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牛乳头瘤病毒1型E2反式激活蛋白和阻遏蛋白使用不同的核定位信号。

The bovine papillomavirus type 1 E2 transactivator and repressor proteins use different nuclear localization signals.

作者信息

Skiadopoulos M H, McBride A A

机构信息

Laboratory of Viral Diseases, National Institute of Allergy and Infectious Diseases, National Institutes of Health, Bethesda, MD 20892-0455, USA.

出版信息

J Virol. 1996 Feb;70(2):1117-24. doi: 10.1128/JVI.70.2.1117-1124.1996.

DOI:10.1128/JVI.70.2.1117-1124.1996
PMID:8551571
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC189919/
Abstract

The E2 gene of bovine papillomavirus type 1 encodes at least three nuclear phosphoproteins that regulate viral transcription and DNA replication. All three proteins have a common C-terminal domain that has DNA-binding and dimerization activities. A basic region in this domain forms an alpha helix which makes direct contact with the DNA target. In this study, it is shown that in addition to its role in DNA binding, this basic region functions as a nuclear localization signal both in the E2 DNA-binding domain and in a heterologous protein. Deletion of this signal sequence resulted in increased accumulation of the E2 transactivator and repressor proteins in the cytoplasm, but nuclear localization was not eliminated. In the full-length transactivator protein, another signal, present in the N-terminal transactivation domain, is used for transport to the nucleus, and the C-terminal nuclear localization signal(s) are masked. The use of different nuclear localization signals could potentially allow differential regulation of the subcellular localization of the E2 transactivator and repressor proteins at some stage in the viral life cycle.

摘要

1型牛乳头瘤病毒的E2基因编码至少三种调节病毒转录和DNA复制的核磷蛋白。这三种蛋白都有一个共同的C端结构域,该结构域具有DNA结合和二聚化活性。该结构域中的一个碱性区域形成一个α螺旋,可与DNA靶标直接接触。在本研究中,结果表明,除了其在DNA结合中的作用外,该碱性区域在E2 DNA结合结构域和异源蛋白中均作为核定位信号发挥作用。删除该信号序列导致E2反式激活蛋白和阻遏蛋白在细胞质中的积累增加,但核定位并未消除。在全长反式激活蛋白中,存在于N端反式激活结构域中的另一个信号用于转运至细胞核,而C端核定位信号被掩盖。在病毒生命周期的某个阶段,使用不同的核定位信号可能会对E2反式激活蛋白和阻遏蛋白的亚细胞定位进行差异调节。

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The acidic transcriptional activation domains of VP16 and p53 bind the cellular replication protein A and stimulate in vitro BPV-1 DNA replication.VP16和p53的酸性转录激活结构域与细胞复制蛋白A结合,并在体外刺激牛乳头瘤病毒1型(BPV-1)DNA复制。
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