Single genome amplification of proviral HIV-1 DNA from dried blood spot specimens collected during early infant screening programs in Lusaka, Zambia

Seu, Lillian; Mwape, Innocent; Guffey, M. Brad

doi:10.1016/j.jviromet.2014.03.001

Cited by 5 publications

(6 citation statements)

References 21 publications

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“…This observation is consistent with findings by others with DBS [9,17,19,21,23]. A possible and most advanced explanation of this repeated finding could be the contribution of intracellular HIV-1 DNA and RNA which is present in the DBS but not in the plasma counterpart [26,27]. Vidya et al [18] suggested that the contribution of intracellular HIV-1 DNA and RNA could be more relevant to specimens with low or undetectable levels viremia than to specimens containing higher levels of extracellular HIV-1 RNA.…”

Section: Discussionsupporting

confidence: 91%

Whatman FTA^®cards versus plasma specimens for the quantitation of HIV-1 RNA using two Real-Time PCR assays

Yacouba

Congo

Dioma

et al. 2019

Preprint

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267 words 1 8 Abstract 2 3Background: Several studies have been conducted to compare the use DBS as 2 4 alternative to plasma specimens, but mainly using Whatman 903 ® cards as filter 2 5paper. The aim of this study was to evaluate Whatman FTA ® cards (FTA cards) 2 6 specimens for HIV-1 viral load testing by comparing it to plasma specimens, using 2 2 7 real-Time PCR assays. 2 8 Methodology: A cross-sectional study was conducted between April 2017 and 2 9 September 2017, in HIV-1 patients admitted at Yalgado Ouédraogo teaching 3 0 hospital. Paired FTA cards and plasma specimens were collected and analyzed 3 1 using Abbott RealTime HIV-1 assay (Abbott) and COBAS ® AmpliPrep/COBAS ® 3 2TaqMan v2.0 (Roche), following manufacturers' protocol. 3 3 Results: A total of 107 patients were included. No Statistical differences (p-value > 3 4 0.05) were observed between the mean viral loads obtained from FTA cards and 3 5 plasma specimens with Roche and Abbott assays. Twenty-nine samples with Roche 3 6 and 15 samples with Abbott assay showed discrepant results. At viral loads of ≤ 1000 3 7 copies/mL, the sensitivity and specificity of FTA cards were 78.6%, and 100% with 3 8 Roche, and 92.3% and 95.9% with Abbott. Strong correlation was found between 3 9 FTA cards and plasma specimens with both assays. With Roche, Bland-Altman 4 0 analysis showed bias of -0.3 and 95% limits of agreement of -2.6 to 1.8 log10, with 4 1 97/99 cases (97.9%) within agreement limits. With Abbott, Bland-Altman analysis 4 2showed bias of -0.1 and 95% limits of agreement of -2.3 to 2.1 log10, with 96/99 4 3 cases (96.9%) within agreement limits. 4Conclusion: Our study demonstrated the feasibility of using FTA cards filter paper 4 5

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Section: Discussionsupporting

confidence: 91%

Whatman FTA^®cards versus plasma specimens for the quantitation of HIV-1 RNA using two Real-Time PCR assays

Yacouba

Congo

Dioma

et al. 2019

Preprint

View full text Add to dashboard Cite

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“…This observation is consistent with the findings reported by other research groups in terms of DBS [9, 17, 20, 22, 24]. The most advanced explanation of this repeated finding could be the contribution of intracellular HIV-1 DNA and RNA, which is present in the DBS but not in the plasma counterpart [27, 28]. Vidya et al .…”

Section: Discussionsupporting

confidence: 91%

Whatman FTA cards versus plasma specimens for the quantitation of HIV-1 RNA using two real-time PCR assays

Yacouba

Congo

Dioma

et al. 2020

Access Microbiology

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Background. Several studies have compared the use of dried blot spot (DBS) as an alternative to plasma specimens, mainly using Whatman 903 cards as filter paper. The aim of this study was to evaluate the use of Whatman FTA card (FTA card) specimens for HIV-1 viral load testing compared to plasma specimens using two real-time PCR assays manufactured by Roche and Abbott. Methodology. A cross-sectional study was conducted between April 2017 and September 2017 on HIV-1 patients admitted to Yalgado Ouédraogo Teaching Hospital. Paired FTA cards and plasma specimens were collected and analysed using the Abbott Real-Time HIV-1 assay (Abbott) and COBAS AmpliPrep/COBAS TaqMan v2.0 (Roche). Results. In total, 107 patients were included. No statistical differences (P>0.05) were observed between the mean viral loads obtained from the FTA cards and those of the plasma specimens using the Roche and Abbott assays. In total, 29 samples with Roche and 15 samples with Abbott assay showed discrepant results. At viral loads of ≤1000 copies ml−1, the sensitivity and specificity of the FTA cards were 78.6 and 100% with Roche, and 92.3 and 95.9% with Abbott, respectively. Both the Roche and Abbott assays showed good correlation and agreement between the FTA cards and plasma values. Conclusion. Our study demonstrates the feasibility of using FTA card filter paper for HIV-1 viral load testing. However, further studies will be required for the validation of the use of FTA card filter paper in HIV-1 treatment monitoring.

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“…At the completion of the cDNA synthesis, the remaining RNA was treated with RNaseOUT (Invitrogen Corp., Life Technologies), and the synthesis mixture was purified using a GeneJet DNA (Thermo Scientific Corporation, Waltham, MA) purification kit. A nested PCR reaction was performed on the cDNA eluate using Platinum Taq DNA polymerase (Invitrogen Corporation, Life Technologies) according to previously published amplification methods (Seu et al, ): a 1,200 bp sequence was first amplified using forward primer (CWF: 5′‐GAAGGACACCAAATGAAAGAYTG‐3′; HXB2 nucleotide position 2,044–2,066) and reverse primer (LSR1: 5′‐ACTGTTTTACATCATTAGTGTGGG ‐3′; HXB2 nucleotide position 3,651–3,628) and a second round PCR amplification using a forward primer (LSF1: 5′‐TCAGAGCAGACCAGAGCCAACAGCCCCA‐3′; HXB2 nt position 2,136–2,163) and reverse primer (Rev7: 5′‐ATCCCTGGGTAAATCTGACTTGCCCA‐3′; HXB2 position 3,370–3,345). Amplicons were directly analyzed via population‐based Sanger Sequencing using BigDye Terminator chemistry and protocols recommended by the manufacturer (Applied Biosystems, Foster City, CA), and sequencing reaction products were analyzed with an ABI 3130XL genetic analyzer (Applied Biosystems).…”

Section: Methodsmentioning

confidence: 99%

Characterization of HIV drug resistance mutations among patients failing first-line antiretroviral therapy from a tertiary referral center in Lusaka, Zambia

et al. 2015

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In settings of resource constraint, an understanding of HIV drug resistance can guide antiretroviral therapy (ART) at switch to second-line therapy. To determine the prevalence of such HIV drug resistance mutations (HIV DRM), we used an in-house sequencing assay in the pol gene (protease and partial reverse transcriptase) in a cohort of patients suspected of failing a first-line regimen, which in Zambia comprises two nucleoside/nucleotide reverse transcriptase inhibitors (NRTIs) and one non-nucleoside reverse transcriptase inhibitor (NNRTI). Our analysis cohort (n=68) was referred to the University Teaching Hospital in Lusaka from November 2009 to October 2012. Median duration on first-line ART to suspected treatment failure was 3.2 years (IQR 1.7–4.7 years). The majority of patients (95%) harbored HIV-1 subtype C virus. Analysis of reverse transcriptase revealed M184V (88%), K103N/S (32%), and Y181C/I/V (41%) DRMs, with the latter conferring reduced susceptibility to the salvage therapy candidates etravirine and rilpivirine. Three patients (5%) had major protease inhibitor (PI) resistance mutations: all three had the V82A mutation, and one patient (Clade J virus) had a concurrent M46I, Q58E, and L76V DRM. HIV-1 genotyping revealed major and minor DRMs as well as high levels of polymorphisms in subtype C isolates from patients failing first-line antiretroviral therapy. Closer monitoring of DRM mutations at first-line failure can inform clinicians about future options for salvage therapy.

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Single genome amplification of proviral HIV-1 DNA from dried blood spot specimens collected during early infant screening programs in Lusaka, Zambia

Cited by 5 publications

References 21 publications

Whatman FTA^®cards versus plasma specimens for the quantitation of HIV-1 RNA using two Real-Time PCR assays

Whatman FTA^®cards versus plasma specimens for the quantitation of HIV-1 RNA using two Real-Time PCR assays

Whatman FTA cards versus plasma specimens for the quantitation of HIV-1 RNA using two real-time PCR assays

Characterization of HIV drug resistance mutations among patients failing first-line antiretroviral therapy from a tertiary referral center in Lusaka, Zambia

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Single genome amplification of proviral HIV-1 DNA from dried blood spot specimens collected during early infant screening programs in Lusaka, Zambia

Cited by 5 publications

References 21 publications

Whatman FTA®cards versus plasma specimens for the quantitation of HIV-1 RNA using two Real-Time PCR assays

Whatman FTA®cards versus plasma specimens for the quantitation of HIV-1 RNA using two Real-Time PCR assays

Whatman FTA cards versus plasma specimens for the quantitation of HIV-1 RNA using two real-time PCR assays

Characterization of HIV drug resistance mutations among patients failing first-line antiretroviral therapy from a tertiary referral center in Lusaka, Zambia

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Product

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Whatman FTA^®cards versus plasma specimens for the quantitation of HIV-1 RNA using two Real-Time PCR assays

Whatman FTA^®cards versus plasma specimens for the quantitation of HIV-1 RNA using two Real-Time PCR assays