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活细胞成像揭示了在细胞间期和有丝分裂过程中,Epstein-Barr 病毒核抗原 1 与细胞染色质之间的多种相互作用。

Live-cell imaging reveals multiple interactions between Epstein-Barr virus nuclear antigen 1 and cellular chromatin during interphase and mitosis.

机构信息

UPMC Université Paris 6, UMRS 872, Paris, France.

出版信息

J Virol. 2012 May;86(9):5314-29. doi: 10.1128/JVI.06303-11. Epub 2012 Feb 15.

Abstract

Epstein-Barr virus (EBV) establishes a life-long latent infection in humans. In proliferating latently infected cells, EBV genomes persist as multiple episomes that undergo one DNA replication event per cell cycle and remain attached to the mitotic chromosomes. EBV nuclear antigen 1 (EBNA-1) binding to the episome and cellular genome is essential to ensure proper episome replication and segregation. However, the nature and regulation of EBNA-1 interaction with chromatin has not been clearly elucidated. This activity has been suggested to involve EBNA-1 binding to DNA, duplex RNA, and/or proteins. EBNA-1 binding protein 2 (EBP2), a nucleolar protein, has been proposed to act as a docking protein for EBNA-1 on mitotic chromosomes. However, there is no direct evidence thus far for EBP2 being associated with EBNA-1 during mitosis. By combining video microscopy and Förster resonance energy transfer (FRET) microscopy, we demonstrate here for the first time that EBNA-1 and EBP2 interact in the nucleoplasm, as well as in the nucleoli during interphase. However, in strong contrast to the current proposed model, we were unable to observe any interaction between EBNA-1 and EBP2 on mitotic chromosomes. We also performed a yeast double-hybrid screening, followed by a FRET analysis, that led us to identify HMGB2 (high-mobility group box 2), a well-known chromatin component, as a new partner for EBNA-1 on chromatin during interphase and mitosis. Although the depletion of HMGB2 partly altered EBNA-1 association with chromatin in HeLa cells during interphase and mitosis, it did not significantly impact the maintenance of EBV episomes in Raji cells.

摘要

EB 病毒(EBV)在人类中建立终身潜伏感染。在增殖潜伏感染的细胞中,EBV 基因组作为多个附加体持续存在,每个细胞周期进行一次 DNA 复制,并附着在有丝分裂染色体上。EBV 核抗原 1(EBNA-1)与附加体和细胞基因组的结合对于确保适当的附加体复制和分离至关重要。然而,EBNA-1 与染色质相互作用的性质和调节尚未得到明确阐明。这种活性被认为涉及 EBNA-1 与 DNA、双链 RNA 和/或蛋白质的结合。核仁蛋白 EBNA-1 结合蛋白 2(EBP2)已被提议作为 EBNA-1 在有丝分裂染色体上的对接蛋白。然而,迄今为止,没有直接证据表明 EBP2 在有丝分裂期间与 EBNA-1 相关。通过结合视频显微镜和Förster 共振能量转移(FRET)显微镜,我们首次证明 EBNA-1 和 EBP2 在核质中以及在间期的核仁中相互作用。然而,与当前提出的模型形成强烈对比的是,我们无法观察到 EBNA-1 和 EBP2 在有丝分裂染色体上的任何相互作用。我们还进行了酵母双杂交筛选,随后进行了 FRET 分析,这使我们确定 HMGB2(高迁移率族盒 2)作为一种新的染色质成分,是间期和有丝分裂期间 EBNA-1 在染色质上的新伴侣。尽管 HMGB2 的耗尽部分改变了 HeLa 细胞间期和有丝分裂期间 EBNA-1 与染色质的关联,但它并没有显著影响 Raji 细胞中 EBV 附加体的维持。

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