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通过亲酸性试剂和共表达的M2蛋白拯救具有生物活性形式的载体表达的禽痘病毒血凝素

Rescue of vector-expressed fowl plague virus hemagglutinin in biologically active form by acidotropic agents and coexpressed M2 protein.

作者信息

Ohuchi M, Cramer A, Vey M, Ohuchi R, Garten W, Klenk H D

机构信息

Institut für Virologie, Philipps-Universität Marburg, Germany.

出版信息

J Virol. 1994 Feb;68(2):920-6. doi: 10.1128/JVI.68.2.920-926.1994.

DOI:10.1128/JVI.68.2.920-926.1994
PMID:8289394
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC236529/
Abstract

The hemagglutinin of the Rostock strain of fowl plague virus was expressed in CV-1 cells by a simian virus 40 vector, and its stability in the exocytotic transport process was examined by a fusion assay. A 50-fold increase in the fusion activity of the hemagglutinin was observed when expression occurred in the presence of ammonium chloride, Tris-HCl, or high doses of amantadine. When chloroquine, another acidotropic agent, was used, the hemagglutinin exposed at the cell surface had to be activated by trypsin, because intracellular cleavage was inhibited by this compound. Hemagglutinin mutants resistant to intracellular cleavage did not require acidotropic agents for full expression of fusion activity, when treated with trypsin after arrival at the cell surface. These results indicate that fowl plague virus hemagglutinin expressed by a simian virus 40 vector is denatured in the acidic milieu of the exocytotic pathway and that cleavage is a major factor responsible for the pH instability. Coexpression with the M2 protein also markedly enhanced the fusion activity of the hemagglutinin, and this effect was inhibited by low doses of amantadine. These results support the concept that M2, known to have ion channel function, protects the hemagglutinin from denaturation by raising the pH in the exocytotic transport system. The data also stress the importance of acidotropic agents or coexpressed M2 for the structural and functional integrity of vector-expressed hemagglutinin.

摘要

用猿猴病毒40载体在CV-1细胞中表达禽痘病毒罗斯托克株的血凝素,并通过融合试验检测其在胞吐转运过程中的稳定性。当在氯化铵、Tris-HCl或高剂量金刚烷胺存在的情况下进行表达时,观察到血凝素的融合活性增加了50倍。当使用另一种亲酸性试剂氯喹时,细胞表面暴露的血凝素必须用胰蛋白酶激活,因为这种化合物抑制了细胞内的裂解。对细胞内裂解具有抗性的血凝素突变体在到达细胞表面后用胰蛋白酶处理时,不需要亲酸性试剂来充分表达融合活性。这些结果表明,由猿猴病毒40载体表达的禽痘病毒血凝素在胞吐途径的酸性环境中发生变性,并且裂解是导致pH不稳定性的主要因素。与M2蛋白共表达也显著增强了血凝素的融合活性,并且这种作用被低剂量的金刚烷胺抑制。这些结果支持了以下概念,即已知具有离子通道功能的M2通过提高胞吐转运系统中的pH值来保护血凝素不发生变性。数据还强调了亲酸性试剂或共表达的M2对载体表达的血凝素的结构和功能完整性的重要性。

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