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博尔纳病病毒聚合酶核定位信号的表征

Characterization of the nuclear localization signal of the borna disease virus polymerase.

作者信息

Walker Michelle Portlance, Lipkin W Ian

机构信息

Emerging Diseases Laboratory, Department of Neurology, University of California-Irvine, 92697-4292, USA.

出版信息

J Virol. 2002 Aug;76(16):8460-7. doi: 10.1128/jvi.76.16.8460-8467.2002.

Abstract

Borna disease virus (BDV) is a nonsegmented negative-strand RNA virus that replicates and transcribes its genome in the nucleus of infected cells. BDV proteins involved in replication and transcription must pass through the nuclear envelope to associate with the genomic viral RNA. The RNA-dependent RNA polymerase (L) of BDV is postulated to be the catalytic enzyme of replication and transcription. We demonstrated previously that BDV L localizes to the nucleus of BDV-infected cells and L-transfected cells. Nuclear localization of the protein presupposes the presence of a nuclear localization signal (NLS) within its primary amino acid sequence or cotransport to the nucleus with another karyophilic protein. Because L localized to the nucleus in the absence of other viral proteins, we investigated the possibility that L contains an NLS. The minimal sequence required for nuclear localization of L was identified by analyzing the subcellular distribution of deletion mutants of L fused to a flag epitope tag or beta-galactosidase. Although the majority of the L fusion proteins localized to the cytoplasm of transfected BSR-T7 cells, a strong NLS (844RVVKLRIAP852) with basic and proline residues was identified. Mutation of this sequence resulted in cytoplasmic distribution of L, confirming that this sequence was necessary and sufficient to drive the nuclear localization of L.

摘要

博尔纳病病毒(BDV)是一种不分节段的负链RNA病毒,在受感染细胞的细胞核中复制并转录其基因组。参与复制和转录的BDV蛋白必须穿过核膜才能与基因组病毒RNA结合。BDV的RNA依赖性RNA聚合酶(L)被认为是复制和转录的催化酶。我们之前证明了BDV L定位于BDV感染细胞和L转染细胞的细胞核中。该蛋白的核定位以其一级氨基酸序列中存在核定位信号(NLS)或与另一种亲核蛋白共转运至细胞核为前提。由于在没有其他病毒蛋白的情况下L定位于细胞核,我们研究了L含有NLS的可能性。通过分析与flag表位标签或β-半乳糖苷酶融合的L缺失突变体的亚细胞分布,确定了L核定位所需的最小序列。尽管大多数L融合蛋白定位于转染的BSR-T7细胞的细胞质中,但鉴定出了一个具有碱性和脯氨酸残基的强NLS(844RVVKLRIAP852)。该序列的突变导致L在细胞质中分布,证实该序列对于驱动L的核定位是必要且充分的。

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