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一种用于检测针对感染 HIV-1 或 SIV 细胞的抗体依赖细胞介导的细胞毒性的新方法显示,与中和和结合测定中测量的抗体不完全重叠。

A novel assay for antibody-dependent cell-mediated cytotoxicity against HIV-1- or SIV-infected cells reveals incomplete overlap with antibodies measured by neutralization and binding assays.

机构信息

Department of Microbiology and Immunobiology, Harvard Medical School, New England Primate Research Center, Southborough, Massachusetts, USA.

出版信息

J Virol. 2012 Nov;86(22):12039-52. doi: 10.1128/JVI.01650-12. Epub 2012 Aug 29.

Abstract

The resistance of human immunodeficiency virus type 1 (HIV-1) to antibody-mediated immunity often prevents the detection of antibodies that neutralize primary isolates of HIV-1. However, conventional assays for antibody functions other than neutralization are suboptimal. Current methods for measuring the killing of virus-infected cells by antibody-dependent cell-mediated cytotoxicity (ADCC) are limited by the number of natural killer (NK) cells obtainable from individual donors, donor-to-donor variation, and the use of nonphysiological targets. We therefore developed an ADCC assay based on NK cell lines that express human or macaque CD16 and a CD4(+) T-cell line that expresses luciferase from a Tat-inducible promoter upon HIV-1 or simian immunodeficiency virus (SIV) infection. NK cells and virus-infected targets are mixed in the presence of serial plasma dilutions, and ADCC is measured as the dose-dependent loss of luciferase activity. Using this approach, ADCC titers were measured in plasma samples from HIV-infected human donors and SIV-infected macaques. For the same plasma samples paired with the same test viruses, this assay was approximately 2 orders of magnitude more sensitive than optimized assays for neutralizing antibodies-frequently allowing the measurement of ADCC in the absence of detectable neutralization. Although ADCC correlated with other measures of Env-specific antibodies, neutralizing and gp120 binding titers did not consistently predict ADCC activity. Hence, this assay affords a sensitive method for measuring antibodies capable of directing ADCC against HIV- or SIV-infected cells expressing native conformations of the viral envelope glycoprotein and reveals incomplete overlap of the antibodies that direct ADCC and those measured in neutralization and binding assays.

摘要

人类免疫缺陷病毒 1 型(HIV-1)对抗体介导的免疫的抗性常常阻止了中和 HIV-1 原始分离株的抗体的检测。然而,除中和作用之外的抗体功能的常规检测方法并不理想。目前用于测量抗体依赖性细胞介导的细胞毒性(ADCC)对病毒感染细胞的杀伤的方法受到从个体供体中获得的自然杀伤(NK)细胞数量、供体间的变异性以及非生理靶标的使用的限制。因此,我们开发了一种基于表达人或猕猴 CD16 的 NK 细胞系和表达来自 Tat 诱导型启动子的荧光素酶的 CD4(+)T 细胞系的 ADCC 测定法,用于 HIV-1 或猴免疫缺陷病毒(SIV)感染。在存在系列血浆稀释液的情况下混合 NK 细胞和病毒感染的靶标,并将 ADCC 作为依赖剂量的荧光素酶活性丧失来测量。使用这种方法,测量了来自 HIV 感染的人类供体和 SIV 感染的猕猴的血浆样品中的 ADCC 效价。对于相同的血浆样品与相同的测试病毒配对,该测定法比用于中和抗体的优化测定法灵敏约 2 个数量级-通常允许在没有可检测到的中和作用的情况下测量 ADCC。尽管 ADCC 与其他 Env 特异性抗体的测量相关,但中和和 gp120 结合效价并不始终预测 ADCC 活性。因此,该测定法提供了一种灵敏的方法,用于测量能够针对表达病毒包膜糖蛋白天然构象的 HIV-或 SIV 感染细胞指导 ADCC 的抗体,并揭示了指导 ADCC 的抗体与中和和结合测定法中测量的抗体之间不完全重叠。

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