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转录抑制因子K-RBP调节卡波西肉瘤相关疱疹病毒的RTA介导的反式激活和裂解复制。

The transcriptional repressor K-RBP modulates RTA-mediated transactivation and lytic replication of Kaposi's sarcoma-associated herpesvirus.

作者信息

Yang Zhilong, Wood Charles

机构信息

Nebraska Center for Virology and School of Biological Sciences, University of Nebraska, E249 Beadle Center, P.O. Box 880666, Lincoln, NE 68588-0666, USA.

出版信息

J Virol. 2007 Jun;81(12):6294-306. doi: 10.1128/JVI.02648-06. Epub 2007 Apr 4.

DOI:10.1128/JVI.02648-06
PMID:17409159
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1900108/
Abstract

The replication and transcription activator (RTA) protein of Kaposi's sarcoma (KS)-associated herpesvirus (KSHV)/human herpesvirus 8 functions as the key regulator to induce KSHV lytic replication from latency through activation of the lytic cascade of KSHV. Elucidation of the host factors involved in RTA-mediated transcriptional activation is pivotal for understanding the transition between viral latency and lytic replication. KSHV-RTA binding protein (K-RBP) was previously isolated as a cellular RTA binding protein of unknown function. Sequence analysis showed that K-RBP contains a Kruppel-associated box (KRAB) at the N terminus and 12 adjacent zinc finger motifs. In similarity to other KRAB-containing zinc finger proteins, K-RBP is a transcriptional repressor. Mutational analysis revealed that the KRAB domain is responsible for the transcriptional suppression activity of this protein and that the repression is histone deacetylase independent. K-RBP was found to repress RTA-mediated transactivation and interact with TIF1beta (transcription intermediary factor 1beta), a common corepressor of KRAB-containing protein, to synergize with K-RBP in repression. Overexpression and knockdown experiment results suggest that K-RBP is a suppressor of RTA-mediated KSHV reactivation. Our findings suggest that the KRAB-containing zinc finger protein K-RBP can suppress RTA-mediated transactivation and KSHV lytic replication and that KSHV utilizes this protein as a regulator to maintain a balance between latency and lytic replication.

摘要

卡波西肉瘤(KS)相关疱疹病毒(KSHV)/人类疱疹病毒8的复制和转录激活因子(RTA)蛋白,作为关键调节因子,通过激活KSHV的裂解级联反应,诱导KSHV从潜伏期进入裂解复制。阐明参与RTA介导的转录激活的宿主因子,对于理解病毒潜伏期和裂解复制之间的转变至关重要。KSHV-RTA结合蛋白(K-RBP)先前被分离为一种功能未知的细胞RTA结合蛋白。序列分析表明,K-RBP在N端含有一个Kruppel相关框(KRAB)和12个相邻的锌指基序。与其他含KRAB的锌指蛋白相似,K-RBP是一种转录抑制因子。突变分析表明,KRAB结构域负责该蛋白的转录抑制活性,且这种抑制不依赖组蛋白去乙酰化酶。发现K-RBP可抑制RTA介导的反式激活,并与TIF1β(转录中介因子1β,一种含KRAB蛋白的常见共抑制因子)相互作用,在抑制作用中与K-RBP协同作用。过表达和敲低实验结果表明,K-RBP是RTA介导的KSHV激活的抑制因子。我们的研究结果表明,含KRAB的锌指蛋白K-RBP可抑制RTA介导的反式激活和KSHV裂解复制,且KSHV利用该蛋白作为调节因子,以维持潜伏期和裂解复制之间的平衡。

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Transcripts encoding K12, v-FLIP, v-cyclin, and the microRNA cluster of Kaposi's sarcoma-associated herpesvirus originate from a common promoter.编码卡波西肉瘤相关疱疹病毒的K12、v-FLIP、v-细胞周期蛋白和微小RNA簇的转录本源自一个共同的启动子。
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The Krüppel-like zinc-finger protein ZNF224 represses aldolase A gene transcription by interacting with the KAP-1 co-repressor protein.类Krüppel锌指蛋白ZNF224通过与共抑制蛋白KAP-1相互作用来抑制醛缩酶A基因的转录。
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Induction of Kaposi's sarcoma-associated herpesvirus latency-associated nuclear antigen by the lytic transactivator RTA: a novel mechanism for establishment of latency.由裂解性反式激活因子RTA诱导卡波西肉瘤相关疱疹病毒潜伏相关核抗原:一种建立潜伏状态的新机制。
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The KSHV immediate-early transcription factor RTA encodes ubiquitin E3 ligase activity that targets IRF7 for proteosome-mediated degradation.卡波西肉瘤相关疱疹病毒(KSHV)即刻早期转录因子RTA编码泛素E3连接酶活性,该活性以干扰素调节因子7(IRF7)为靶点,使其通过蛋白酶体介导的途径降解。
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