A high-throughput, microplate reader-based method to monitor in vitro HIV latency reversal in the absence of flow cytometry

Chantal Emade Nkwelle, Unique Stephens, Kimberly Liang, Joel Cassel, Joseph Salvino, Luis J. Montaner, Roland N Ndip, Seraphine N Esemu, Fidele Ntie-Kang, Ian Tietjen
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Abstract

J-Lat cells are derivatives of the Jurkat CD4+ T cell line that contain a non-infectious, inducible HIV provirus with a GFP tag. While these cells have substantially advanced our understanding of HIV latency, their use by many laboratories in low and middle-income countries is restricted by limited access to flow cytometry. To overcome this barrier, we describe a modified J-Lat assay using a standard microplate reader that detects HIV-GFP expression following treatment with latency-reversing agents (LRAs). We show that HIV reactivation by control LRAs like prostratin and romidepsin is readily detected with dose dependence and with significant correlation and sensitivity to standard flow cytometry. For example, 10 micromol prostratin induced a 20.1 +/- 3.3-fold increase in GFP fluorescence in the microplate reader assay, which corresponded to 64.2 +/- 5.0% GFP-positive cells detected by flow cytometery. Similarly, 0.3 micromol prostratin induced a 1.7 +/- 1.2-fold increase compared to 8.7 +/- 5.7% GFP-positive cells detected. Using this method, we screen 79 epigenetic modifiers and identify molibresib, quisinostat, and CUDC-101 as novel LRAs. This microplate reader-based method offers accessibility to researchers in resource-limited regions to work with J-Lat cells and more actively participate in global HIV cure research efforts.
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一种基于微孔板阅读器的高通量方法,可在没有流式细胞仪的情况下监测体外艾滋病毒潜伏逆转情况
J-Lat 细胞是 Jurkat CD4+ T 细胞系的衍生物,含有非感染性、可诱导的带有 GFP 标记的 HIV 病毒。虽然这些细胞大大推进了我们对 HIV 潜伏期的了解,但由于流式细胞仪的使用受到限制,许多中低收入国家的实验室都无法使用这些细胞。为了克服这一障碍,我们介绍了一种改进的 J-Lat 检测方法,它使用标准微孔板阅读器检测潜伏期逆转剂 (LRA) 处理后的 HIV-GFP 表达。我们的研究表明,Prostratin 和 romidepsin 等对照 LRAs 可轻易检测到 HIV 的再激活,且与剂量相关,与标准流式细胞术有显著的相关性和灵敏度。例如,在微孔板阅读器检测中,10 微摩尔 prostratin 可诱导 GFP 荧光增加 20.1 +/- 3.3 倍,与流式细胞仪检测到的 64.2 +/- 5.0% GFP 阳性细胞相对应。类似地,0.3 微摩尔 prostratin 诱导的 GFP 阳性细胞增加了 1.7 +/- 1.2 倍,而流式细胞仪检测到的 GFP 阳性细胞为 8.7 +/- 5.7%。利用这种方法,我们筛选了 79 种表观遗传修饰剂,并确定了 molibresib、quininostat 和 CUDC-101 作为新型 LRA。这种基于微孔板阅读器的方法为资源有限地区的研究人员提供了使用J-Lat细胞的便利,使他们能更积极地参与全球艾滋病治愈研究工作。
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