Quantitation of hepatitis B virus genomic DNA by real-time detection PCR

被引:227
作者
Abe, A
Inoue, K
Tanaka, T
Kato, J
Kajiyama, N
Kawaguchi, R
Tanaka, S
Yoshiba, M
Kohara, M
机构
[1] Tokyo Metropolitan Inst Med Sci, Dept Microbiol, Bunkyo Ku, Tokyo 1138613, Japan
[2] Tokyo Metropolitan Komagome Hosp, Liver Unit, Bunkyo Ku, Tokyo 1138613, Japan
[3] SRL Inc, Ctr Mol Biol & Cytogenesis, Tokyo 1920002, Japan
[4] Showa Univ, Fujigaoka Hosp, Div Gastroenterol, Aoba Ku, Yokohama, Kanagawa 2278501, Japan
[5] Tokyo Womens Med Coll, Inst Gastroenterol, Shinjyuku Ku, Tokyo 1620054, Japan
关键词
D O I
10.1128/JCM.37.9.2899-2903.1999
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Quantitation of hepatitis B virus (HBV) DNA in serum is a useful method for the monitoring of HBV replication. We attempted to develop a quantitative assay system for HBV DNA that is more sensitive, accurate, and reproducible than existing systems. We detected HBV DNA by real-time detection PCR (RTD-PCR) based on Tag Man chemistry. The efficacy of this assay was evaluated by quantitatively measuring sequential levels of synthetic DNA and DNA in clinical serum samples. The detection limit of this system was as few as 10 DNA copies/reaction. A linear standard curve was obtained between 10(1) and 10(8) DNA copies/reaction. The coefficient of variation for both intra- and interexperimental variability indicated remarkable reproducibility, This system detected HBV DNA in 100% of chronic hepatitis B patients tested and never detected HBV DNA in healthy volunteers who were negative for HBV markers. These observations suggest that RTD-PCR is an excellent candidate for a standard HBV quantification method.
引用
收藏
页码:2899 / 2903
页数:5
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