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传染性胰腺坏死病毒:含VP3的核糖核蛋白核心结构的鉴定及衣壳蛋白VP2 O-连接糖基化的证据

Infectious pancreatic necrosis virus: identification of a VP3-containing ribonucleoprotein core structure and evidence for O-linked glycosylation of the capsid protein VP2.

作者信息

Hjalmarsson A, Carlemalm E, Everitt E

机构信息

Department of Microbiology, Lund University, Lund, Sweden.

出版信息

J Virol. 1999 Apr;73(4):3484-90. doi: 10.1128/JVI.73.4.3484-3490.1999.

Abstract

Virions of infectious pancreatic necrosis virus (IPNV) were completely disintegrated upon dialysis against salt-free buffers. Direct visualization of such preparations by electron microscopy revealed 5.0- to 6.5-nm-thick entangled filaments. By using a specific colloidal gold immunolabeling technique, these structures were shown to contain the viral protein VP3. Isolation by sucrose gradient centrifugation of the filaments, followed by serological analysis, demonstrated that the entire VP3 content of the virion was recovered together with the radiolabeled genomic material forming the unique threadlike ribonucleoprotein complexes. In a sensitive blotting assay, the outer capsid component of IPNV, i.e., the major structural protein VP2, was shown to specifically bind lectins recognizing sugar moieties of N-acetylgalactosamine, mannose, and fucose. Three established metabolic inhibitors of N-linked glycosylation did not prevent addition of sugar residues to virions, and enzymatic deglycosylation of isolated virions using N-glycosidase failed to remove sugar residues of VP2 recognized by lectins. However, gentle alkaline beta elimination clearly reduced the ability of lectins to recognize VP2. These results suggest that the glycosylation of VP2 is of the O-linked type when IPNV is propagated in RTG-2 cells.

摘要

传染性胰腺坏死病毒(IPNV)的病毒粒子在与无盐缓冲液透析时会完全解体。通过电子显微镜直接观察此类制剂,发现有5.0至6.5纳米厚的缠结细丝。通过使用特定的胶体金免疫标记技术,这些结构被证明含有病毒蛋白VP3。通过蔗糖梯度离心分离细丝,随后进行血清学分析,结果表明病毒粒子的整个VP3含量与形成独特丝状核糖核蛋白复合物的放射性标记基因组物质一起被回收。在一项灵敏的印迹分析中,IPNV的外衣壳成分,即主要结构蛋白VP2,被证明能特异性结合识别N-乙酰半乳糖胺、甘露糖和岩藻糖糖基部分的凝集素。三种已确定的N-连接糖基化代谢抑制剂并不能阻止糖残基添加到病毒粒子上,并且使用N-糖苷酶对分离出的病毒粒子进行酶促去糖基化未能去除凝集素识别的VP2糖残基。然而,温和的碱性β消除明显降低了凝集素识别VP2的能力。这些结果表明,当IPNV在RTG-2细胞中繁殖时,VP2的糖基化是O-连接型。

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