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一种基于细胞的荧光素酶报告质粒检测法,可用于高通量筛选,以鉴定新型 FDA 批准的 HPV-16 感染药物抑制剂。

A Cell-Based Luminescence Reporter Plasmid Assay for High-Throughput Screening to Identify Novel FDA-Approved Drug Inhibitors of HPV-16 Infection.

机构信息

Department of Community Health Systems, School of Nursing, University of California, San Francisco, CA, USA.

Department of Infectious Disease, Palefsky Laboratory, School of Medicine, University of California, San Francisco, CA, USA.

出版信息

SLAS Discov. 2020 Jan;25(1):79-86. doi: 10.1177/2472555219860771. Epub 2019 Jul 30.

Abstract

Like cervical cancer, anal cancer is caused by human papillomavirus (HPV). HPV is the most common sexually transmitted agent and is found in the anal canal of almost all HIV-positive men who have sex with men (MSM). Rates of HPV anal cancer are disproportionately higher in this population. Although the nanovalent HPV vaccine is efficacious in protecting against oncogenic HPV types, a substantial proportion of MSM remains unvaccinated and anal HPV infection continues to be an important public health burden. Therefore, it is important to identify strategies to prevent HPV infection. We report on two promising and interlinked strategies: (1) the development of a cell-based luminescence reporter assay using HPV-16 pseudovirions that encapsidate SV40-driven luminescence reporter expression plasmid and (2) use of this assay for high-throughput screening (HTS) of FDA- and internationally approved drugs to identify those that could be repurposed to prevent HPV infection. We conducted a screen of 1906 drugs. The assay was valid with a Z' of 0.67 ± 0.04, percent coefficient of variance of 10.0, and signal-to-background noise window of 424.0 ± 8.0. Five drugs were chosen for further analyses based on selection parameters of ≥77.0% infection of HPV-16 pseudovirion-driven expression with <20.0% cytotoxicity. Of these, the antifungal pentamidine and a gamma-amino butyric acid receptor agonist securinine exhibited ≥90.0% infection with <10.0% cytotoxicity. This luminescent cell-based reporter expression plasmid assay for HTS is a valid method to identify FDA- and internationally approved drugs with the potential to be repurposed into prevention modalities for HPV infection.

摘要

与宫颈癌一样,肛门癌也是由人乳头瘤病毒(HPV)引起的。HPV 是最常见的性传播病原体,几乎存在于所有与男性发生性关系的 HIV 阳性男性(MSM)的肛门管中。在这一人群中,HPV 肛门癌的发病率高得不成比例。虽然九价 HPV 疫苗在预防致癌 HPV 型方面有效,但相当一部分 MSM 仍未接种疫苗,肛门 HPV 感染仍然是一个重要的公共卫生负担。因此,确定预防 HPV 感染的策略非常重要。我们报告了两种有前途且相互关联的策略:(1)使用 HPV-16 假病毒来开发基于细胞的发光报告基因检测,该假病毒封装 SV40 驱动的发光报告基因表达质粒;(2)使用该检测方法对 FDA 和国际上批准的药物进行高通量筛选(HTS),以鉴定可用于预防 HPV 感染的药物。我们进行了 1906 种药物的筛选。该检测方法的 Z' 值为 0.67 ± 0.04,变异系数为 10.0%,信号与背景噪声窗口为 424.0 ± 8.0。根据 ≥77.0%感染 HPV-16 假病毒驱动的表达且 ≤20.0%细胞毒性的选择参数,选择了 5 种药物进行进一步分析。其中,抗真菌药物戊双脒和γ-氨基丁酸受体激动剂瓜氨酸表现出 ≥90.0%的感染率,且细胞毒性<10.0%。这种用于 HTS 的发光细胞基础报告基因表达质粒检测方法是一种有效的方法,可以鉴定出具有潜在用途的 FDA 和国际上批准的药物,可将其重新用于预防 HPV 感染。

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