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细胞因子YY1在体内和体外通过一个与转录起始位点重叠的负性元件下调人乳头瘤病毒16 E6/E7启动子P97。

Cellular factor YY1 downregulates the human papillomavirus 16 E6/E7 promoter, P97, in vivo and in vitro from a negative element overlapping the transcription-initiation site.

作者信息

Lace Michael J, Yamakawa Yasushi, Ushikai Masato, Anson James R, Haugen Thomas H, Turek Lubomir P

机构信息

Department of Pathology, University of Iowa Roy J. and Lucille A. Carver College of Medicine, Iowa City, IA 52242, USA.

Veterans Affairs Medical Center, 601 Highway 6 West, Iowa City, IA 52246, USA.

出版信息

J Gen Virol. 2009 Oct;90(Pt 10):2402-2412. doi: 10.1099/vir.0.012708-0. Epub 2009 Jun 24.

DOI:10.1099/vir.0.012708-0
PMID:19553391
Abstract

Cellular factors that bind to cis sequences in the human papillomavirus 16 (HPV-16) upstream regulatory region (URR) positively and negatively regulate the viral E6 and E7 oncogene promoter, P97. DNase I footprinting has revealed the binding of cellular proteins to two previously undetected cis elements overlapping and 3' of the transcription-initiation site of the P97 promoter. Mutations within homologous motifs found in both of these cis elements abolished their negative function in vivo and the binding of the same cellular complex in vitro. This factor was identified as YY1 by complex mobility and binding specificity in comparison with vaccinia virus-expressed, purified recombinant YY1 protein and by antigenic reactivity with YY1 antisera. Cis mutations in the 'initiator' YY1 site activated the P97 promoter in vivo and in vitro. P97 was also activated threefold in vitro by depletion of endogenous YY1 with wild-type, but not mutant, YY1 oligonucleotides from the IgH kappa E3' enhancer. Furthermore, increasing concentrations of exogenous, purified recombinant YY1 repressed wild-type P97 transcript levels by up to threefold, but did not influence the P97 promoter mutated in the 'initiator' YY1 site. Thus, the promoter-proximal YY1 site was not necessary for correct transcription initiation at the P97 promoter, but was found to be required for downregulation of P97 transcription in vivo and in vitro. In contrast to other viral and cellular promoters, where YY1 is thought to function as a positive transcription-'initiator' factor, HPV-16 P97 transcription is downregulated by YY1 from a critical motif overlapping the transcription start site.

摘要

与人类乳头瘤病毒16型(HPV - 16)上游调控区(URR)顺式序列结合的细胞因子可正向和负向调节病毒E6和E7癌基因启动子P97。DNA酶I足迹法揭示了细胞蛋白与两个先前未检测到的顺式元件的结合,这两个元件与P97启动子转录起始位点重叠且位于其3'端。在这两个顺式元件中发现的同源基序内的突变消除了它们在体内的负功能以及在体外与同一细胞复合物的结合。通过与痘苗病毒表达的纯化重组YY1蛋白比较复合物迁移率和结合特异性,以及与YY1抗血清的抗原反应性,该因子被鉴定为YY1。“起始子”YY1位点的顺式突变在体内和体外激活了P97启动子。用来自IgHκE3'增强子的野生型而非突变型YY1寡核苷酸耗尽内源性YY1后,P97在体外也被激活了三倍。此外,增加外源纯化重组YY1的浓度可使野生型P97转录水平下调多达三倍,但不影响在“起始子”YY1位点发生突变的P97启动子。因此,启动子近端的YY1位点对于P97启动子的正确转录起始不是必需的,但发现在体内和体外P97转录的下调中是必需的。与其他病毒和细胞启动子不同,在其他启动子中YY1被认为是一种正转录“起始子”因子,而HPV - 16 P97转录通过YY1从与转录起始位点重叠的关键基序下调。

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