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  4. Inverse polymerase chain reaction for cloning cellular sequences adjacent to integrated hepatitis B virus DNA in hepatocellular carcinomas
 
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Inverse polymerase chain reaction for cloning cellular sequences adjacent to integrated hepatitis B virus DNA in hepatocellular carcinomas

Journal
Journal of Virological Methods
Journal Volume
49
Journal Issue
3
Pages
269-284
Date Issued
1994
Author(s)
Tsuei D.-J.
PEI-JER CHEN  
Lai M.-Y.
Chen D.-S.
Yang C.-S.
Chen J.-Y.
Hsu T.-Y.
DOI
10.1016/0166-0934(94)90142-2
URI
https://www.scopus.com/inward/record.uri?eid=2-s2.0-0028077914&doi=10.1016%2f0166-0934%2894%2990142-2&partnerID=40&md5=ff385645e350310412efe9fcd55e0eee
https://scholars.lib.ntu.edu.tw/handle/123456789/568898
Abstract
Integration of hepatitis B virus (HBV) DNA is found in most HBV-related human hepatocellular carcinomas (HCCs). In the past, construction of genomic libraries was mainly employed to study the role of viral integration. However, large amounts of tissue DNA and a laborious screening procedures were required. Inverse polymerase chain reaction (IPCR) is based on the simple procedures of digestion of DNA with restriction enzymes and circularization of cleavage products before amplification using primers synthesized in the opposite orientations to those normally employed for PCR. This technique allows the in vitro amplification of DNA flanking a region of known sequence. By employing this method, starting from nanograms of hepatoma DNA, two adjacent cellular sequences were cloned from 11 HBV integrants in three HCCs. The original configurations in the chromosomes were further confirmed. One of the flanking cellular sequences was identified as the human 28S rRNA gene, the other was not found homologous to any known human sequences. This method appears to be practical and can be improved further to clone more flanking cellular sequences, especially in early and small HCCs. ? 1994.
Subjects
HBV integration; Hepatocellular carcinoma; Inverse polymerase chain reaction
SDGs

[SDGs]SDG3

Other Subjects
virus dna; article; controlled study; hepatitis b virus; human; human cell; human tissue; integration; liver cell carcinoma; molecular cloning; nonhuman; polymerase chain reaction; priority journal; Base Sequence; Carcinoma, Hepatocellular; Cloning, Molecular; DNA Primers; DNA, Viral; Gene Amplification; Gene Rearrangement; Hepatitis B Virus; Human; Liver Neoplasms; Molecular Sequence Data; Polymerase Chain Reaction; Support, Non-U.S. Gov't; Virus Integration; Hepatitis B virus
Type
journal article

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