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血液和内皮细胞中内皮糖蛋白的表达受Ets/Gata成血管细胞编码的模块化组装差异调控。

Endoglin expression in blood and endothelium is differentially regulated by modular assembly of the Ets/Gata hemangioblast code.

作者信息

Pimanda John E, Chan Wan Y I, Wilson Nicola K, Smith Aileen M, Kinston Sarah, Knezevic Kathy, Janes Mary E, Landry Josette-Renée, Kolb-Kokocinski Anja, Frampton Jonathan, Tannahill David, Ottersbach Katrin, Follows George A, Lacaud Georges, Kouskoff Valerie, Göttgens Berthold

机构信息

Department of Haematology, Cambridge Institute for Medical Research, University of Cambridge, Cambridge, United Kingdom.

出版信息

Blood. 2008 Dec 1;112(12):4512-22. doi: 10.1182/blood-2008-05-157560. Epub 2008 Sep 19.

Abstract

Endoglin is an accessory receptor for TGF-beta signaling and is required for normal hemangioblast, early hematopoietic, and vascular development. We have previously shown that an upstream enhancer, Eng -8, together with the promoter region, mediates robust endothelial expression yet is inactive in blood. To identify hematopoietic regulatory elements, we used array-based methods to determine chromatin accessibility across the entire locus. Subsequent transgenic analysis of candidate elements showed that an endothelial enhancer at Eng +9 when combined with an element at Eng +7 functions as a strong hemato-endothelial enhancer. Chromatin immunoprecipitation (ChIP)-chip analysis demonstrated specific binding of Ets factors to the promoter as well as to the -8, +7+9 enhancers in both blood and endothelial cells. By contrast Pu.1, an Ets factor specific to the blood lineage, and Gata2 binding was only detected in blood. Gata2 was bound only at +7 and GATA motifs were required for hematopoietic activity. This modular assembly of regulators gives blood and endothelial cells the regulatory freedom to independently fine-tune gene expression and emphasizes the role of regulatory divergence in driving functional divergence.

摘要

内皮糖蛋白是转化生长因子-β信号传导的辅助受体,对于正常的成血管细胞、早期造血及血管发育是必需的。我们之前已经表明,一个上游增强子Eng -8与启动子区域一起介导了强大的内皮细胞表达,但在血液中无活性。为了鉴定造血调控元件,我们使用基于芯片的方法来确定整个基因座的染色质可及性。随后对候选元件的转基因分析表明,Eng +9处的一个内皮细胞增强子与Eng +7处的一个元件结合时,可作为一个强大的造血-内皮细胞增强子发挥作用。染色质免疫沉淀(ChIP)芯片分析表明,Ets因子在血液和内皮细胞中均特异性结合到启动子以及-8、+7和+9增强子上。相比之下,血液谱系特异性的Ets因子Pu.1以及Gata2的结合仅在血液中检测到。Gata2仅结合在+7处,并且造血活性需要GATA基序。这种调控因子的模块化组装赋予血液和内皮细胞独立微调基因表达的调控自由度,并强调了调控差异在驱动功能差异中的作用。

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