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使用RNA流式荧光原位杂交技术对罕见的HIV感染细胞进行多参数表征。

Multiparametric characterization of rare HIV-infected cells using an RNA-flow FISH technique.

作者信息

Baxter Amy E, Niessl Julia, Fromentin Rémi, Richard Jonathan, Porichis Filippos, Massanella Marta, Brassard Nathalie, Alsahafi Nirmin, Routy Jean-Pierre, Finzi Andrés, Chomont Nicolas, Kaufmann Daniel E

机构信息

Research Centre of the Centre Hospitalier de l'Université de Montréal (CRCHUM) and Université de Montréal, Montreal, Quebec, Canada.

Center for HIV/AIDS Vaccine Immunology and Immunogen Discovery (CHAVI-ID), La Jolla, California, USA.

出版信息

Nat Protoc. 2017 Oct;12(10):2029-2049. doi: 10.1038/nprot.2017.079. Epub 2017 Sep 7.

Abstract

Efforts to cure HIV are hampered by limited characterization of the cells supporting HIV replication in vivo and inadequate methods for quantifying the latent viral reservoir in individuals receiving antiretroviral therapy (ART). We describe a protocol for flow cytometric identification of viral reservoirs, based on concurrent detection of cellular HIV Gagpol mRNA by in situ RNA hybridization combined with antibody staining for the HIV Gag protein. By simultaneously detecting both HIV RNA and protein, the CD4 T cells harboring translation-competent virus can be identified. The HIV method is 1,000-fold more sensitive than Gag protein staining alone, with a detection limit of 0.5-1 Gagpol mRNA/Gag protein cells per million CD4 T cells. Uniquely, the HIV assay also allows parallel phenotyping of viral reservoirs, including reactivated latent reservoirs in clinical samples. The assay takes 2 d, and requires antibody labeling for surface and intracellular markers, followed by mRNA labeling and multiple signal amplification steps.

摘要

治愈艾滋病病毒(HIV)的努力受到多种因素的阻碍,其中包括对体内支持HIV复制的细胞特征描述有限,以及在接受抗逆转录病毒疗法(ART)的个体中量化潜伏病毒库的方法不足。我们描述了一种通过流式细胞术鉴定病毒库的方案,该方案基于原位RNA杂交同时检测细胞内HIV Gagpol mRNA,并结合HIV Gag蛋白的抗体染色。通过同时检测HIV RNA和蛋白质,可以识别携带具有翻译能力病毒的CD4 T细胞。该HIV检测方法比单独的Gag蛋白染色灵敏1000倍,检测限为每百万CD4 T细胞中有0.5 - 1个Gagpol mRNA/Gag蛋白细胞。独特的是,该HIV检测还允许对病毒库进行平行表型分析,包括临床样本中重新激活的潜伏病毒库。该检测需要2天时间,需要对表面和细胞内标志物进行抗体标记,随后进行mRNA标记和多个信号放大步骤。

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