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Dried Blood Spots Versus Plasma for the Quantification of HIV-1 RNA Using the Manual (PCR-ELISA) Amplicor Monitor HIV-1 Version 1.5 Assay in Yaounde, Cameroon

Objectives: Considering the recent accrued need for viral load quantification in resource-limited settings, this study evaluated the use of dried blood spots (DBS) compared to plasma as a means of sample collection and storage for HIV-1 RNA quantification using a non-automated assay. Methods: Venous...

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Published in:Journal of the International Association of Physicians in AIDS Care (Chicago, Ill. : 2002) Ill. : 2002), 2009-05, Vol.8 (3), p.181-184
Main Authors: Ikomey, G.M., Atashili, J., Okomo-Assoumou, M.C., Mesembe, M., Ndumbe, P.M.
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container_title Journal of the International Association of Physicians in AIDS Care (Chicago, Ill. : 2002)
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creator Ikomey, G.M.
Atashili, J.
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Mesembe, M.
Ndumbe, P.M.
description Objectives: Considering the recent accrued need for viral load quantification in resource-limited settings, this study evaluated the use of dried blood spots (DBS) compared to plasma as a means of sample collection and storage for HIV-1 RNA quantification using a non-automated assay. Methods: Venous blood was collected from 60 consenting HIV-1-positive patients, plasma separated within 4 hours, and stored at -20°C. Venous blood, 50 μL, was blotted on 4 designated areas of Whatman filter paper and air-dried at room temperature for 2 hours. Results: There was a strong statistically significant correlation between HIV-1 RNA viral load using plasma and DBS (r = .955, P < .001). On average plasma viral loads were only slightly higher than DBS viral loads (mean difference: 0.06 log10 copies/mL). Conclusion: Even when using an entirely manual HIV-quantification assay, DBS may provide a reliable, cost-effective method for sample collection and storage for HIV-1 RNA quantification in resource-limited settings.
doi_str_mv 10.1177/1545109709333111
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Methods: Venous blood was collected from 60 consenting HIV-1-positive patients, plasma separated within 4 hours, and stored at -20°C. Venous blood, 50 μL, was blotted on 4 designated areas of Whatman filter paper and air-dried at room temperature for 2 hours. Results: There was a strong statistically significant correlation between HIV-1 RNA viral load using plasma and DBS (r = .955, P &lt; .001). On average plasma viral loads were only slightly higher than DBS viral loads (mean difference: 0.06 log10 copies/mL). 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subjects Adolescent
Adult
Blood
Blood - virology
Cameroon
Enzyme-Linked Immunosorbent Assay
Female
HIV
HIV Infections - blood
HIV Infections - virology
HIV-1 - genetics
HIV-1 - isolation & purification
Human immunodeficiency virus
Human immunodeficiency virus 1
Humans
Male
Middle Aged
Plasma - virology
Polymerase Chain Reaction
RNA, Viral - blood
Specimen Handling - methods
Viral Load - methods
Young Adult
title Dried Blood Spots Versus Plasma for the Quantification of HIV-1 RNA Using the Manual (PCR-ELISA) Amplicor Monitor HIV-1 Version 1.5 Assay in Yaounde, Cameroon
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