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Ets因子GA结合蛋白α对TMS1/ASC的甲基化敏感调控。

Methylation-sensitive regulation of TMS1/ASC by the Ets factor, GA-binding protein-alpha.

作者信息

Lucas Mary E, Crider Krista S, Powell Doris R, Kapoor-Vazirani Priya, Vertino Paula M

机构信息

Graduate Program in Genetics and Molecular Biology, the Winship Cancer Institute, Emory University, Atlanta, Georgia 30322, USA.

出版信息

J Biol Chem. 2009 May 29;284(22):14698-709. doi: 10.1074/jbc.M901104200. Epub 2009 Mar 25.

Abstract

Epigenetic silencing involving the aberrant DNA methylation of promoter-associated CpG islands is one mechanism leading to the inactivation of tumor suppressor genes in human cancers. However, the molecular mechanisms underlying this event remains poorly understood. TMS1/ASC is a novel proapoptotic signaling factor that is subject to epigenetic silencing in human breast and other cancers. The TMS1 promoter is embedded within a CpG island that is unmethylated in normal cells and is spanned by three DNase I-hypersensitive sites (HS). Silencing of TMS1 in cancer cells is accompanied by local alterations in histone modification, remodeling of the HS, and hypermethylation of DNA. In this study, we probed the functional significance of the CpG island-specific HS. We identified a methylation-sensitive complex that bound a 55-bp intronic element corresponding to HS2. Affinity chromatography and mass spectrometry identified a component of this complex to be the GA-binding protein (GABP) alpha. Supershift analysis indicated that the GABPalpha binding partner, GABPbeta1, was also present in the complex. The HS2 element conferred a 3-fold enhancement in TMS1 promoter activity, which was dependent on both intact tandem ets binding sites and the presence of GABPalpha/beta1 in trans. GABPalpha was selectively enriched at HS2 in human cells, and its occupancy was inversely correlated with CpG island methylation. Down-regulation of GABPalpha led to a concomitant decrease in TMS1 expression. These data indicate that the intronic HS2 element acts in cis to maintain transcriptional competency at the TMS1 locus and that this activity is mediated by the ets transcription factor, GABPalpha.

摘要

涉及启动子相关CpG岛异常DNA甲基化的表观遗传沉默是导致人类癌症中肿瘤抑制基因失活的一种机制。然而,这一事件背后的分子机制仍知之甚少。TMS1/ASC是一种新型促凋亡信号因子,在人类乳腺癌和其他癌症中会发生表观遗传沉默。TMS1启动子位于一个CpG岛内,该岛在正常细胞中未甲基化,并被三个DNase I超敏位点(HS)跨越。癌细胞中TMS1的沉默伴随着组蛋白修饰的局部改变、HS的重塑以及DNA的高甲基化。在本研究中,我们探究了CpG岛特异性HS的功能意义。我们鉴定出一种甲基化敏感复合物,它结合了一个对应于HS2的55 bp内含子元件。亲和层析和质谱分析确定该复合物的一个组分为GA结合蛋白(GABP)α。超迁移分析表明,GABPα的结合伴侣GABPβ1也存在于该复合物中。HS2元件使TMS1启动子活性增强了3倍,这依赖于完整的串联ets结合位点以及反式存在的GABPα/β1。GABPα在人类细胞的HS2处选择性富集,其占据情况与CpG岛甲基化呈负相关。GABPα的下调导致TMS1表达随之降低。这些数据表明内含子HS2元件顺式作用以维持TMS1基因座的转录能力,并且这种活性由ets转录因子GABPα介导。

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