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确定HIV潜伏逆转实验中的稳定参照基因。

Defining stable reference genes in HIV latency reversal experiments.

作者信息

Ceriani Cristina, Streeter Gabrielle S, Lemu Kena J, James Katherine S, Ghofrani Simon, Allard Brigitte, Shook-Sa Bonnie E, Margolis David M, Archin Nancie M

机构信息

UNC HIV Cure Center, The University of North Carolina at Chapel Hill, Chapel Hill, NC 27514, United States.

Department of Medicine, The University of North Carolina at Chapel Hill, Chapel Hill, NC 27154, United States.

出版信息

J Virol. 2021 May 10;95(11). doi: 10.1128/JVI.02305-20. Epub 2021 Mar 24.

Abstract

Quantification of cell associated HIV RNA (ca-RNA) is one of the most important and commonly used methods to evaluate the performance of latency-reversing agents (LRAs). Copies of HIV RNA measured by qPCR, are often normalized to the input RNA or cell number. However, these could be affected by biological variability and/or technical errors, which can be avoided by using an internal reference gene. To obtain reliable data, it is essential to select stable reference genes (RGs) of which the expression is not influenced by biological variability, the type of cells, or the LRAs used. However, to date, no study has carefully evaluated RG stability following LRA exposure. We analyzed the stability of six widely used RGs (, , , , and ) in human PBMC and CD4+ T cells. LRA exposure significantly influenced the stability of these RGs. Overall, , , and were the most stable RGs in all tested conditions. was generally the most stable RG whereas varied the most. Finally, we evaluated the impact of applying different RG normalizers to host genes and HIV ca-RNA data. Altered results were observed both in host and HIV gene expression when unstable RGs were used. Our data underline the importance of testing the stability of RGs utilized to evaluate LRA-induced HIV ca-RNA expression. To our knowledge, this is the first careful evaluation of the stability of RGs after LRA exposure and will significantly contribute to the quality of data analysis in regard to gene expression.Latency-reversing agents (LRAs) are ubiquitously used in the "shock-and-kill" HIV cure strategy and their performance is often evaluated by ex-vivo quantification of cell associated HIV RNA. HIV RNA, measured by qPCR, is often normalized to internal reference genes, but the expression of these genes should not be influenced by the experimental settings. We found that treatment of human PBMC and CD4+ T cells with LRAs significantly altered the expression of several commonly used reference genes, such as GAPDH. Finally, we evaluate the impact of different reference genes on normalization of host genes and HIV cell associated RNA expression and demonstrated that using unstable reference genes dramatically altered experimental outcome. Our data highlight the importance of using reference genes that are unaffected by LRAs under study to correctly evaluate host gene and cell associated HIV RNA expression induced by latency-reversing agents.

摘要

细胞相关HIV RNA(ca-RNA)的定量分析是评估潜伏逆转剂(LRA)性能的最重要且常用的方法之一。通过qPCR测量的HIV RNA拷贝数通常会根据输入RNA或细胞数量进行标准化。然而,这些可能会受到生物学变异性和/或技术误差的影响,而使用内部参考基因可以避免这些问题。为了获得可靠的数据,选择稳定的参考基因(RG)至关重要,其表达不受生物学变异性、细胞类型或所用LRA的影响。然而,迄今为止,尚无研究仔细评估LRA暴露后RG的稳定性。我们分析了六种广泛使用的RG(、、、、和)在人外周血单个核细胞(PBMC)和CD4 + T细胞中的稳定性。LRA暴露显著影响了这些RG的稳定性。总体而言,、和在所有测试条件下是最稳定的RG。通常是最稳定的RG,而变化最大。最后,我们评估了应用不同的RG标准化因子对宿主基因和HIV ca-RNA数据的影响。当使用不稳定的RG时,宿主基因和HIV基因表达均观察到结果改变。我们的数据强调了测试用于评估LRA诱导的HIV ca-RNA表达的RG稳定性的重要性。据我们所知,这是首次对LRA暴露后RG的稳定性进行仔细评估,将显著有助于基因表达数据分析的质量。潜伏逆转剂(LRA)在“激活并清除”HIV治愈策略中被广泛使用,其性能通常通过体外定量细胞相关HIV RNA来评估。通过qPCR测量的HIV RNA通常会根据内部参考基因进行标准化,但这些基因的表达不应受实验设置的影响。我们发现用LRA处理人PBMC和CD4 + T细胞会显著改变几种常用参考基因的表达,如甘油醛-3-磷酸脱氢酶(GAPDH)。最后,我们评估了不同参考基因对宿主基因标准化和HIV细胞相关RNA表达的影响,并证明使用不稳定的参考基因会显著改变实验结果。我们的数据突出了使用不受所研究LRA影响の参考基因来正确评估潜伏逆转剂诱导的宿主基因和细胞相关HIV RNA表达的重要性。

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