An International Collaboration To Standardize HIV-2 Viral Load Assays: Results from the 2009 ACHI E V 2E Quality Control Study

Author:

Damond F.1,Benard A.2,Balotta Claudia3,Böni Jürg4,Cotten Matthew5,Duque Vitor6,Ferns Bridget7,Garson Jeremy7,Gomes Perpetua89,Gonçalves Fátima8,Gottlieb Geoffrey10,Kupfer Bernd11,Ruelle Jean12,Rodes Berta13,Soriano Vicente13,Wainberg Mark14,Taieb Audrey2,Matheron Sophie1516,Chene Genevieve2,Brun-Vezinet Francoise116,

Affiliation:

1. APHP, Hôpital Bichat-Claude Bernard, Laboratoire de Virologie, Paris F-75018, France

2. INSERM, U593, ISPED, Université Victor Segalen, Bordeaux, France

3. Laboratory of Department of Clinical Sciences, Section of Infectious Diseases and Immunopathology, L. Sacco Hospital, University of Milan, Milan, Italy

4. National Centre for Retroviruses, Institute of Medical Virology, University of Zürich, Zurich, Switzerland

5. Medical Research Council Laboratories, Fajara, the Gambia

6. Laboratório de Virologia, Departamento de Doenças Infecciosas, Hospitais da Universidade de Coimbra, Coimbra, Portugal

7. Centre for Virology, Research Department of Infection, UCL Medical School, London, United Kingdom

8. Laboratório de Biologia Molecular, CHLO-Hospital Egas Moniz, Lisbon, Portugal

9. Instituto Superior de Saúde Egas Moniz, Quinta da Granja, Monte de Caparica, Portugal

10. Division of Allergy and Infectious Diseases, University of Washington School of Medicine, Seattle, Washington

11. Institute of Virology, Bonn, Germany

12. AIDS Reference Laboratory, Université Catholique de Louvain, Louvain, Belgium

13. Department of Infectious Diseases, Hospital Carlos III, Madrid, Spain

14. McGill University AIDS Centre, Lady Davis Institute for Medical Research, Jewish General Hospital, Montreal, Quebec, Canada

15. APHP, Hôpital Bichat-Claude Bernard, Service de Maladies Infectieuses et Tropicales, Paris, France

16. Faculté de Médecine Denis Diderot, Paris 7 University, Paris, France

Abstract

ABSTRACT Accurate HIV-2 plasma viral load quantification is crucial for adequate HIV-2 patient management and for the proper conduct of clinical trials and international cohort collaborations. This study compared the homogeneity of HIV-2 RNA quantification when using HIV-2 assays from ACHI E V 2E study sites and either in-house PCR calibration standards or common viral load standards supplied to all collaborators. Each of the 12 participating laboratories quantified blinded HIV-2 samples, using its own HIV-2 viral load assay and standard as well as centrally validated and distributed common HIV-2 group A and B standards ( http://www.hiv.lanl.gov/content/sequence/HelpDocs/subtypes-more.html ). Aliquots of HIV-2 group A and B strains, each at 2 theoretical concentrations (2.7 and 3.7 log 10 copies/ml), were tested. Intralaboratory, interlaboratory, and overall variances of quantification results obtained with both standards were compared using F tests. For HIV-2 group A quantifications, overall and interlaboratory and/or intralaboratory variances were significantly lower when using the common standard than when using in-house standards at the concentration levels of 2.7 log 10 copies/ml and 3.7 log 10 copies/ml, respectively. For HIV-2 group B, a high heterogeneity was observed and the variances did not differ according to the type of standard used. In this international collaboration, the use of a common standard improved the homogeneity of HIV-2 group A RNA quantification only. The diversity of HIV-2 group B, particularly in PCR primer-binding regions, may explain the heterogeneity in quantification of this strain. Development of a validated HIV-2 viral load assay that accurately quantifies distinct circulating strains is needed.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

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