Detection of Hepatitis B Virus DNA in Serum by a Simple Spot Hybridization Technique: Comparison with Results for Other Viral Markers

Authors

J Scotto

Published

September 21, 2007

Abstract

HepatologyVolume 3, Issue 3 p. 279-284 Original ArticlesFree Access Detection of Hepatitis B Virus DNA in Serum by a Simple Spot Hybridization Technique: Comparison with Results for Other Viral Markers Jacques Scotto, Corresponding Author Jacques Scotto Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Dr. Jacques Scotto, INSERM U 56, Hǒpital de Bicětre, F 94270 Le Kremlin-Bicětre, France.===Search for more papers by this authorMichelle Hadchouel, Michelle Hadchouel Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this authorChristiane Hery, Christiane Hery Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this authorJeannine Yvart, Jeannine Yvart Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this authorPierre Tiollais, Pierre Tiollais Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this authorChristian Brechot, Christian Brechot Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this author Jacques Scotto, Corresponding Author Jacques Scotto Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Dr. Jacques Scotto, INSERM U 56, Hǒpital de Bicětre, F 94270 Le Kremlin-Bicětre, France.===Search for more papers by this authorMichelle Hadchouel, Michelle Hadchouel Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this authorChristiane Hery, Christiane Hery Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this authorJeannine Yvart, Jeannine Yvart Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this authorPierre Tiollais, Pierre Tiollais Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this authorChristian Brechot, Christian Brechot Unité de Recherche d'Hépatologie Infantile (INSERM U 56) & Clinique de Pédiatrie, Université Paris-Sud, Hǒpital d'Enfants and Service de Médecine Nucléaire, CHU de Bicětre, Bicětre, France, F 94270; and Unité de Recombinaison et Expression Génétique (INSERM U163), Institut Pasteur, Paris, France, F 75015Search for more papers by this author First published: 1983 https://doi.org/10.1002/hep.1840030301Citations: 268AboutPDF ToolsRequest permissionExport citationAdd to favoritesTrack citation ShareShare Give accessShare full text accessShare full-text accessPlease review our Terms and Conditions of Use and check box below to share full-text version of article.I have read and accept the Wiley Online Library Terms and Conditions of UseShareable LinkUse the link below to share a full-text version of this article with your friends and colleagues. Learn more.Copy URL Share a linkShare onFacebookTwitterLinked InRedditWechat Abstract A simplified spot method for determination in serum of hepatitis B virus DNA (HBV DNA) by molecular hybridization is proposed. For simultaneous testing of 30 serum samples, it reduced to about 1 hr the duration of the steps preceding hybridization proper. The method also greatly reduced the loss of DNA during these steps and allowed more sensitive detection in samples of only 25 or 50 m̈1. HBV DNA was determined in 181 serum samples by this method, and the results were pooled with 67 previous determinations by the Southern blot technique. Results for the pool were then compared to those obtained with radioimmunoassay for serological HBV markers. Ninety-six of the 248 samples were HBV DNA positive. Eleven others gave variable or inconclusive results, probably due to low viral particle titers. Seventy-two HBsAg- and HBeAg-positive sera contained HBV DNA, confirming that HBeAg is a marker of active viral replication. Fourteen other HBsAg- and HBeAg-positive sera, obtained from eight patients, were either HBV DNA negative or oscillated between negative and positive, or, again, were weakly positive; serological follow-up in 7 patients showed seroconversion to anti-HBe in 5, 3 of which became HBsAg negative. Eight of the HBsAg-positive sera were negative or borderline for HBeAg but contained HBV DNA and may, therefore, have been infective; seven of these sera had anti-HBe. Six HBsAg-negative sera contained HBV DNA and may also have been infective; five of these exhibited HBV antibodies. These results indicate that molecular hybridization not only provides a more sensitive and direct method for detecting hepatitis B virus in serum but also defines additional serological patterns with predictive or epidemiological value. Citing Literature Volume3, Issue31983Pages 279-284 ReferencesRelatedInformation