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Virology

Nonisotopic Detection and Typing of Human Papillomavirus DNA in Genital Samples by the Line Blot Assay

François Coutlée, Patti Gravitt, Harriet Richardson, Catherine Hankins, Eduardo Franco, Normand Lapointe, Hélène Voyer, The Canadian Women’s HIV Study Group‡
François Coutlée
Départements de Microbiologie-Immunologie et de Pédiatrie, Université de Montréal,
Centre de Recherche et Département de Microbiologie et Infectiologie, Centre Hospitalier de l’Université de Montréal, Campus Notre-Dame,
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Patti Gravitt
Roche Molecular Systems, Alameda, California
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Harriet Richardson
Department of Epidemiology and Biostatistics, McGill University, and
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Catherine Hankins
Department of Epidemiology and Biostatistics, McGill University, and
Unité de Maladies Infectieuses, Direction de la Santé Publique de Montréal-Centre,
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Eduardo Franco
Department of Epidemiology and Biostatistics, McGill University, and
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Normand Lapointe
Départements de Microbiologie-Immunologie et de Pédiatrie, Université de Montréal,
Centre Maternel et Infantile sur le SIDA, Centre de Recherche de l’Hôpital Sainte-Justine, Hôpital Sainte-Justine,Montréal, Québec, Canada, and
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Hélène Voyer
Centre de Recherche et Département de Microbiologie et Infectiologie, Centre Hospitalier de l’Université de Montréal, Campus Notre-Dame,
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‡
DOI: 10.1128/JCM.37.6.1852-1857.1999
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ABSTRACT

The line blot assay, a gene amplification method that combines PCR with nonisotopic detection of amplified DNA, was evaluated for its ability to detect human papillomavirus (HPV) DNA in genital specimens. Processed samples were amplified with biotin-labeled primers for HPV detection (primers MY09, MY11, and HMB01) and for β-globin detection (primers PC03 and PC04). Amplified DNA products were hybridized by a reverse blot method with oligonucleotide probe mixtures fixed on a strip that allowed the identification of 27 HPV genotypes. The line blot assay was compared to a standard consensus PCR test in which HPV amplicons were detected with radiolabeled probes in a dot blot assay. Two hundred fifty-five cervicovaginal lavage specimens and cervical scrapings were tested in parallel by both PCR tests. The line blot assay consistently detected 25 copies of HPV type 18 per run. The overall positivity for the DNA of HPV types detectable by both methods was 37.7% (96 of 255 samples) by the line blot assay, whereas it was 43.5% (111 of 255 samples) by the standard consensus PCR assay. The sensitivity and specificity of the line blot assay reached 84.7% (94 of 111 samples) and 98.6% (142 of 144 samples), respectively. The agreement for HPV typing between the two PCR assays reached 83.9% (214 of 255 samples). Of the 37 samples with discrepant results, 33 (89%) were resolved by avoiding coamplification of β-globin and modifying the amplification parameters. With these modifications, the line blot assay compared favorably to an assay that used radiolabeled probes. Its convenience allows the faster analysis of samples for large-scale epidemiological studies. Also, the increased probe spectrum in this single hybridization assay permits more complete type discrimination.

  • Copyright © 1999 American Society for Microbiology
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Nonisotopic Detection and Typing of Human Papillomavirus DNA in Genital Samples by the Line Blot Assay
François Coutlée, Patti Gravitt, Harriet Richardson, Catherine Hankins, Eduardo Franco, Normand Lapointe, Hélène Voyer, The Canadian Women’s HIV Study Group‡
Journal of Clinical Microbiology Jun 1999, 37 (6) 1852-1857; DOI: 10.1128/JCM.37.6.1852-1857.1999

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Nonisotopic Detection and Typing of Human Papillomavirus DNA in Genital Samples by the Line Blot Assay
François Coutlée, Patti Gravitt, Harriet Richardson, Catherine Hankins, Eduardo Franco, Normand Lapointe, Hélène Voyer, The Canadian Women’s HIV Study Group‡
Journal of Clinical Microbiology Jun 1999, 37 (6) 1852-1857; DOI: 10.1128/JCM.37.6.1852-1857.1999
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