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YY1通过抑制AP-1活性来抑制16型人乳头瘤病毒的转录。

YY1 represses human papillomavirus type 16 transcription by quenching AP-1 activity.

作者信息

O'Connor M J, Tan S H, Tan C H, Bernard H U

机构信息

Laboratory for Papillomavirus Biology, Institute of Molecular and Cell Biology, National University of Singapore.

出版信息

J Virol. 1996 Oct;70(10):6529-39. doi: 10.1128/JVI.70.10.6529-6539.1996.

Abstract

YY1 is a multifunctional transcription factor that has been shown to regulate the expression of a number of cellular and viral genes, including the human papillomavirus (HPV) oncogenes E6 and E7. In this study, we have analyzed the YY1-mediated repression of the HPV type 16 (HPV-16) E6-E7 promoter. A systematic analysis to identify YY1 sites present in the HPV-16 long control region showed that of 30 potential YY1 binding motifs, 24 bound purified recombinant YY1 protein, but only 10 of these were able to bind YY1 when nuclear extracts of HeLa cells were used. Of these, only a cluster of five sites, located in the vicinity of an AP-1 motif, were found to be responsible for repressing the HPV-16 P97 promoter. All five sites were required for repression, the mutation of any one site giving rise to a four- to sixfold increase in transcriptional activity. The target for YY1-mediated repression was identified as being a highly conserved AP-1 site, and we propose that AP-1 may represent a common target for YY1 repression. We also provide data demonstrating that YY1 can bind the transcriptional coactivator CREB-binding protein and propose a potentially novel mechanism by which YY1 represses AP-1 activity as a result of this YY1-CREB-binding protein interaction.

摘要

YY1是一种多功能转录因子,已被证明可调节许多细胞和病毒基因的表达,包括人乳头瘤病毒(HPV)癌基因E6和E7。在本研究中,我们分析了YY1介导的对16型HPV(HPV - 16)E6 - E7启动子的抑制作用。一项旨在鉴定HPV - 16长控制区中存在的YY1位点的系统分析表明,在30个潜在的YY1结合基序中,有24个能结合纯化的重组YY1蛋白,但当使用HeLa细胞核提取物时,其中只有10个能结合YY1。在这些位点中,仅发现位于AP - 1基序附近的一组五个位点负责抑制HPV - 16 P97启动子。所有这五个位点对于抑制都是必需的,任何一个位点的突变都会导致转录活性增加4至6倍。YY1介导的抑制作用的靶点被确定为一个高度保守的AP - 1位点,并且我们提出AP - 1可能代表YY1抑制作用的一个共同靶点。我们还提供数据证明YY1可以结合转录共激活因子CREB结合蛋白,并提出一种潜在的新机制,即由于这种YY1 - CREB结合蛋白的相互作用,YY1抑制AP - 1活性。

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