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补体和特异性抗体与HIV-1外膜糖蛋白120的相互作用。

Interaction of complement and specific antibodies with the external glycoprotein 120 of HIV-1.

作者信息

Prohászka Z, Hidvégi T, Ujhelyi E, Stoiber H, Dierich M P, Süsal C, Füst G

机构信息

National Institute of Haematology, Blood Transfusion and Immunology, Budapest, Hungary.

出版信息

Immunology. 1995 Jun;85(2):184-9.

Abstract

Previously we have investigated the interaction of human complement as well as one polyclonal and three human monoclonal antibody preparations with the human immunodeficiency virus type-1 (HIV-1) transmembrane recombinant glycoprotein (rgp41). A strong competition was found between the antibodies and deposited complement proteins for the same binding sites located within the immunodominant region of rgp41. The aim of the present experiments was to see if the same type of antibody-complement-HIV-1 interactions could be observed with the outer envelope glycoprotein (rgp120) of HIV-1. Three different glycosylated rgp120 preparations, as well as a synthetic peptide corresponding to the V3 loop of the MN strain, were adsorbed to enzyme-linked immunosorbent assay (ELISA) plates and incubated with mixtures of anti-rgp120 antibodies and normal human serum (NHS) as a complement source. Fixed complement proteins and antibodies were detected with specific, peroxidase-labelled antibodies against different complement proteins (C1q, C4b, C3b) and the gamma-chain of antibodies. In the absence of anti-rgp120, high amounts of C3 were deposited to each rgp120 preparation tested (including the V3 peptide) but significant differences in the amounts of bound C1q and C4b were observed. Using sera deficient in different complement proteins, we found that both the classical and the alternative pathways contributed to the C3 binding to rgp120. Addition of specific antibodies did not increase complement activation by rgp120 and only in the case of a monoclonal antibody to the V3-loop could we see complement-dependent inhibition of antibody binding.

摘要

此前我们已经研究了人补体以及一种多克隆抗体和三种人单克隆抗体制剂与人类免疫缺陷病毒1型(HIV-1)跨膜重组糖蛋白(rgp41)的相互作用。发现抗体与沉积的补体蛋白之间在rgp41免疫显性区域内的相同结合位点存在强烈竞争。本实验的目的是观察是否能在HIV-1的外膜糖蛋白(rgp120)上观察到相同类型的抗体-补体-HIV-1相互作用。将三种不同糖基化的rgp120制剂以及对应于MN株V3环的合成肽吸附到酶联免疫吸附测定(ELISA)板上,并与抗rgp120抗体和作为补体来源的正常人血清(NHS)的混合物一起孵育。用针对不同补体蛋白(C1q、C4b、C3b)和抗体γ链的特异性过氧化物酶标记抗体检测固定的补体蛋白和抗体。在没有抗rgp120的情况下,大量的C3沉积到每个测试的rgp120制剂(包括V3肽)上,但观察到结合的C1q和C4b量存在显著差异。使用缺乏不同补体蛋白的血清,我们发现经典途径和替代途径都有助于C3与rgp120的结合。添加特异性抗体不会增加rgp120介导的补体激活,只有在针对V3环的单克隆抗体的情况下,我们才能看到补体依赖性的抗体结合抑制。

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本文引用的文献

1
Complement activation by gp160 glycoprotein of HIV-1.
AIDS Res Hum Retroviruses. 1993 Mar;9(3):229-33. doi: 10.1089/aid.1993.9.229.
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AIDS. 1993 Oct;7(10):1307-13. doi: 10.1097/00002030-199310000-00002.
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Complement activation by human monoclonal antibodies to human immunodeficiency virus.
J Virol. 1993 Jan;67(1):53-9. doi: 10.1128/JVI.67.1.53-59.1993.

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