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一类被命名为gC-I(gB)的人巨细胞病毒糖蛋白复合物的结构与组成

Structure and composition of a family of human cytomegalovirus glycoprotein complexes designated gC-I (gB).

作者信息

Kari B, Liu Y N, Goertz R, Lussenhop N, Stinski M F, Gehrz R

机构信息

Biochemistry Division, Children's Hospital, St Paul, Minnesota 55102.

出版信息

J Gen Virol. 1990 Nov;71 ( Pt 11):2673-80. doi: 10.1099/0022-1317-71-11-2673.

DOI:10.1099/0022-1317-71-11-2673
PMID:1701480
Abstract

Murine monoclonal antibodies (MAbs) were made to the 52,000 (gp52) and the 93,000 to 130,000 Mr (gp93-130) glycoproteins from a human cytomegalovirus (HCMV) glycoprotein complex designated gC-I or the gB homologue. MAbs recognizing either gp52 or gp93-130 could immunoprecipitate unreduced gC-I complexes from non-ionic detergent extracts of HCMV. Western blotting was performed with immunoaffinity-purified gC-I complexes which were reduced prior to analysis. MAbs made against gp52 recognized gp52 and a 158,000 Mr glycoprotein (gp158). MAbs which recognized gp93-130 in a Western blot also reacted with gp158, which is a gC-I precursor glycoprotein. The origin of gp93-130 was demonstrated by the reactivity of our gp93-130 MAbs with a recombinant protein containing the N-terminal portion of the gB gene. These data are consistent with the hypothesis that gp52 and gp93-130 are generated from the same high Mr precursor by proteolysis. MAbs recognizing either gp52 or gp93-130 neutralized Towne strain HCMV, but MAbs recognizing gp52 required complement to neutralize whereas MAbs recognizing gp93-130 did not. It was also determined that gp93-130 and gp 158 have detectable amounts of O-linked glycans but gp52 does not, showing a difference in the glycosylation of these glycoproteins. Analysis of gC-I disulphide bonds showed that two types were present, one which was very susceptible to reduction and a second which was less susceptible. These complexes could consist of very susceptible inter-complex disulphide bonds and less susceptible intra-complex disulphide bonds.

摘要

针对人巨细胞病毒(HCMV)糖蛋白复合物gC-I或gB同系物中52,000(gp52)以及93,000至130,000分子量(gp93 - 130)的糖蛋白制备了鼠单克隆抗体(MAbs)。识别gp52或gp93 - 130的单克隆抗体能够从HCMV的非离子去污剂提取物中免疫沉淀未还原的gC-I复合物。对免疫亲和纯化的gC-I复合物进行蛋白质印迹分析,该复合物在分析前先进行还原处理。针对gp52制备的单克隆抗体识别gp52和一种158,000分子量的糖蛋白(gp158)。在蛋白质印迹中识别gp93 - 130的单克隆抗体也与gp158发生反应,gp158是一种gC-I前体糖蛋白。我们针对gp93 - 130的单克隆抗体与包含gB基因N端部分的重组蛋白发生反应,从而证明了gp93 - 130的来源。这些数据与gp52和gp93 - 130是由同一高分子量前体经蛋白水解产生的假说一致。识别gp52或gp93 - 130的单克隆抗体能够中和Towne株HCMV,但识别gp52的单克隆抗体需要补体才能中和,而识别gp93 - 130的单克隆抗体则不需要。还确定gp93 - 130和gp158含有可检测量的O-连接聚糖,而gp52则没有,这表明这些糖蛋白在糖基化方面存在差异。对gC-I二硫键的分析表明存在两种类型,一种对还原非常敏感,另一种则较不敏感。这些复合物可能由非常敏感的复合物间二硫键和较不敏感的复合物内二硫键组成。

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