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ATF/CREB位点是人类RNA甲基转移酶样1(RNMTL1)基因转录的关键元件,RNMTL1是一个新发现的位于17p13.3的基因。

The ATF/CREB site is the key element for transcription of the human RNA methyltransferase like 1(RNMTL1) gene, a newly discovered 17p13.3 gene.

作者信息

Xu Jian, De Zhu Jing, Ni Min, Wan Fang, Gu Jian Ren

机构信息

The State-key Laboratory for Oncogenes and Related Genes, Shanghai Cancer Institute, Xie-tu China.

出版信息

Cell Res. 2002 Sep;12(3-4):177-97. doi: 10.1038/sj.cr.7290124.

DOI:10.1038/sj.cr.7290124
PMID:12296377
Abstract

The human RNA methyltransferase like 1 gene (RNMTL1) is one of thirteen newly discovered genes within a 116 Kb segment of the chromosome 17p13.3 that suffers from a high frequent loss of heterozygosity in human hepatocellular carcinoma in China[1-5]. To understand the molecular mechanisms underlying transcription control of the RNMTL1 gene in human cancers, we decline using of the conventional approach where the cis-elements bound by the known transcription factors are primary targets, and carried out the systematic analyses to dissect the promoter structure and identify/characterize the key cis-elements that are responsible for its strong expression in cell. The molecular approaches applied included 1, the primer extension for mapping of the transcription starts; 2, the transient transfection/reporter assays on a large number of deletion and site-specific mutants of the promoter segment for defining the minimal promoter and the crucial elements within; and 3, the electrophoresis mobility shift assay with specific antibodies for reconfirming the nature of the transcription factors and their cognate cis-elements. We have shown that the interaction of an ATF/CREB element (-38 to -31) and its cognate transcription factors play a predominant role in the promoter activity of the RNMTL1 gene. The secondary DNA structures of the ATF/CREB element play a more vital role in the protein-DNA interaction. Finally, we reported a novel mechanism underlying the YY1 mediated transcription repression, namely, the ATF/CREB dependent transcription-repression by YY1 is executed in absence of its own sequence-specific binding.

摘要

人类RNA甲基转移酶样1基因(RNMTL1)是17号染色体p13.3区域116 Kb片段内新发现的13个基因之一,在中国的人类肝细胞癌中该区域存在高频杂合性缺失[1-5]。为了了解人类癌症中RNMTL1基因转录调控的分子机制,我们摒弃了传统方法(即以已知转录因子结合的顺式元件为主要靶点),并进行了系统分析以剖析启动子结构,鉴定/表征负责其在细胞中强表达的关键顺式元件。所应用的分子方法包括:1. 用于转录起始位点定位的引物延伸;2. 对启动子片段的大量缺失和位点特异性突变体进行瞬时转染/报告基因分析,以确定最小启动子及其内的关键元件;3. 用特异性抗体进行电泳迁移率变动分析,以再次确认转录因子及其同源顺式元件的性质。我们已经表明,ATF/CREB元件(-38至-31)及其同源转录因子的相互作用在RNMTL1基因的启动子活性中起主要作用。ATF/CREB元件的二级DNA结构在蛋白质-DNA相互作用中发挥更重要的作用。最后,我们报道了一种YY1介导的转录抑制的新机制,即YY1在没有其自身序列特异性结合的情况下执行ATF/CREB依赖性转录抑制。

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Cell Res. 2002 Sep;12(3-4):177-97. doi: 10.1038/sj.cr.7290124.
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