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人类GLI2启动子的克隆:转化生长因子-β通过SMAD3/β-连环蛋白协同作用进行转录激活。

Cloning of the human GLI2 Promoter: transcriptional activation by transforming growth factor-beta via SMAD3/beta-catenin cooperation.

作者信息

Dennler Sylviane, André Jocelyne, Verrecchia Franck, Mauviel Alain

机构信息

INSERM, U697, Université Paris-Diderot, 75010 Paris, France.

出版信息

J Biol Chem. 2009 Nov 13;284(46):31523-31. doi: 10.1074/jbc.M109.059964. Epub 2009 Sep 21.

Abstract

GLI2 (GLI-Kruppel family member 2), a zinc finger transcription factor that mediates Hedgehog signaling, is implicated in the progression of an ever-growing number of human malignancies, including prostate and pancreatic cancer, as well as basal cell carcinoma of the skin. Its expression is up-regulated by transforming growth factor-beta (TGF-beta) in a variety of cell types, both normal and transformed. We report herein that TGF-beta-driven GLI2 expression is transcriptional and does not result from stabilization of GLI2 transcripts. We describe the characterization of the 5'-flanking sequence of human GLI2 mRNA, the identification of a transcription start site, the cloning of approximately 1,600 bp of the regulatory promoter region and the identification and functional analysis of a TGF-beta-responsive region mapped to a 91-bp sequence between nucleotides -119 and -29 of the promoter. This region harbors SMAD and lymphoid enhancer factor/T cell factor binding sites that allow functional cooperation between SMAD3 and beta-catenin, recruited to the promoter in response to TGF-beta to drive GLI2 gene transcription.

摘要

GLI2(GLI-Kruppel家族成员2)是一种介导刺猬信号通路的锌指转录因子,与越来越多的人类恶性肿瘤进展有关,包括前列腺癌、胰腺癌以及皮肤基底细胞癌。在多种正常和转化细胞类型中,其表达受转化生长因子-β(TGF-β)上调。我们在此报告,TGF-β驱动的GLI2表达是转录性的,并非由GLI2转录本的稳定所致。我们描述了人类GLI2 mRNA 5'侧翼序列的特征、转录起始位点的鉴定、约1600 bp调控启动子区域的克隆,以及映射到启动子核苷酸-119至-29之间91 bp序列的TGF-β反应区域的鉴定和功能分析。该区域含有SMAD和淋巴样增强因子/T细胞因子结合位点,可使SMAD3和β-连环蛋白之间进行功能协作,它们响应TGF-β被招募到启动子以驱动GLI2基因转录。

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