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鉴定和表征 CCAAT 增强子结合蛋白 (C/EBP) 作为 Epstein-Barr 病毒癌基因潜伏膜蛋白 1 的转录激活因子。

Identification and characterization of CCAAT enhancer-binding protein (C/EBP) as a transcriptional activator for Epstein-Barr virus oncogene latent membrane protein 1.

机构信息

Division of Virology, Aichi Cancer Center Research Institute, 1-1, Kanokoden, Chikusa-ku, Nagoya 464-8681; Department of Oncology, Graduate School of Pharmaceutical Sciences, Nagoya City University, Nagoya 467-8603.

Division of Virology, Aichi Cancer Center Research Institute, 1-1, Kanokoden, Chikusa-ku, Nagoya 464-8681.

出版信息

J Biol Chem. 2011 Dec 9;286(49):42524-42533. doi: 10.1074/jbc.M111.271734. Epub 2011 Oct 19.

Abstract

Epstein-Barr virus LMP1, a major oncoprotein expressed in latent infection, is critical for primary B cell transformation, functioning as a TNFR family member by aggregation in the plasma membrane resulting in constitutive activation of cellular signals, such as NF-κB, MAPK, JAK/STAT, and AKT. Although transcription of LMP1 in latent type III cells is generally under the control of the viral coactivator EBNA2, little is known about EBNA2-independent LMP1 expression in type II latency. We thus screened a cDNA library for factors that can activate the LMP1 promoter in an EBNA2-independent manner, using a reporter assay system. So far, we have screened >20,000 clones, and here identified C/EBPε as a new transcriptional activator. Exogenous expression of C/EBPα, -β, or -ε efficiently augmented LMP1 mRNA and protein levels in EBV-positive cell lines, whereas other members of the C/EBP family exhibited modest or little activity. It has been demonstrated that LMP1 gene transcription depends on two promoter regions: proximal (ED-L1) and distal (TR-L1). Interestingly, although we first used the proximal promoter for screening, we found that C/EBP increased transcription from both promoters in latent EBV-positive cells. Mutagenesis in reporter assays and EMSA identified only one functional C/EBP binding site, through which activation of both proximal and distal promoters is mediated. Introduction of point mutations into the identified C/EBP site in EBV-BAC caused reduced LMP1 transcription from both LMP1 promoters in epithelial cells. In conclusion, C/EBP is a newly identified transcriptional activator of the LMP1 gene, independent of the EBNA2 coactivator.

摘要

EB 病毒 LMP1,潜伏感染中表达的主要癌蛋白,对于原代 B 细胞转化至关重要,通过在质膜中聚集充当 TNFR 家族成员,导致细胞信号的组成性激活,如 NF-κB、MAPK、JAK/STAT 和 AKT。尽管潜伏型 III 细胞中的 LMP1 转录通常受病毒共激活因子 EBNA2 的控制,但对于 II 型潜伏状态下 EBNA2 独立的 LMP1 表达知之甚少。因此,我们使用报告基因检测系统筛选了一个 cDNA 文库,以寻找可在 EBNA2 非依赖性方式激活 LMP1 启动子的因子。迄今为止,我们已经筛选了 >20,000 个克隆,并在此鉴定了 C/EBPε 作为一种新的转录激活因子。外源性表达 C/EBPα、-β 或 -ε 可有效增强 EBV 阳性细胞系中的 LMP1 mRNA 和蛋白水平,而 C/EBP 家族的其他成员则表现出适度或微弱的活性。已经证明 LMP1 基因转录依赖于两个启动子区域:近端(ED-L1)和远端(TR-L1)。有趣的是,尽管我们最初使用近端启动子进行筛选,但我们发现 C/EBP 增加了潜伏性 EBV 阳性细胞中两个启动子的转录。报告基因检测和 EMSA 中的突变实验鉴定了一个功能 C/EBP 结合位点,通过该位点介导了两个近端和远端启动子的激活。在 EBV-BAC 中向鉴定出的 C/EBP 位点引入点突变会导致上皮细胞中两个 LMP1 启动子的 LMP1 转录减少。总之,C/EBP 是 LMP1 基因的一种新鉴定的转录激活因子,独立于 EBNA2 共激活因子。

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