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RUNX3在人类L1转录和逆转录转座中的重要作用。

An important role for RUNX3 in human L1 transcription and retrotransposition.

作者信息

Yang Nuo, Zhang Lin, Zhang Yue, Kazazian Haig H

机构信息

Department of Genetics, University of Pennsylvania School of Medicine, Philadelphia, PA 19104, USA.

出版信息

Nucleic Acids Res. 2003 Aug 15;31(16):4929-40. doi: 10.1093/nar/gkg663.

Abstract

LINE-1s (long interspersed nuclear elements-1) are abundant non-LTR retrotransposons that comprise 17% of the human genome. The 5' untranslated region (5'UTR) of human L1 (L1Hs) houses a poorly understood internal promoter. Here we report that mutations at a putative runt-domain transcription factor (RUNX) site (+83 to +101) in the 5'UTR decreased L1Hs transcription and retrotransposition in cell culture-based assays. Exogenous expression of RUNX3, but not the other two RUNX family members, RUNX1 and RUNX2, increased L1Hs transcription and retrotransposition, which were otherwise decreased by siRNAs targeting RUNX3 and a dominant negative RUNX. Further more, the specific interaction between RUNX3 and its binding site was demonstrated by an electrophoretic mobility shift assay (EMSA) using an anti-RUNX3 antibody. Interestingly, RUNX3 may also regulate the antisense promoter activity of L1Hs 5'UTR via another putative RUNX site (+526 to +508), as revealed by site-directed mutations and exogenous expression of RUNX factors. Our results indicate an important role for RUNX3 in L1Hs retrotransposition as well as transcription from its 5'UTR in both sense and antisense directions, and they should contribute to our understanding of the mechanism underlying L1Hs retrotransposition and its impact on the expression of adjacent cellular genes.

摘要

LINE-1元件(长散在核元件-1)是丰富的非长末端重复逆转录转座子,占人类基因组的17%。人类L1(L1Hs)的5'非翻译区(5'UTR)含有一个了解甚少的内部启动子。在此我们报告,在细胞培养实验中,5'UTR中一个假定的 runt结构域转录因子(RUNX)位点(+83至+101)处的突变降低了L1Hs的转录和逆转座。RUNX3的外源性表达增加了L1Hs的转录和逆转座,而RUNX家族的其他两个成员RUNX1和RUNX2则没有这种作用,靶向RUNX3的小干扰RNA和显性负性RUNX会降低L1Hs的转录和逆转座。此外,使用抗RUNX3抗体的电泳迁移率变动分析(EMSA)证明了RUNX3与其结合位点之间的特异性相互作用。有趣的是,定点突变和RUNX因子的外源性表达表明,RUNX3可能还通过另一个假定的RUNX位点(+526至+508)调节L1Hs 5'UTR的反义启动子活性。我们的结果表明RUNX3在L1Hs逆转座以及其5'UTR正反义方向的转录中起重要作用,这将有助于我们理解L1Hs逆转座的机制及其对相邻细胞基因表达的影响。

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