Detection of hepatitis B virus DNA in paraffin‐embedded liver tissues in chronic hepatitis B or non‐A, non‐B hepatitis using the polymerase chain reaction

We developed a polymerase chain reaction assay for the direct detection of hepatitis B virus in paraffinembedded liver tissue and applied this assay to determine whether hepatitis B virus DNA exists in livers with chronic hepatitis non‐A, non‐B. Fifty five liver biopsy samples were studied: 11 from...

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Bibliographic Details
Published in:Hepatology (Baltimore, Md.) Md.), 1991-01, Vol.13 (1), p.167-171
Main Authors: Shindo, Michiko, Okuno, Tadao, Arai, Ken, Matsumoto, Masayuki, Takeda, Makoto, Kashima, Kei, Shimada, Mamoru, Fujiwara, Yoshiaki, Sokawa, Yoshihiro
Format: Article
Language:English
Subjects:
Adult
Chronic Disease
DNA, Viral - analysis
Female
Hepatitis B - metabolism
Hepatitis B - microbiology
Hepatitis B virus - genetics
Hepatitis C - metabolism
Hepatitis C - microbiology
Humans
Liver - chemistry
Liver - microbiology
Male
Middle Aged
Polymerase Chain Reaction
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Summary:We developed a polymerase chain reaction assay for the direct detection of hepatitis B virus in paraffinembedded liver tissue and applied this assay to determine whether hepatitis B virus DNA exists in livers with chronic hepatitis non‐A, non‐B. Fifty five liver biopsy samples were studied: 11 from patients with HBeAg‐positive chronic hepatitis (paraffin‐embedded) and 44 from patients with chronic hepatitis non‐A, non‐B (21 paraffin‐embedded 25 fresh frozen). Thirty three (75%) of the non‐A, non‐B cases were positive for hepatitis C virus antibodies. Approximately 1 to 10 ng of DNA was extracted from the paraffin‐embedded tissue and amplified using oligonucleotide (23‐mer) primers specific for the S gene (positions 261 to 692). The β‐globin gene was used as an internal control for sensitivity because this is a single copy gene and allows for relative quantification. In each of the chronic hepatitis B livers, the expected 432‐base‐pair amplification product for hepatitis B virus DNA and β‐globin gene product were both detected. On the other hand, in the 21 paraffin‐embedded chronic hepatitis non‐A, non‐B livers, no hepatitis B virus DNA was detected, although β‐globin gene was observed in all. Furthermore, in all 25 frozen non‐A, non‐B livers, β‐globin gene was observed, but no hepatitis B virus band was seen. The limit of detection of hepatitis B virus DNA by this method was estimated to be one genomic copy of hepatitis B virus DNA per cell. Thus all patients with chronic hepatitis B, but no patients with clinically diagnosed non‐A, non‐B hepatitis, had hepatitis B virus DNA in liver at a level of or above one copy per hepatocyte. (HEPATOLOGY 1991;13:167–171).
ISSN:0270-9139
1527-3350
DOI:10.1002/hep.1840130124