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人类疱疹病毒7型U27基因产物的特性及其核定位信号的鉴定

Characterization of human herpesvirus 7 U27 gene product and identification of its nuclear localization signal.

作者信息

Takeda K, Haque M, Nagoshi E, Takemoto M, Shimamoto T, Yoneda Y, Yamanishi K

机构信息

Department of Microbiology, Department of Anatomy and Cell Biology, Osaka University Medical School, 2-2 Yamada-oka, Osaka, Suita, 565-0871, Japan.

出版信息

Virology. 2000 Jul 5;272(2):394-401. doi: 10.1006/viro.2000.0364.

DOI:10.1006/viro.2000.0364
PMID:10873783
Abstract

A monoclonal antibody, 5H4, that recognizes human herpesvirus 7 (HHV-7) was used in Western analysis to probe HHV-7-infected SupT1 cells. This antibody recognizes a 40-kDa virus-specific polypeptide that is expressed in the absence of viral DNA synthesis. By screening a lambdagt11 HHV-7 cDNA library, the gene encoding the protein was identified as the U27 open reading frame previously reported [J. Virol. (1996) 70, 5975-5989]. Immunofluorescent studies showed a punctate nuclear localization of the protein in both HHV-7-infected cells and transfected cells. A computer program predicted two classic nuclear localization signals (NLSs) in the middle and C-terminal regions of the protein. A C-terminal deletion mutant of the protein could not enter the nucleus, whereas green fluorescent protein or maltose binding protein fused to the C-terminal region of the protein was transported into the nucleus. These findings demonstrate that the predicted C-terminal, but not middle, NLS of the protein actually function as NLS. In addition, nuclear transport of a maltose binding protein-fusion protein containing the C-terminal NLS of the U27 protein was inhibited by both wheat germ agglutinin and a Q69L Ran-GTP mutant, indicating that the U27 protein is transported into the nucleus from the cytoplasm by means of classic nuclear transport machinery. Interestingly, this NLS motif is highly conserved at the C-termini of all herpesvirus DNA polymerase processivity factors that have been examined.

摘要

一种识别人类疱疹病毒7型(HHV - 7)的单克隆抗体5H4被用于蛋白质免疫印迹分析,以检测HHV - 7感染的SupT1细胞。该抗体识别一种40 kDa的病毒特异性多肽,这种多肽在没有病毒DNA合成的情况下表达。通过筛选λgt11 HHV - 7 cDNA文库,编码该蛋白的基因被鉴定为先前报道的U27开放阅读框[《病毒学杂志》(1996年)70卷,5975 - 5989页]。免疫荧光研究显示,在HHV - 7感染的细胞和转染细胞中,该蛋白呈点状核定位。一个计算机程序预测该蛋白的中部和C端区域有两个典型的核定位信号(NLSs)。该蛋白的C端缺失突变体无法进入细胞核,而与该蛋白C端区域融合的绿色荧光蛋白或麦芽糖结合蛋白则被转运到细胞核中。这些发现表明,预测的该蛋白C端而非中部的NLS实际上作为NLS发挥作用。此外,含有U27蛋白C端NLS的麦芽糖结合蛋白融合蛋白的核转运受到麦胚凝集素和Q69L Ran - GTP突变体的抑制,这表明U27蛋白通过经典的核转运机制从细胞质转运到细胞核中。有趣的是,在所有已检测的疱疹病毒DNA聚合酶持续合成因子的C端,这种NLS基序高度保守。

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