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复制型 HIV-1 分子克隆表达海肾荧光素酶,有助于分析 PBMC 中的抗体抑制作用。

Replication competent molecular clones of HIV-1 expressing Renilla luciferase facilitate the analysis of antibody inhibition in PBMC.

机构信息

Department of Molecular and Cellular Pathology, University of Alabama at Birmingham, 701 19th Street South, Birmingham, AL 35294, USA.

出版信息

Virology. 2010 Dec 5;408(1):1-13. doi: 10.1016/j.virol.2010.08.028. Epub 2010 Sep 21.

Abstract

Effective vaccine development for human immunodeficiency virus type 1 (HIV-1) will require assays that ascertain the capacity of vaccine immunogens to elicit neutralizing antibodies (NAb) to diverse HIV-1 strains. To facilitate NAb assessment in peripheral blood mononuclear cell (PBMC)-based assays, we developed an assay-adaptable platform based on a Renilla luciferase (LucR) expressing HIV-1 proviral backbone. LucR was inserted into pNL4-3 DNA, preserving all viral open reading frames. The proviral genome was engineered to facilitate expression of diverse HIV-1 env sequences, allowing analysis in an isogenic background. The resulting Env-IMC-LucR viruses are infectious, and LucR is stably expressed over multiple replications in PBMC. HIV-1 neutralization, targeting TZM-bl cells, was highly correlative comparing virus (LucR) and cell (firefly luciferase) readouts. In PBMC, NAb activity can be analyzed either within a single or multiple cycles of replication. These results represent advancement toward a standardizable PBMC-based neutralization assay for assessing HIV-1 vaccine immunogen efficacy.

摘要

为了开发出有效的人类免疫缺陷病毒 1 型(HIV-1)疫苗,我们需要确定疫苗免疫原激发针对不同 HIV-1 毒株的中和抗体(NAb)的能力。为了在基于外周血单核细胞(PBMC)的检测中促进 NAb 的评估,我们开发了一种基于表达荧光素酶(LucR)的 HIV-1 前病毒骨架的可适应检测平台。LucR 被插入 pNL4-3 DNA 中,保留了所有病毒开放阅读框。前病毒基因组经过工程改造,以促进多样化 HIV-1 env 序列的表达,从而在同基因背景下进行分析。由此产生的 Env-IMC-LucR 病毒具有感染性,并且 LucR 在 PBMC 中多次复制过程中稳定表达。HIV-1 中和作用针对 TZM-bl 细胞,病毒(LucR)和细胞(荧光素酶)读数之间具有高度相关性。在 PBMC 中,可以在单个或多个复制周期内分析 NAb 活性。这些结果代表朝着用于评估 HIV-1 疫苗免疫原功效的标准化 PBMC 中和测定法的前进。

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