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N-连接聚糖的碳水化合物决定簇NeuAc-Galβ(1-4)调节人类免疫缺陷病毒1型糖蛋白gp120的抗原活性。

Carbohydrate determinant NeuAc-Gal beta (1-4) of N-linked glycans modulates the antigenic activity of human immunodeficiency virus type 1 glycoprotein gp120.

作者信息

Bolmstedt A, Olofsson S, Sjögren-Jansson E, Jeansson S, Sjöblom I, Akerblom L, Hansen J E, Hu S L

机构信息

Department of Clinical Virology, University of Göteborg, Sweden.

出版信息

J Gen Virol. 1992 Dec;73 ( Pt 12):3099-105. doi: 10.1099/0022-1317-73-12-3099.

DOI:10.1099/0022-1317-73-12-3099
PMID:1281869
Abstract

In the present study we investigated to what extent the peripheral carbohydrate structure of N-linked glycans influences the antigenic properties of human immunodeficiency virus type 1 glycoprotein 120 (gp120). Recombinant gp120 was purified from GMK cells infected with a recombinant vaccinia virus expressing gp120. Purified gp120 was then coated onto 96-well ELISA microplates and subjected to sequential removal of peripheral monosaccharide units. Modified or unmodified gp120 was then incubated with monoclonal antibodies recognizing specific epitopes of gp120 and with a reporter lectin to determine the extent of carbohydrate elimination. Antibody and lectin binding was quantified in an enzyme-linked system. We found that the carbohydrate structure NeuAc-Gal beta (1-4) of N-linked glycans, defined both by lectin reactivity and by specific glycosidases, is involved in modulating the binding of antibody to a number of epitopes of peptide nature. The binding of antibody to one class of epitopes, situated in a region between amino acids 200 and 230, was strongly increased by removal of NeuAc-Gal beta (1-4), whereas the binding to epitopes in the V3 region was decreased and the binding to epitopes in the far N-terminal region was not altered by the treatment. These results suggested that peripheral structures of N-glycans are involved in modulating the overall conformation of gp120.

摘要

在本研究中,我们调查了N-连接聚糖的外周碳水化合物结构在多大程度上影响1型人类免疫缺陷病毒糖蛋白120(gp120)的抗原特性。重组gp120从感染了表达gp120的重组痘苗病毒的GMK细胞中纯化得到。然后将纯化的gp120包被到96孔酶联免疫吸附测定(ELISA)微孔板上,并依次去除外周单糖单元。接着将修饰或未修饰的gp120与识别gp120特定表位的单克隆抗体以及一种报告凝集素一起孵育,以确定碳水化合物去除的程度。在酶联系统中对抗体和凝集素的结合进行定量。我们发现,通过凝集素反应性和特定糖苷酶定义的N-连接聚糖的碳水化合物结构NeuAc-Galβ(1-4)参与调节抗体与许多肽性质表位的结合。去除NeuAc-Galβ(1-4)后,抗体与位于氨基酸200至230之间区域的一类表位的结合显著增加,而与V3区域表位的结合减少,与远N端区域表位的结合不受该处理影响。这些结果表明,N-聚糖的外周结构参与调节gp120的整体构象。

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