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Journal of Clinical Microbiology, April 1998, p. 1056-1063, Vol. 36, No. 4
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Comparison of Culture- and Non-Culture-Based Methods for Quantification of Viral Load and Resistance to Antiretroviral Drugs in Patients Given Zidovudine Monotherapy

Richard S. Tedder,1 Steve Kaye,1,* Clive Loveday,2 Ian V. D. Weller,3 Don Jeffries,4 Jane Norman,4 Jonathan Weber,5 Michel Bourelly,5 Russell Foxall,5 Abdel Babiker,6 and Janet H. Darbyshire6

Department of Virology, University College London Medical School, London W1P 6DB,1 Department of Retrovirology, Royal Free Hospital School of Medicine, London NW3 2PF,2 Department of STDs, University College London Medical School, London WC1E 6AU,3 Department of Virology, St. Bartholomew's Hospital, London EC1A 7BE,4 Department of Genitourinary Medicine and Communicable Diseases, Imperial College London School of Medicine at St. Mary's, London W2 1NY,5 and Medical Research Council HIV Clinical Trials Centre, UCL Medical School, The Mortimer Market Centre, London WC1E 6AU,6 United Kingdom

Received 3 November 1997/Returned for modification 9 December 1997/Accepted 29 December 1997

Virological assays for human immunodeficiency virus type 1 load and drug resistance can broadly be divided into culture-based and molecular biology-based methods. Culture-based methods give a direct measure of infectious virus load and phenotypic drug resistance, whereas molecular biology-based methods are indirect, assaying nucleic acid levels to determine virus load and point mutations associated with drug resistance. We have compared culture-based and non-culture-based methods for patients enrolled in a placebo-controlled trial of zidovudine (the Concorde Trial). Virus loads were assayed by culture of peripheral blood mononuclear cells (PBMCs) or quantitative PCR, and drug resistance was assayed in culture or in a quantitative, PCR-based point mutation assay. The rates of detection of viremia and drug resistance were higher by PCR than by culture for this population of subjects. Comparison of the virus loads by the two measures showed a good correlation for virus loads in PBMCs but a poor correlation for virus loads in plasma. The latter result probably reflected the inaccuracies of culture in assaying plasma with the low infectious virus titers seen in the study population. The concordance of phenotypic and genotypic drug resistance methods was high, with all phenotypically resistant isolates having at least one resistance-associated mutation and with no mutations being found in a drug-sensitive isolate. Genomic resistance scores (weighted sums of levels of resistance mutations) showed good correlations with the levels of phenotypic resistance, and both resistance measures were observed to increase as the duration of exposure to drug increased. Overall, non-culture-based methods were shown to correlate well with culture-based methods and offer a low-cost, high-throughput alternative. However, culture-based methods remain the final arbiters of infectious virus load and phenotypic drug resistance and are unlikely to be superseded entirely.


* Corresponding author. Mailing address: Department of Virology, University College London Medical School, Windeyer Building, 46 Cleveland St., London W1P 6DB, United Kingdom. Phone: 0171-380-9490. Fax: 0171-580-5896. E-mail: s.kaye{at}ucl.ac.uk.


Journal of Clinical Microbiology, April 1998, p. 1056-1063, Vol. 36, No. 4
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.



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