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油橄榄潜隐病毒2假定运动蛋白的亚细胞定位及体内鉴定

Subcellular localization and in vivo identification of the putative movement protein of olive latent virus 2.

作者信息

Grieco F, Castellano M A, Di Sansebastiano G P, Maggipinto G, Neuhaus J M, Martelli G P

出版信息

J Gen Virol. 1999 May;80 ( Pt 5):1103-1109. doi: 10.1099/0022-1317-80-5-1103.

DOI:10.1099/0022-1317-80-5-1103
PMID:10355755
Abstract

The gene encoding the 36.5 kDa ('36K') nonstructural protein located on RNA3 of olive latent virus 2 (OLV-2) was cloned, expressed with the Escherichia coli pGEX-2T system and the purified protein used to raise a polyclonal antiserum. Immunoblot analysis of OLV-2-infected Nicotiana benthamiana plants showed that the 36K protein accumulated in the early stages of infection and was associated with a subcellular fraction enriched in cytoplasmic membranes. In infected cells there were tubular structures, some containing virus-like particles, scattered in the cytoplasm or protruding from or penetrating the cell wall at the plasmodesmata. Immunogold labelling localized the 36K protein in the plasmodesmata of OLV-2-infected cells and showed it to be associated with virus-containing tubules. Leaf trichome cells of N. tabacum plants, transformed with a 36K-green fluorescent protein (GFP) fusion construct, revealed localized fluorescence in the cell walls, possibly due to association of the fusion protein with plasmodesmata. When the same 36K-GFP fusion protein was expressed in N. tabacum protoplasts, long tubular fluorescent structures protruded from the protoplast surface, suggesting that the 36K protein is responsible for tubule induction. The conclusion is drawn that this protein is likely to be the OLV-2 movement protein, mediating cell-to-cell virus movement, and that movement is by a tubule-guided mechanism.

摘要

克隆了位于油橄榄潜隐病毒2(OLV-2)RNA3上编码36.5 kDa(“36K”)非结构蛋白的基因,利用大肠杆菌pGEX-2T系统进行表达,并使用纯化后的蛋白制备多克隆抗血清。对感染OLV-2的本氏烟草植株进行免疫印迹分析表明,36K蛋白在感染早期积累,并与富含细胞质膜的亚细胞组分相关。在受感染的细胞中,存在一些管状结构,其中一些含有病毒样颗粒,散布在细胞质中,或在胞间连丝处从细胞壁突出或穿透细胞壁。免疫金标记将36K蛋白定位在感染OLV-2细胞的胞间连丝中,并表明它与含病毒的小管相关。用36K-绿色荧光蛋白(GFP)融合构建体转化的烟草植株的叶毛细胞,在细胞壁中显示出局部荧光,这可能是由于融合蛋白与胞间连丝相关。当相同的36K-GFP融合蛋白在烟草原生质体中表达时,长管状荧光结构从原生质体表面突出,表明36K蛋白负责小管诱导。得出的结论是,该蛋白可能是OLV-2运动蛋白,介导病毒在细胞间的移动,并且移动是通过小管引导机制进行的。

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