037, USA.

出版信息

J Biol Chem. 2004 Apr 9;279(15):14520-30. doi: 10.1074/jbc.M310259200. Epub 2004 Jan 26.

DOI:10.1074/jbc.M310259200
PMID:14744868
Abstract

BARX2 is a homeobox transcription factor that influences cellular differentiation in various developmental contexts. To begin to identify the gene targets that mediate its effects, chromatin immunoprecipitation (ChIP) was used to isolate BARX2 binding sites from the human MCF7 breast cancer cell line. Cloning and sequencing of BARX2-ChIP-derived DNA fragments identified 60 potential BARX2 target loci that were proximal to or within introns of genes involved in cytoskeletal organization, cell adhesion, growth factor signaling, transcriptional regulation, and RNA metabolism. The sequences of over half of the fragments showed homology with the mouse genome, and several sequences could be mapped to orthologous human and mouse genes. Binding of BARX2 to 21 genomic loci examined was confirmed quantitatively by replicate ChIP assays. A combination of sequence analysis and electrophoretic mobility shift assays revealed homeodomain binding sites within several fragments that bind to BARX2 in vitro. The majority of BARX2 binding fragments tested (14/19), also affected transcription in luciferase reporter gene assays. Mutation analyses of three fragments showed that their transcriptional activities required the HBS, and suggested that BARX2 regulates gene expression by binding to DNA elements containing paired TAAT motifs that are separated by a poly(T) sequence. Inhibition of BARX2 expression in MCF7 cells led to reduced expression of eight genes associated with BARX2 binding sites, indicating that BARX2 directly regulates their expression. The data suggest that BARX2 can coordinate the expression of a network of genes that influence the growth of MCF7 cells.

摘要

BARX2是一种同源盒转录因子,在多种发育环境中影响细胞分化。为了开始鉴定介导其作用的基因靶点,采用染色质免疫沉淀(ChIP)技术从人MCF7乳腺癌细胞系中分离出BARX2结合位点。对BARX2-ChIP衍生的DNA片段进行克隆和测序,确定了60个潜在的BARX2靶基因座,这些基因座位于参与细胞骨架组织、细胞粘附、生长因子信号传导、转录调控和RNA代谢的基因的内含子附近或内部。超过一半的片段序列与小鼠基因组具有同源性,并且几个序列可以定位到直系同源的人类和小鼠基因。通过重复的ChIP分析定量证实了BARX2与21个检测的基因组位点的结合。序列分析和电泳迁移率变动分析相结合,揭示了几个片段中的同源结构域结合位点,这些位点在体外与BARX2结合。大多数测试的BARX2结合片段(14/19)在荧光素酶报告基因分析中也影响转录。对三个片段的突变分析表明,它们的转录活性需要同源结构域结合位点(HBS),并表明BARX2通过与包含由聚(T)序列隔开的成对TAAT基序的DNA元件结合来调节基因表达。抑制MCF7细胞中BARX2的表达导致与BARX2结合位点相关的八个基因的表达降低,表明BARX2直接调节它们的表达。数据表明,BARX2可以协调影响MCF7细胞生长的基因网络的表达。

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