Accurate episomal HIV 2-LTR circles quantification using optimized DNA isolation and droplet digital PCR

INTRODUCTION: In HIV-infected patients on combination antiretroviral therapy (cART), the detection of episomal HIV 2-LTR circles is a potential marker for ongoing viral replication. Quantification of 2-LTR circles is based on quantitative PCR or more recently on digital PCR assessment, but is hamper...

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Autores principales: Malatinkova, Eva, Kiselinova, Maja, Bonczkowski, Pawel, Trypsteen, Wim, Messiaen, Peter, Vermeire, Jolien, Verhasselt, Bruno, Vervisch, Karen, Vandekerckhove, Linos, De Spiegelaere, Ward
Formato: Online Artículo Texto
Lenguaje:English
Publicado: International AIDS Society 2014
Materias:
Poster Sessions – Abstract P142
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4225365/
https://www.ncbi.nlm.nih.gov/pubmed/25397424
http://dx.doi.org/10.7448/IAS.17.4.19674
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author Malatinkova, Eva
Kiselinova, Maja
Bonczkowski, Pawel
Trypsteen, Wim
Messiaen, Peter
Vermeire, Jolien
Verhasselt, Bruno
Vervisch, Karen
Vandekerckhove, Linos
De Spiegelaere, Ward
author_facet Malatinkova, Eva
Kiselinova, Maja
Bonczkowski, Pawel
Trypsteen, Wim
Messiaen, Peter
Vermeire, Jolien
Verhasselt, Bruno
Vervisch, Karen
Vandekerckhove, Linos
De Spiegelaere, Ward
author_sort Malatinkova, Eva
collection PubMed
description INTRODUCTION: In HIV-infected patients on combination antiretroviral therapy (cART), the detection of episomal HIV 2-LTR circles is a potential marker for ongoing viral replication. Quantification of 2-LTR circles is based on quantitative PCR or more recently on digital PCR assessment, but is hampered due to its low abundance. Sample pre-PCR processing is a critical step for 2-LTR circles quantification, which has not yet been sufficiently evaluated in patient derived samples. MATERIALS AND METHODS: We compared two sample processing procedures to more accurately quantify 2-LTR circles using droplet digital PCR (ddPCR). Episomal HIV 2-LTR circles were either isolated by genomic DNA isolation or by a modified plasmid DNA isolation, to separate the small episomal circular DNA from chromosomal DNA. This was performed in a dilution series of HIV-infected cells and HIV-1 infected patient derived samples (n=59). Samples for the plasmid DNA isolation method were spiked with an internal control plasmid. RESULTS: Genomic DNA isolation enables robust 2-LTR circles quantification. However, in the lower ranges of detection, PCR inhibition caused by high genomic DNA load substantially limits the amount of sample input and this impacts sensitivity and accuracy. Moreover, total genomic DNA isolation resulted in a lower recovery of 2-LTR templates per isolate, further reducing its sensitivity. The modified plasmid DNA isolation with a spiked reference for normalization was more accurate in these low ranges compared to genomic DNA isolation. A linear correlation of both methods was observed in the dilution series (R2=0.974) and in the patient derived samples with 2-LTR numbers above 10 copies per million peripheral blood mononuclear cells (PBMCs), (R2=0.671). Furthermore, Bland–Altman analysis revealed an average agreement between the methods within the 27 samples in which 2-LTR circles were detectable with both methods (bias: 0.3875±1.2657 log(10)). CONCLUSIONS: 2-LTR circles quantification in HIV-infected patients proved to be more accurate with a modified plasmid DNA isolation procedure compared to total genomic DNA isolation. This method enables the processing of more blood cells, thus enhancing quantification accuracy and sensitivity. An improved quantification of 2-LTR circles will contribute to the better understanding of ongoing replication in the HIV reservoir of patients on cART.
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spelling pubmed-42253652014-11-13 Accurate episomal HIV 2-LTR circles quantification using optimized DNA isolation and droplet digital PCR Malatinkova, Eva Kiselinova, Maja Bonczkowski, Pawel Trypsteen, Wim Messiaen, Peter Vermeire, Jolien Verhasselt, Bruno Vervisch, Karen Vandekerckhove, Linos De Spiegelaere, Ward J Int AIDS Soc Poster Sessions – Abstract P142 INTRODUCTION: In HIV-infected patients on combination antiretroviral therapy (cART), the detection of episomal HIV 2-LTR circles is a potential marker for ongoing viral replication. Quantification of 2-LTR circles is based on quantitative PCR or more recently on digital PCR assessment, but is hampered due to its low abundance. Sample pre-PCR processing is a critical step for 2-LTR circles quantification, which has not yet been sufficiently evaluated in patient derived samples. MATERIALS AND METHODS: We compared two sample processing procedures to more accurately quantify 2-LTR circles using droplet digital PCR (ddPCR). Episomal HIV 2-LTR circles were either isolated by genomic DNA isolation or by a modified plasmid DNA isolation, to separate the small episomal circular DNA from chromosomal DNA. This was performed in a dilution series of HIV-infected cells and HIV-1 infected patient derived samples (n=59). Samples for the plasmid DNA isolation method were spiked with an internal control plasmid. RESULTS: Genomic DNA isolation enables robust 2-LTR circles quantification. However, in the lower ranges of detection, PCR inhibition caused by high genomic DNA load substantially limits the amount of sample input and this impacts sensitivity and accuracy. Moreover, total genomic DNA isolation resulted in a lower recovery of 2-LTR templates per isolate, further reducing its sensitivity. The modified plasmid DNA isolation with a spiked reference for normalization was more accurate in these low ranges compared to genomic DNA isolation. A linear correlation of both methods was observed in the dilution series (R2=0.974) and in the patient derived samples with 2-LTR numbers above 10 copies per million peripheral blood mononuclear cells (PBMCs), (R2=0.671). Furthermore, Bland–Altman analysis revealed an average agreement between the methods within the 27 samples in which 2-LTR circles were detectable with both methods (bias: 0.3875±1.2657 log(10)). CONCLUSIONS: 2-LTR circles quantification in HIV-infected patients proved to be more accurate with a modified plasmid DNA isolation procedure compared to total genomic DNA isolation. This method enables the processing of more blood cells, thus enhancing quantification accuracy and sensitivity. An improved quantification of 2-LTR circles will contribute to the better understanding of ongoing replication in the HIV reservoir of patients on cART. International AIDS Society 2014-11-02 /pmc/articles/PMC4225365/ /pubmed/25397424 http://dx.doi.org/10.7448/IAS.17.4.19674 Text en © 2014 Malatinkova E et al; licensee International AIDS Society http://creativecommons.org/licenses/by/3.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Poster Sessions – Abstract P142
Malatinkova, Eva
Kiselinova, Maja
Bonczkowski, Pawel
Trypsteen, Wim
Messiaen, Peter
Vermeire, Jolien
Verhasselt, Bruno
Vervisch, Karen
Vandekerckhove, Linos
De Spiegelaere, Ward
Accurate episomal HIV 2-LTR circles quantification using optimized DNA isolation and droplet digital PCR
title Accurate episomal HIV 2-LTR circles quantification using optimized DNA isolation and droplet digital PCR
title_full Accurate episomal HIV 2-LTR circles quantification using optimized DNA isolation and droplet digital PCR
title_fullStr Accurate episomal HIV 2-LTR circles quantification using optimized DNA isolation and droplet digital PCR
title_full_unstemmed Accurate episomal HIV 2-LTR circles quantification using optimized DNA isolation and droplet digital PCR
title_short Accurate episomal HIV 2-LTR circles quantification using optimized DNA isolation and droplet digital PCR
title_sort accurate episomal hiv 2-ltr circles quantification using optimized dna isolation and droplet digital pcr
topic Poster Sessions – Abstract P142
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4225365/
https://www.ncbi.nlm.nih.gov/pubmed/25397424
http://dx.doi.org/10.7448/IAS.17.4.19674
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