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登革2型病毒非结构糖蛋白NS-1的功能和抗原结构域

Functional and antigenic domains of the dengue-2 virus nonstructural glycoprotein NS-1.

作者信息

Putnak J R, Charles P C, Padmanabhan R, Irie K, Hoke C H, Burke D S

机构信息

Department of Virus Diseases, Walter Reed Army Institute of Research, Washington D.C. 20307.

出版信息

Virology. 1988 Mar;163(1):93-103. doi: 10.1016/0042-6822(88)90236-x.

Abstract

The gene coding for the nonstructural glycoprotein of dengue-2 virus was cloned, sequenced, and expressed in Escherichia coli. There was about 70% conservation at the amino acid level with dengue serotypes 1 and 4 suggesting an important common function for this protein. Conserved hydrophobic domains were found both before the amino-terminus and at the carboxy-terminus, consistent with transmembrane roles. Evidence for at least partial translocation of NS-1 through the inner membrane of E. coli was found. Also conserved were two signals for N-linked glycosylation located near the middle of NS-1. Various regions of NS-1 were tested for antigenicity with mouse and rabbit polyclonal and mouse monoclonal antibodies. The mouse polyclonal antibodies, made against a crude dengue-infected mouse brain immunogen, reacted most strongly with N-terminal regions of NS-1, whereas, the rabbit antiserum, made against purified NS-1 protein, reacted strongest with C-terminal regions. These findings suggest that immunogen presentation or species differences could be important. Although most of the monoclonals appeared to be unreactive in Western blots with expressed NS-1 proteins, two appeared to react strongly; the region from amino acid (a.a.) 273 to a.a. 346 was required for antibody binding. This region, located adjacent to the two conserved C-terminal hydrophobic domains, is highly charged and contains 5 of the 10 conserved cysteine residues of NS-1.

摘要

登革2型病毒非结构糖蛋白的编码基因被克隆、测序,并在大肠杆菌中表达。该蛋白与登革1型和4型病毒在氨基酸水平上约有70%的保守性,表明其具有重要的共同功能。在氨基末端之前和羧基末端均发现了保守的疏水结构域,这与跨膜作用一致。发现了NS-1至少部分通过大肠杆菌内膜转运的证据。在NS-1中部附近还发现了两个N-连接糖基化信号。用小鼠和兔多克隆抗体以及小鼠单克隆抗体对NS-1的各个区域进行了抗原性检测。针对登革病毒感染的小鼠脑粗免疫原制备的小鼠多克隆抗体与NS-1的N端区域反应最强,而针对纯化的NS-1蛋白制备的兔抗血清与C端区域反应最强。这些发现表明免疫原呈递或物种差异可能很重要。尽管大多数单克隆抗体在蛋白质印迹中与表达的NS-1蛋白似乎无反应,但有两种单克隆抗体反应强烈;抗体结合需要氨基酸273至346区域。该区域位于两个保守的C端疏水结构域附近,电荷密度高,包含NS-1的10个保守半胱氨酸残基中的5个。

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