Novel Assays for Measurement of Total Cell-Associated HIV-1 DNA and RNA

Although a number of PCR-based quantitative assays for measuring HIV-1 persistence during suppressive antiretroviral therapy (ART) have been reported, a simple, sensitive, reproducible method is needed for application to large clinical trials. We developed novel quantitative PCR assays for cell-asso...

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Bibliographic Details
Published in:	Journal of clinical microbiology Vol. 54; no. 4; pp. 902 - 911
Main Authors:	Hong, Feiyu, Aga, Evgenia, Cillo, Anthony R, Yates, Aarika L, Besson, Guillaume, Fyne, Elizabeth, Koontz, Dianna L, Jennings, Cheryl, Zheng, Lu, Mellors, John W
Format:	Journal Article
Language:	English
Published:	United States American Society for Microbiology 01-04-2016
Subjects:	Adult DNA, Viral - analysis DNA, Viral - genetics Female HIV Infections - virology HIV-1 - genetics HIV-1 - isolation & purification Humans Leukocytes, Mononuclear - virology Longitudinal Studies Male Middle Aged Reproducibility of Results RNA, Viral - analysis RNA, Viral - genetics Sensitivity and Specificity Viral Load - methods Virology
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Summary:	Although a number of PCR-based quantitative assays for measuring HIV-1 persistence during suppressive antiretroviral therapy (ART) have been reported, a simple, sensitive, reproducible method is needed for application to large clinical trials. We developed novel quantitative PCR assays for cell-associated (CA) HIV-1 DNA and RNA, targeting a highly conserved region in HIV-1pol, with sensitivities of 3 to 5 copies/1 million cells. We evaluated the performance characteristics of the assays using peripheral blood mononuclear cells (PBMCs) from 5 viremic patients and 20 patients receiving effective ART. Total and resting CD4(+)T cells were isolated from a subset of patients and tested for comparison with PBMCs. The estimated standard deviations including interassay variability and intra-assay variability of the assays were modest, i.e., 0.15 and 0.10 log10copies/10(6)PBMCs, respectively, for CA HIV-1 DNA and 0.40 and 0.19 log10copies/10(6)PBMCs for CA HIV-1 RNA. Testing of longitudinally obtained PBMC samples showed little variation for either viremic patients (median fold differences of 0.80 and 0.88 for CA HIV-1 DNA and RNA, respectively) or virologically suppressed patients (median fold differences of 1.14 and 0.97, respectively). CA HIV-1 DNA and RNA levels were strongly correlated (r= 0.77 to 1;P= 0.0001 to 0.037) for assays performed using PBMCs from different sources (phlebotomy versus leukapheresis) or using total or resting CD4(+)T cells purified by either bead selection or flow cytometric sorting. Their sensitivity, reproducibility, and broad applicability to small numbers of mononuclear cells make these assays useful for observational and interventional studies that examine longitudinal changes in the numbers of HIV-1-infected cells and their levels of transcription.
Bibliography:	ObjectType-Article-1 SourceType-Scholarly Journals-1 ObjectType-Feature-2 content type line 23 Present address: Aarika L. Yates, University of Pittsburgh, Department of Immunology, Pittsburgh, Pennsylvania, USA; Guillaume Besson, Community College of Allegheny County, Pittsburgh, Pennsylvania, USA; Elizabeth Fyne, UPMC Hospital, Pittsburgh, Pennsylvania, USA. Citation Hong F, Aga E, Cillo AR, Yates AL, Besson G, Fyne E, Koontz DL, Jennings C, Zheng L, Mellors JW. 2016. Novel assays for measurement of total cell-associated HIV-1 DNA and RNA. J Clin Microbiol 54:902–911. doi:10.1128/JCM.02904-15.
ISSN:	0095-1137 1098-660X
DOI:	10.1128/jcm.02904-15