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小鼠肝脏中雌激素受体α结合位点的全基因组鉴定。

Genome-wide identification of estrogen receptor alpha-binding sites in mouse liver.

作者信息

Gao Hui, Fält Susann, Sandelin Albin, Gustafsson Jan-Ake, Dahlman-Wright Karin

机构信息

Department of Biosciences and Nutrition, Karolinska Institutet, Novum, S-14157 Huddinge, Sweden.

出版信息

Mol Endocrinol. 2008 Jan;22(1):10-22. doi: 10.1210/me.2007-0121. Epub 2007 Sep 27.

Abstract

We report the genome-wide identification of estrogen receptor alpha (ERalpha)-binding regions in mouse liver using a combination of chromatin immunoprecipitation and tiled microarrays that cover all nonrepetitive sequences in the mouse genome. This analysis identified 5568 ERalpha-binding regions. In agreement with what has previously been reported for human cell lines, many ERalpha-binding regions are located far away from transcription start sites; approximately 40% of ERalpha-binding regions are located within 10 kb of annotated transcription start sites. Almost 50% of ERalpha-binding regions overlap genes. The majority of ERalpha-binding regions lie in regions that are evolutionarily conserved between human and mouse. Motif-finding algorithms identified the estrogen response element, and variants thereof, together with binding sites for activator protein 1, basic-helix-loop-helix proteins, ETS proteins, and Forkhead proteins as the most common motifs present in identified ERalpha-binding regions. To correlate ERalpha binding to the promoter of specific genes, with changes in expression levels of the corresponding mRNAs, expression levels of selected mRNAs were assayed in livers 2, 4, and 6 h after treatment with ERalpha-selective agonist propyl pyrazole triol. Five of these eight selected genes, Shp, Stat3, Pdgds, Pck1, and Pdk4, all responded to propyl pyrazole triol after 4 h treatment. These results extend our previous studies using gene expression profiling to characterize estrogen signaling in mouse liver, by characterizing the first step in this signaling cascade, the binding of ERalpha to DNA in intact chromatin.

摘要

我们运用染色质免疫沉淀技术与覆盖小鼠基因组所有非重复序列的平铺式微阵列相结合的方法,报告了在小鼠肝脏中对雌激素受体α(ERα)结合区域的全基因组鉴定。该分析确定了5568个ERα结合区域。与之前关于人类细胞系的报道一致,许多ERα结合区域远离转录起始位点;约40%的ERα结合区域位于注释转录起始位点的10 kb范围内。几乎50%的ERα结合区域与基因重叠。大多数ERα结合区域位于人类和小鼠之间进化保守的区域。基序查找算法确定雌激素反应元件及其变体,以及激活蛋白1、碱性螺旋-环-螺旋蛋白、ETS蛋白和叉头蛋白的结合位点是在已鉴定的ERα结合区域中最常见的基序。为了将ERα与特定基因启动子的结合与相应mRNA表达水平的变化相关联,在用ERα选择性激动剂丙基吡唑三醇处理后2、4和6小时,测定了肝脏中选定mRNA的表达水平。在这八个选定基因中,Shp、Stat3、Pdgds、Pck1和Pdk4这五个基因在处理4小时后均对丙基吡唑三醇有反应。这些结果通过表征该信号级联反应的第一步,即ERα在完整染色质中与DNA的结合,扩展了我们之前利用基因表达谱来表征小鼠肝脏中雌激素信号传导的研究。

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