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具有诱变羧基末端疏水结构域的人巨细胞病毒糖蛋白B(gpUL55)的组成型表达

Constitutive expression of human cytomegalovirus glycoprotein B (gpUL55) with mutagenized carboxy-terminal hydrophobic domains.

作者信息

Reschke M, Reis B, Nöding K, Rohsiepe D, Richter A, Mockenhaupt T, Garten W, Radsak K

机构信息

Institut für Virologie, Philipps-Universität, Marburg, Germany.

出版信息

J Gen Virol. 1995 Jan;76 ( Pt 1):113-22. doi: 10.1099/0022-1317-76-1-113.

DOI:10.1099/0022-1317-76-1-113
PMID:7844520
Abstract

Stable transfectants were selected from human astrocytoma cells (U373) after transfection with recombinant expression vectors carrying the human cytomegalovirus (HCMV) glycoprotein B (gB; gpUL55) gene with alternative deletions of hydrophobic domain segment 1 (hd1) or segment 2 (hd2) of the carboxy-terminal potential bipartite membrane anchor domain. Comparative analysis of HCMV gB forms from cell lines gB(Mhd1) and gB(Mhd2), expressing mutagenized gB, and those from cells expressing authentic gB showed that deletion of hd1, but not that of hd2, interfered with efficient proteolytic cleavage of the gB precursor. Both mutagenized gB forms exhibited correct transport to the cell surface. Deletion of hd2, but not that of hd1, caused loss of membrane anchoring of the gB molecule, resulting in secretion of the respective gB form into the culture medium. The carboxy-terminal cleavage product of the soluble gB molecule, which migrated more slowly than its authentic counterpart, was modified by complex carbohydrate side chains and formed disulphide-linked complexes. Our observations indicate that hd2 is essential as well as sufficient for membrane anchoring of the HCMV gB molecule. For hd1, a potential fusogenic role is suggested by the conserved positional pattern of glycine residues, which is comparable to that of known fusion peptides of other viruses.

摘要

用携带人巨细胞病毒(HCMV)糖蛋白B(gB;gpUL55)基因的重组表达载体转染人星形细胞瘤细胞(U373)后,筛选出稳定转染子,该基因在羧基末端潜在的双部分膜锚定结构域的疏水结构域片段1(hd1)或片段2(hd2)处有选择性缺失。对表达诱变gB的细胞系gB(Mhd1)和gB(Mhd2)以及表达天然gB的细胞中HCMV gB形式的比较分析表明,hd1的缺失而非hd2的缺失会干扰gB前体的有效蛋白水解切割。两种诱变的gB形式均表现出正确转运至细胞表面。hd2的缺失而非hd1的缺失导致gB分子的膜锚定丧失,从而使相应的gB形式分泌到培养基中。可溶性gB分子的羧基末端切割产物迁移速度比其天然对应物慢,被复杂碳水化合物侧链修饰并形成二硫键连接的复合物。我们的观察结果表明,hd2对于HCMV gB分子的膜锚定至关重要且足够。对于hd1,甘氨酸残基的保守位置模式提示其具有潜在的融合作用,这与其他病毒已知的融合肽相似。

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