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卡波西肉瘤相关疱疹病毒裂解开关蛋白RTA结合位点的全基因组鉴定

Genome-wide identification of binding sites for Kaposi's sarcoma-associated herpesvirus lytic switch protein, RTA.

作者信息

Chen Jiguo, Ye Fengchun, Xie Jianping, Kuhne Kurt, Gao Shou-Jiang

机构信息

Department of Pediatrics, Greehey Children's Cancer Research Institute, The University of Texas Health Science Center at San Antonio, 8403 Floyd Curl Drive, San Antonio, TX 78229, USA.

出版信息

Virology. 2009 Apr 10;386(2):290-302. doi: 10.1016/j.virol.2009.01.031. Epub 2009 Feb 23.

Abstract

Kaposi's sarcoma-associated herpesvirus (KSHV) replication and transcription activator (RTA) encoded by ORF50 is a lytic switch protein for viral reactivation from latency. The expression of RTA activates the expression of downstream viral genes, and is necessary for triggering the full viral lytic program. Using chromatin immunoprecipitation assay coupled with a KSHV whole-genome tiling microarray (ChIP-on-chip) approach, we identified a set of 19 RTA binding sites in the KSHV genome in a KSHV-infected cell line BCBL-1. These binding sites are located in the regions of promoters, introns, or exons of KSHV genes including ORF8, ORFK4.1, ORFK5, PAN, ORF16, ORF29, ORF45, ORF50, ORFK8, ORFK10.1, ORF59, ORFK12, ORF71/72, ORFK14/ORF74, and ORFK15, the two origins of lytic replication OriLyt-L and OriLyt-R, and the microRNA cluster. We confirmed these RTA binding sites by ChIP and quantitative real-time PCR. We further mapped the RTA binding site in the first intron of the ORFK15 gene, and determined that it is RTA-responsive. The ORFK15 RTA binding sequence TTCCAGGAA TTCCTGGAA consists of a palindromic structure of two tandem repeats, of which each itself is also an imperfect inverted repeat. Reporter assay and electrophoretic mobility shift assay confirmed the binding of the RTA protein to this sequence in vitro. Sequence alignment with other RTA binding sites identified the RTA consensus binding motif as TTCCAGGAT(N)(0-16)TTCCTGGGA. Interestingly, most of the identified RTA binding sites contain only half or part of this RTA binding motif. These results suggest the complexity of RTA binding in vivo, and the involvement of other cellular or viral transcription factors during RTA transactivation of target genes.

摘要

由ORF50编码的卡波西肉瘤相关疱疹病毒(KSHV)复制与转录激活因子(RTA)是一种使病毒从潜伏状态重新激活的裂解开关蛋白。RTA的表达激活下游病毒基因的表达,并且对于触发完整的病毒裂解程序是必需的。通过将染色质免疫沉淀分析与KSHV全基因组平铺微阵列(芯片上的染色质免疫沉淀)方法相结合,我们在KSHV感染的细胞系BCBL-1中鉴定出KSHV基因组中的一组19个RTA结合位点。这些结合位点位于KSHV基因的启动子、内含子或外显子区域,包括ORF8、ORFK4.1、ORFK5、PAN、ORF16、ORF29、ORF45、ORF50、ORFK8、ORFK10.1、ORF59、ORFK12、ORF71/72、ORFK14/ORF74和ORFK15,裂解复制的两个起始位点OriLyt-L和OriLyt-R,以及微小RNA簇。我们通过染色质免疫沉淀和定量实时PCR证实了这些RTA结合位点。我们进一步绘制了ORFK15基因第一个内含子中的RTA结合位点,并确定它对RTA有反应。ORFK15的RTA结合序列TTCCAGGAA TTCCTGGAA由两个串联重复序列的回文结构组成,其中每个自身也是一个不完全反向重复序列。报告基因检测和电泳迁移率变动分析证实了RTA蛋白在体外与该序列的结合。与其他RTA结合位点的序列比对确定RTA共有结合基序为TTCCAGGAT(N)(0 - 16)TTCCTGGGA。有趣的是,大多数鉴定出的RTA结合位点仅包含该RTA结合基序的一半或部分。这些结果表明RTA在体内结合的复杂性,以及在RTA对靶基因反式激活过程中其他细胞或病毒转录因子的参与。

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