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在响应蜗牛(Snail)和E47转录因子的表达时,激活的细胞外信号调节激酶/丝裂原活化蛋白激酶(Erk/MAPK)途径可诱导MDCK上皮细胞中Id-1的产生。

Id-1 is induced in MDCK epithelial cells by activated Erk/MAPK pathway in response to expression of the Snail and E47 transcription factors.

作者信息

Jordà Mireia, Vinyals Antònia, Marazuela Anna, Cubillo Eva, Olmeda David, Valero Eva, Cano Amparo, Fabra Angels

机构信息

IDIBELL-Institut de Recerca Oncològica, Centre d'Oncologia Molecular, Barcelona, Spain.

出版信息

Exp Cell Res. 2007 Jul 1;313(11):2389-403. doi: 10.1016/j.yexcr.2007.04.001. Epub 2007 May 9.

DOI:10.1016/j.yexcr.2007.04.001
PMID:17490644
Abstract

Id-1, a member of the helix-loop-helix transcription factor family has been shown to be involved in cell proliferation, angiogenesis and invasion of many types of human cancers. We have previously shown that stable expression of E47 and Snail repressors of the E-cadherin promoter in MDCK epithelial cell line triggers epithelial mesenchymal transition (EMT) concomitantly with changes in gene expression. We show here that both factors activate the Id-1 gene promoter and induce Id-1 mRNA and protein. The upregulation of the Id-1 gene occurs through the transactivation of the promoter by the Erk/MAPK signaling pathway. Moreover, oncogenic Ras is also able to activate Id-1 promoter in MDCK cells in the absence of both E47 and Snail transcription factors. Several transcriptionally active regulatory elements have been identified in the proximal promoter, including AP-1, Sp1 and four putative E-boxes. By EMSA, we only detected an increased binding to Sp1 and AP-1 elements in E47- and Snail-expressing cells. Binding is affected by the treatment of cells with PD 98059 MEK inhibitor, suggesting that MAPK/Erk contributes to the recruitment or assembly of proteins to Id-1 promoter. Small interfering RNA directed against Sp1 reduced Id-1 expression and the upregulation of the promoter, indicating that Sp1 is required for Id-1 induction in E47- and Snail-expressing cells. Our results provide new insights into how some target genes are activated during and/or as a consequence of the EMT triggered by both E47 and Snail transcription factors.

摘要

Id-1是螺旋-环-螺旋转录因子家族的成员之一,已被证明与多种人类癌症的细胞增殖、血管生成和侵袭有关。我们之前已经表明,在MDCK上皮细胞系中,E-钙黏蛋白启动子的E47和Snail阻遏物的稳定表达会触发上皮-间质转化(EMT),同时伴随着基因表达的变化。我们在此表明,这两种因子均可激活Id-1基因启动子并诱导Id-1 mRNA和蛋白的产生。Id-1基因的上调是通过Erk/MAPK信号通路对启动子的反式激活而发生的。此外,致癌性Ras在缺乏E47和Snail转录因子的情况下,也能够激活MDCK细胞中的Id-1启动子。在近端启动子中已鉴定出几个具有转录活性的调控元件,包括AP-1、Sp1和四个假定的E-盒。通过电泳迁移率变动分析(EMSA),我们仅在表达E47和Snail的细胞中检测到与Sp1和AP-1元件的结合增加。用PD 98059 MEK抑制剂处理细胞会影响这种结合,这表明MAPK/Erk有助于蛋白质募集或组装到Id-1启动子上。针对Sp1的小干扰RNA降低了Id-1的表达以及启动子的上调,这表明Sp1是在表达E47和Snail的细胞中诱导Id-1所必需的。我们的研究结果为在E47和Snail转录因子触发的EMT过程中和/或作为其结果时某些靶基因如何被激活提供了新的见解。

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