Original Article
Free Access
Assay of hepatitis B virus DNA by polymerase chain reaction and its relationship to Pre-S- and S-encoded viral surface antigens
Guido Gerken,
Patricia Paterlini, Michael Manns,
Chantal Housset, Sylvie Terre, Hans-Peter Dienes,
Georg Hess,
Wolfram H. Gerlich,
Pierre Berthelot, Karl-Hermann Meyer Zum Büschenfelde,
Christian Brechot,
Corresponding Author
Guido Gerken
1INSERM U 75 C.H.U. Necker, Paris, France
I. Med. Klinik und Poliklinik, Johannes Gutenberg Universität Mainz, Langenbeckstr. 1, D-65 Mainz, F.R.G.
INSERM U 75 C.H.U. Necker, 156 Rue de Vaugirard, F-75730 Paris Cedex 15, France===Search for more papers by this authorMichael Manns
I. Medizinische Klinik u. Poliklinik der Johannes Gutenberg—Universität Mainz, FRG
Search for more papers by this authorHans-Peter Dienes
Pathologisches Institut der Universität Mainz, FRG
Search for more papers by this authorGeorg Hess
I. Medizinische Klinik u. Poliklinik der Johannes Gutenberg—Universität Mainz, FRG
Search for more papers by this authorWolfram H. Gerlich
Abteilung Medizinische Mikrobiologie der Universität Göttingen, Göttingen, FRG
Search for more papers by this authorKarl-Hermann Meyer Zum Büschenfelde
I. Medizinische Klinik u. Poliklinik der Johannes Gutenberg—Universität Mainz, FRG
Search for more papers by this authorChristian Brechot
1INSERM U 75 C.H.U. Necker, Paris, France
Liver Unit, Hǒpital Laennec, Paris, France
Institut Pasteur, Laboratoire Hybridotest, Paris, France
Search for more papers by this authorGuido Gerken,
Patricia Paterlini, Michael Manns,
Chantal Housset, Sylvie Terre, Hans-Peter Dienes,
Georg Hess,
Wolfram H. Gerlich,
Pierre Berthelot, Karl-Hermann Meyer Zum Büschenfelde,
Christian Brechot,
Corresponding Author
Guido Gerken
1INSERM U 75 C.H.U. Necker, Paris, France
I. Med. Klinik und Poliklinik, Johannes Gutenberg Universität Mainz, Langenbeckstr. 1, D-65 Mainz, F.R.G.
INSERM U 75 C.H.U. Necker, 156 Rue de Vaugirard, F-75730 Paris Cedex 15, France===Search for more papers by this authorMichael Manns
I. Medizinische Klinik u. Poliklinik der Johannes Gutenberg—Universität Mainz, FRG
Search for more papers by this authorHans-Peter Dienes
Pathologisches Institut der Universität Mainz, FRG
Search for more papers by this authorGeorg Hess
I. Medizinische Klinik u. Poliklinik der Johannes Gutenberg—Universität Mainz, FRG
Search for more papers by this authorWolfram H. Gerlich
Abteilung Medizinische Mikrobiologie der Universität Göttingen, Göttingen, FRG
Search for more papers by this authorKarl-Hermann Meyer Zum Büschenfelde
I. Medizinische Klinik u. Poliklinik der Johannes Gutenberg—Universität Mainz, FRG
Search for more papers by this authorChristian Brechot
1INSERM U 75 C.H.U. Necker, Paris, France
Liver Unit, Hǒpital Laennec, Paris, France
Institut Pasteur, Laboratoire Hybridotest, Paris, France
Search for more papers by this authorAbstract
The polymerase chain reaction was evaluated as a diagnostic tool in 72 chronic hepatitis B virus carriers. Hepatitis B virus DNA was detectable in the serum of HBsAg—positive virus carriers using aliquots as small as 100 al. The detection limit for cloned hepatitis B virus DNA was 100 ag. Primer pairs for different regions of the HBV genome resulted in different sensitivity. Detection of the amplified hepatitis B virus DNA by Southern blotting and subsequent scintillation counting or densitometry allowed a semiquantitative assay. Using several primer pairs in parallel for optimal detection, all HBeAg-positive HBsAg carriers, 80% of HBe antibody—positive symptomatic HBsAg carriers and 57% of asymptomatic HBe antibody—positive HBsAg carriers were found to have hepatitis B virus DNA in the serum. During antiviral therapy hepatitis B virus DNA disappeared by the polymerase chain reaction assay in patients who became HBeAg negative, but polymerase chain reaction detected a relapse earlier than did the conventional dot blot. Pre-S antigens were assayed in serum and liver samples from most chronic carriers by enzyme-linked immunosorbent assay and/or immunoblot. Although most viremic carriers were strongly positive for pre-S1 and pre-S2 antigens, some hepatitis B virus DNA—positive HBsAg carriers did not have detectable pre-S antigens, and vice versa. Our data show that assay of hepatitis B virus DNA in the serum by polymerase chain reaction is by far more proficient than by dot blot and that it cannot be replaced by serological assays of HBeAg or pre-S antigen. (HEPATOLOGY 1991;13:158–166).
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