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菊花病毒B p12蛋白的锌指和碱性基序在核酸结合、蛋白定位以及从病毒载体表达时诱导过敏反应中的作用

Role of the zinc-finger and basic motifs of chrysanthemum virus B p12 protein in nucleic acid binding, protein localization and induction of a hypersensitive response upon expression from a viral vector.

作者信息

Lukhovitskaya N I, Ignatovich I V, Savenkov E I, Schiemann J, Morozov S Yu, Solovyev A G

机构信息

Department of Plant Biology and Forest Genetics, Swedish University of Agricultural Sciences (SLU), Box 7080, SE-750 07 Uppsala, Sweden.

A. N. Belozersky Institute of Physico-Chemical Biology, Moscow State University, 119992 Moscow, Russia.

出版信息

J Gen Virol. 2009 Mar;90(Pt 3):723-733. doi: 10.1099/vir.0.005025-0.

DOI:10.1099/vir.0.005025-0
PMID:19218219
Abstract

The genomes of carlaviruses encode cysteine-rich proteins (CRPs) of unknown function. The 12 kDa CRP of chrysanthemum virus B (CVB), p12, has been shown previously to induce a hypersensitive response (HR) when expressed from potato virus X (PVX). This study demonstrated that a p12-induced HR was preceded by induction of a number of genes related to pathogenesis, stress and systemic acquired resistance. p12 localized predominantly to the nucleus. Interestingly, it was found that p12 bound both RNA and DNA in vitro, but notably exhibited a preference for DNA in the presence of Zn(2+) ions. Mutational analysis of the p12 conserved sequence motifs demonstrated that the basic motif is required for p12 translocation to the nucleus, thus representing part of the protein nuclear localization signal, whereas the predicted zinc finger motif is needed for both Zn(2+)-dependent DNA binding and eliciting an HR in PVX-infected leaves. Collectively, these results link, for the first time, nuclear localization of the protein encoded by a cytoplasmically replicating virus and its DNA-binding capacity with HR induction. Furthermore, these data suggest that p12 may mediate induction of the host genes by binding to the plant genomic DNA, and emphasize that CVB p12 is functionally distinct from other known nuclear-localized proteins encoded by the plant positive-stranded RNA viruses.

摘要

香石竹潜隐病毒属病毒的基因组编码功能未知的富含半胱氨酸的蛋白(CRP)。菊花B病毒(CVB)的12 kDa CRP,即p12,先前已证明当从马铃薯X病毒(PVX)表达时会诱导超敏反应(HR)。本研究表明,p12诱导的HR之前会诱导许多与发病机制、胁迫和系统获得性抗性相关的基因。p12主要定位于细胞核。有趣的是,发现p12在体外能结合RNA和DNA,但在Zn(2+)离子存在时明显表现出对DNA的偏好。对p12保守序列基序的突变分析表明,基本基序是p12转运至细胞核所必需的,因此代表了蛋白质核定位信号的一部分,而预测的锌指基序对于Zn(2+)依赖的DNA结合以及在PVX感染叶片中引发HR都是必需的。总的来说,这些结果首次将细胞质复制病毒编码的蛋白质的核定位及其DNA结合能力与HR诱导联系起来。此外,这些数据表明p12可能通过与植物基因组DNA结合来介导宿主基因的诱导,并强调CVB p12在功能上与植物正链RNA病毒编码的其他已知核定位蛋白不同。

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