Robichaux Spencer, Lacour Nedra, Bagby Gregory J, Amedee Angela M
Louisiana State University Health Sciences Center, New Orleans, United States.
Louisiana State University Health Sciences Center, New Orleans, United States.
J Virol Methods. 2016 Oct;236:245-251. doi: 10.1016/j.jviromet.2016.08.004. Epub 2016 Aug 7.
Persistent HIV reservoirs and the absolute quantification of viral RNA copies in tissues have become a prominent focus of multiple areas ofHIV/SIV research. Absolute quantification of viral RNA via reverse transcription, quantitative PCR (RT-qPCR) necessitates the use of an appropriate RNA reference gene whose expression is unaffected by both experimental and confounding conditions. In this study, we demonstrate the utility of ribosomal protein S13 mRNA (RPS13) as a stable, medium abundance reference gene for RT-qPCR normalization of HIV/SIV RNA copy number. We developed a RPS13 RNA standard assay utilizing an in vitro RNA transcript for normalization of absolute SIV RNA quantities in tissues reservoirs. The RT-qPCR assay showed a high degree of repeatability and reproducibility across RNA levels appropriate for absolute SIV quantification. In assessing the utility of RPS13 as a reference gene, limited variation in the absolute, inter-tissue quantities of RPS13 mRNA was observed within multiple tissue samples obtained from rhesus macaques (average CV=2.86%). We demonstrate rhesus macaque RPS13 mRNA expression is not affected by alcohol administration, SIV infection, or antiviral therapy (PMPA/FTC). Additionally, assay functionality was validated for normalization of SIV copy number using cellular RNA prepared from samples of variable RNA integrity. RPS13 is a suitable reference gene for normalization of absolute SIV RNA quantities in tissues and is most appropriate for intra-tissue or similar tissue type comparisons of SIV copy number.
持续存在的HIV储存库以及组织中病毒RNA拷贝的绝对定量已成为HIV/SIV研究多个领域的一个突出重点。通过逆转录定量PCR(RT-qPCR)对病毒RNA进行绝对定量,需要使用一种合适的RNA参照基因,其表达不受实验条件和混杂因素的影响。在本研究中,我们证明了核糖体蛋白S13 mRNA(RPS13)作为一种稳定的、中等丰度的参照基因,可用于HIV/SIV RNA拷贝数的RT-qPCR标准化。我们开发了一种RPS13 RNA标准检测方法,利用体外RNA转录本来标准化组织储存库中SIV RNA的绝对量。RT-qPCR检测在适合SIV绝对定量的RNA水平上显示出高度的重复性和再现性。在评估RPS13作为参照基因的效用时,在从恒河猴获得的多个组织样本中,观察到RPS13 mRNA的绝对组织间量的变化有限(平均CV=2.86%)。我们证明恒河猴RPS13 mRNA表达不受酒精给药、SIV感染或抗病毒治疗(替诺福韦酯/恩曲他滨)的影响。此外,使用从具有可变RNA完整性的样本制备的细胞RNA对SIV拷贝数标准化的检测功能进行了验证。RPS13是用于组织中SIV RNA绝对量标准化的合适参照基因,最适合于SIV拷贝数的组织内或类似组织类型比较。