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由 HIV 潜伏感染 CD4+ 淋巴细胞诱导的病毒粒子的复制能力。

Replication competence of virions induced from CD4+ lymphocytes latently infected with HIV.

机构信息

San Diego Veterans Affairs Healthcare System, San Diego, CA, USA.

University of California San Diego, La Jolla, CA, USA.

出版信息

Retrovirology. 2019 Feb 15;16(1):4. doi: 10.1186/s12977-019-0466-1.

Abstract

Latently infected CD4 lymphocytes preclude cure of HIV infection, even with the most effective antiretroviral therapy. The replication competent latent HIV reservoir has been quantified with the terminal dilution quantitative viral outgrowth assay, which induces virus propagation in CD4 T cell culture supernatants following cellular activation. Efforts to improve the sensitivity of this inefficient assay have introduced more sensitive p24 ELISA and RNA PCR based endpoints, but these more sensitive endpoints have raised the question whether they are measuring induced replication competent or defective virions. Here we performed parallel terminal dilution assays with CD4 lymphocytes from subjects effectively treated with antiretroviral therapy. An HIV integrase inhibitor was incorporated into one set of parallel cultures to compare the frequency of cells that can be induced to produce virions to those that produce virus that can propagate and amplify with co-culture in permissive cells. The majority of cells that can be induced to generate virus particles are producing replication competent virus, thus justifying more sensitive and faster assays of this reservoir.

摘要

潜伏感染的 CD4 淋巴细胞会阻碍 HIV 感染的治愈,即使采用最有效的抗逆转录病毒疗法也是如此。利用末端稀释定量病毒生长检测法对具有复制能力的潜伏 HIV 储存库进行了定量,该检测法在细胞激活后诱导 CD4 T 细胞培养上清液中的病毒增殖。为了提高该低效检测法的灵敏度,引入了更灵敏的 p24 ELISA 和基于 RNA PCR 的终点,但这些更灵敏的终点引发了一个问题,即它们是否在测量诱导产生的具有复制能力的病毒还是缺陷型病毒。在此,我们使用经过抗逆转录病毒治疗的有效治疗的受试者的 CD4 淋巴细胞进行了平行的末端稀释检测。将一种 HIV 整合酶抑制剂纳入一组平行培养物中,以比较可以诱导产生病毒颗粒的细胞与那些可以产生具有复制能力并能在允许细胞中进行共培养而扩增的病毒的细胞的频率。大多数可以诱导产生病毒颗粒的细胞都在产生具有复制能力的病毒,因此证明了对该储存库进行更灵敏和更快的检测是合理的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5fdf/6377736/9a4ad9cdad4b/12977_2019_466_Fig1_HTML.jpg

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