Development and Application of a Broadly Sensitive Dried-Blood-Spot-Based Genotyping Assay for Global Surveillance of HIV-1 Drug Resistance

Author:

Yang Chunfu1,McNulty Amanda1,Diallo Karidia1,Zhang Jing12,Titanji Boghuma3,Kassim Sidibe1,Wadonda-Kabondo Nellie4,Aberle-Grasse John5,Kibuka Tabitha6,Ndumbe Peter M.3,Vedapuri Shanmugam1,Zhou Zhiyong1,Chilima Benson4,Nkengasong John N.1

Affiliation:

1. Division of Global AIDS, NCHHSTP, Centers for Disease Control and Prevention, Atlanta, Georgia

2. Institute of AIDS/HIV Control and Prevention, Shandong Center for Disease Control and Prevention, Shandong, China

3. Center for the Study and Control of Communicable Diseases (CSCCD), University of Yaounde, Yaounde, Cameroon

4. Community Health Sciences Unit, Malawi Ministry of Health

5. CDC/GAP, Lilongwe, Malawi

6. CDC/GAP, Dar es Salaam, Tanzania

Abstract

ABSTRACT As antiretroviral therapy (ART) is scaled up in resource-limited countries, surveillance for HIV drug resistance (DR) is vital to ensure sustained effectiveness of first-line ART. We have developed and applied a broadly sensitive dried-blood-spot (DBS)-based genotyping assay for surveillance of HIV-1 DR in international settings. In 2005 and 2006, 171 DBS samples were collected under field conditions from newly diagnosed HIV-1-infected individuals from Malawi ( n = 58), Tanzania ( n = 60), and China ( n =53). In addition, 30 DBS and 40 plasma specimens collected from ART patients in China and Cameroon, respectively, were also tested. Of the 171 DBS analyzed at the protease and RT regions, 149 (87.1%) could be genotyped, including 49 (81.7%) from Tanzania, 47 (88.7%) from China, and 53 (91.4%) from Malawi. Among the 70 ART patient samples analyzed, 100% (30/30) of the Chinese DBS and 90% (36/40) of the Cameroonian plasma specimens were genotyped, including 8 samples with a viral load of <400 copies/ml. The results of phylogenetic analyses indicated that the subtype, circulating recombinant form (CRF), and unique recombinant form (URF) distribution was as follows: 73 strains were subtype C (34%), 37 were subtype B (17.2%), 24 each were CRF01_AE or CRF02_AG (11.2% each), 22 were subtype A1 (10.2%), and 9 were unclassifiable (UC) (4.2%). The remaining samples were minor strains comprised of 6 that were CRF07_BC (2.8%), 5 that were CRF10_CD (2.3%), 3 each that were URF_A1C and CRF08_BC (1.4%), 2 each that were G, URF_BC, and URF_D/UC (0.9%), and 1 each that were subtype F1, subtype F2, and URF_A1D (0.5%). Our results indicate that this broadly sensitive genotyping assay can be used to genotype DBS collected from areas with diverse HIV-1 group M subtypes and CRFs. Thus, the assay is likely to become a useful screening tool in the global resistance surveillance and monitoring of HIV-1 where multiple subtypes and CRFs are found.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

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