Prospective evaluation of accuracy of HIV viral load monitoring using the Aptima HIV Quant Dx assay with fingerstick and venous dried blood spots prepared under field conditions in Kenya

Mwau, Matilu; Danda, Jeff; Mbugua, Joseph; Handa, Allan; Fortunko, Jacqueline; Worlock, Andrew; Nair, Sangeetha Vijaysri

doi:10.1371/journal.pone.0249376

Cited by 8 publications

(10 citation statements)

References 29 publications

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“…Although only venous DBS were tested in this study, we previously compared the recovery of HIV-1 from venous DBS, fingerstick DBS, and plasma with the Aptima test [ 23 ] showing good agreement between plasma, venous DBS, and fingerstick DBS. One limitation of the current study is that no replicate testing or retesting of invalid specimens was performed due to volume limitation for these clinical samples.…”

Section: Discussionmentioning

confidence: 99%

“…In a previous study [ 23 ], we investigated the performance of the Aptima HIV Quant Dx assay using fingerstick and venous dried blood spots prepared under field conditions. In that study, we did not compare HIV-1 VL in Aptima with those in other assays using DBS.…”

Section: Introductionmentioning

confidence: 99%

“…Instead it was compared to the Aptima plasma HIV-1 VL. In fact, whereas multiple studies compared VL results of paired DBS and plasma samples at the medical decision point of 1000 copies/ mL by testing both sample types in Aptima [23][24][25][26], there is no published information comparing the performance of DBS specimens tested in Aptima and other assays at the medical decision point (MDP) of 1000 copies/mL.…”

Section: Introductionmentioning

confidence: 99%

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Comparison of the performance of Aptima HIV-1 Quant Dx Assay with Abbott RealTime HIV Assay for viral load monitoring using plasma and Dried Blood Spots collected in Kenya

Mwau

Schaffer²,

Kimani³

et al. 2022

PLoS ONE

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Introduction HIV-1 viral Load (VL) testing is recommended for the monitoring of antiretroviral treatment. Dried Blood Spots (DBS) are an effective sample type in resource limited settings, where safe phlebotomy and reliable shipping are hard to guarantee. In HIV high burden countries, high throughput assays can improve access to testing services. The Hologic Aptima HIV-1 Quant Dx Assay (Aptima Assay) is a high throughput assay that runs on the CE-IVD approved Panther platform. The objectives of this study were to assess the performance characteristics of Aptima for VL monitoring using plasma and venous DBS specimens and to determine the stability of HIV-1 RNA in DBS. Materials and methods This was a cross-sectional study of 2227 HIV infected adults visiting health facilities in Nairobi and Busia, Kenya. Each provided a venous blood sample; plasma was prepared from 1312 samples while paired DBS samples and plasma were prepared from the remaining 915 samples. The agreement between the Aptima assay and the Abbott RealTime HIV-1 Assay (Abbott RT) was analysed by comparing the HIV-1 VL in both assays at the medical decision point of 1000 copies/mL. To assess stability of HIV-1 RNA in DBS, VL in DBS spotted on day 0 were compared with that from the same DBS card after 21 days of storage at room temperature. Results Overall, 436 plasma samples had quantifiable results in both Aptima and Abbott RT. The agreement between the two assays at 1000 copies/mL was 97.48% with a Pearson’s correlation coefficient (r) of 0.9589 and gave a mean bias of 0.33 log copies/mL on Bland-Altman analysis. For fresh DBS, the agreement in both assays was 94.64% at 1000 copies/mL, with an r of 0.8692 and a mean bias of 0.35 log copies/mL. The overall agreement between DBS tested in Aptima on day 0 versus day 21 was 95.71%, with a mean bias of -0.154. Conclusion The Aptima HIV-1 Quant Dx assay is an accurate test for VL monitoring of HIV-1 using DBS and plasma sample types in Kenya.

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Comparison of the performance of Aptima HIV-1 Quant Dx Assay with Abbott RealTime HIV Assay for viral load monitoring using plasma and Dried Blood Spots collected in Kenya

Mwau

Schaffer²,

Kimani³

et al. 2022

PLoS ONE

Self Cite

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“…Most viral load testing in LMICs is done in centralized public laboratories using expensive, government owned platforms requiring high maintenance costs, highly skilled labour, and long test turnaround times. Widely used commercial VL assays include the Real-time HIV-1 (Abbott Molecular, USA); the COBAS® AmpliPrep/COBAS® TaqMan® HIV-1 Test, v2.0 (Roche Molecular Diagnostics, Basel, Switzerland) 15 ; and the Hologic Aptima® HIV-1 Quant Dx Assay on the Panther platform 15 , 16 . The high cost of the assays (up to $100 per test) coupled with the logistics of cold-chain transport of reagents and samples to centralized testing laboratories continues to limit the accessibility of VL testing in resource-constrained settings (RCS) 9 .…”

Section: Introductionmentioning

confidence: 99%

Use of laboratory-developed assays in global HIV-1 treatment-monitoring and research

Malisa

Manak²,

Michelo³

et al. 2023

Sci Rep

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There has been a surge in the emergence of HIV-1 drug resistance in Low and Middle-Income Countries (LMICs) due to poor drug-adherence and limited access to viral load testing, the current standard for treatment-monitoring. It is estimated that only 75% of people living with HIV (PLWH) worldwide have access to viral load testing. In LMICs, this figure is below 50%. In a recent WHO survey in mostly LMICs, 21 out of 30 countries surveyed found HIV-1 first-line pre-treatment drug resistance in over 10% of study participants. In the worst-affected regions, up to 68% of infants born to HIV-1 positive mothers were found to harbour first-line HIV-1 treatment resistance. This is a huge public health concern. Greater access to treatment-monitoring is required in LMICs if the UNAIDS “third 95” targets are to be achieved by 2030. Here, we review the current challenges of viral load testing and present the case for greater utilization of Laboratory-based assays that quantify intracellular HIV-1 RNA and/or DNA to provide broader worldwide access to HIV-1 surveillance, drug-resistance monitoring, and cure-research.

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“…Выяснено, что провоцирующими этиологическими факторами развития некротизирующих заболеваний пародонта являются курение, наличие грибов видов Candida, неправильное питание и отсутствие гигиены полости рта [66]. Вышеперечисленными факторами ряд авторов объяснил развитие ЯНГ у пациентов без тяжелого иммунодефицита [68][69][70].…”

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Oral manifestations of HIV-infection in patients based on CD4+ T-lymphocyte counts

Lyogkih,

Gaisina,

Dobrinskaya

et al. 2023

Humans and their Health

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Objective - analysis and generalization of the available data on the manifestations of human immunodeficiency virus in the oral cavity depending on the number of CD4+ T-lymphocytes in the blood. Materials and methods. A search of clinical studies, systematic reviews, and online meta-analyses was conducted from 2004-2023 in the PubMed, Elsiever, Scopus, Cochrane, and Elibrary databases, which described oral manifestations of HIV infection as a function of CD4+ T-lymphocyte count. Results. Pseudomembranous candidiasis, hairy leukoplakia, Kaposi's sarcoma, and non-Hodgkin's lymphoma develop against a background of severe immunodeficiency when the CD4+ T-lymphocyte count is <200 cells/μL blood. Kaposi's sarcoma also develops in people with a high CD8+ T-lymphocyte count (>1000 cells/μL of blood) or with a low CD4+ to CD8+ ratio (CD4+:CD8+ ≤0.5). Non-Hodgkin's lymphoma develops not only with CD4+ T-cells <200/μL, but also with a high number of CD8+ T-cells (≥2000 cells/μL of blood). Specific periodontal disease develops with moderate to severe immunodeficiency (CD4+ T-cells 200-500 cells/μL of blood). Necrotic ulcerative gingivitis is more often seen in severe immunodeficiency (CD4+ T-lymphocytes <200 cells/μL). Conclusion. The development of pseudomembranous candidiasis (p<0,05), "hairy" leukoplakia (p<0,01), Kaposi sarcoma (p<0,0001) statistically significantly correlates with CD4+ T-lymphocyte count <200 cells/μl blood. In addition, the development of Kaposi's sarcoma, in addition to the low number of CD4+ T-cells, is affected by a high number of CD8+ cytotoxic lymphocytes >1000 cells/μL (p=0.0003) and a low CD4+:CD8+ ratio ≤0.5 (p<0.0003), which is statistically significant.

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Prospective evaluation of accuracy of HIV viral load monitoring using the Aptima HIV Quant Dx assay with fingerstick and venous dried blood spots prepared under field conditions in Kenya

Cited by 8 publications

References 29 publications

Comparison of the performance of Aptima HIV-1 Quant Dx Assay with Abbott RealTime HIV Assay for viral load monitoring using plasma and Dried Blood Spots collected in Kenya

Comparison of the performance of Aptima HIV-1 Quant Dx Assay with Abbott RealTime HIV Assay for viral load monitoring using plasma and Dried Blood Spots collected in Kenya

Use of laboratory-developed assays in global HIV-1 treatment-monitoring and research

Oral manifestations of HIV-infection in patients based on CD4+ T-lymphocyte counts

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