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携带天然 HIV 包膜三聚体的假病毒颗粒促进了一种新的方法来产生针对 HIV 的人源中和性单克隆抗体。

Pseudovirion particles bearing native HIV envelope trimers facilitate a novel method for generating human neutralizing monoclonal antibodies against HIV.

机构信息

Department of Pediatrics, Vanderbilt University Medical Center, Nashville, TN 37232-2905, USA.

出版信息

J Acquir Immune Defic Syndr. 2010 Jul;54(3):223-35. doi: 10.1097/QAI.0b013e3181dc98a3.

DOI:10.1097/QAI.0b013e3181dc98a3
PMID:20531016
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2930513/
Abstract

Monomeric HIV envelope vaccines fail to elicit broadly neutralizing antibodies or to protect against infection. Neutralizing antibodies against HIV bind to native functionally active Env trimers on the virion surface. Gag-Env pseudovirions recapitulate the native trimer and could serve as an effective epitope presentation platform for study of the neutralizing antibody response in HIV-infected individuals. To address if pseudovirions can recapitulate native HIV virion epitope structures, we carefully characterized these particles, concentrating on the antigenic structure of the coreceptor binding site. By blue native gel shift assays, Gag-Env pseudovirions were shown to contain native trimers that were competent for binding to neutralizing monoclonal antibodies. In enzyme-linked immunosorbent assay, pseudovirions exhibited increased binding of known CD4-induced antibodies after addition of CD4. Using flow cytometric analysis, fluorescently labeled pseudovirions specifically identified a subset of antigen-specific B cells in HIV-infected subjects. Interestingly, the sequence of one of these novel human antibodies, identified during cloning of single HIV-specific B cells and designated 2C6, exhibited homology to mAb 47e, a known anti-CD4-induced coreceptor binding site antibody. The secreted monoclonal antibody 2C6 did not bind monomeric gp120, but specifically bound envelope on pseudovirions. A recombinant form of the antibody 2C6 acted as a CD4-induced epitope-specific antibody in neutralization assays, yet did not bind monomeric gp120. These findings imply specificity against a quaternary epitope presented on the pseudovirion envelope spike. These data demonstrate that Gag-Env pseudovirions recapitulate CD4 and coreceptor binding pocket antigenic structures and can facilitate identification of B-cell clones that secrete neutralizing antibodies.

摘要

单体 HIV 包膜疫苗未能引发广泛中和抗体或预防感染。HIV 的中和抗体结合在病毒表面的天然功能活性 Env 三聚体上。Gag-Env 假病毒可再现天然三聚体,并可作为研究 HIV 感染者中和抗体反应的有效表位呈递平台。为了确定假病毒是否可以再现天然 HIV 病毒衣壳的表位结构,我们仔细表征了这些颗粒,重点研究了核心受体结合位点的抗原结构。通过蓝色非变性凝胶电泳,显示 Gag-Env 假病毒包含有能力结合中和单克隆抗体的天然三聚体。在酶联免疫吸附试验中,添加 CD4 后,假病毒显示出增加了与已知 CD4 诱导抗体的结合。通过流式细胞分析,荧光标记的假病毒特异性识别了 HIV 感染个体中抗原特异性 B 细胞的亚群。有趣的是,这些新的人类抗体之一的序列,在克隆单个 HIV 特异性 B 细胞期间被鉴定出来,并被指定为 2C6,与 mAb 47e 表现出同源性,这是一种已知的抗 CD4 诱导的核心受体结合位点抗体。分泌的单克隆抗体 2C6 不与单体 gp120 结合,但特异性结合假病毒上的包膜。抗体 2C6 的重组形式在中和试验中充当 CD4 诱导的表位特异性抗体,但不与单体 gp120 结合。这些发现意味着针对假病毒包膜刺突上呈现的四级表位的特异性。这些数据表明,Gag-Env 假病毒再现了 CD4 和核心受体结合口袋的抗原结构,并可以促进识别分泌中和抗体的 B 细胞克隆。

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