| Literature DB >> 23928222 |
Nora Martel1, Selma A Gomes, Isabelle Chemin, Christian Trépo, Alan Kay.
Abstract
For functional analysis of HBV isolates, epidemiological studies and correct identification of recombinant genomes, the amplification of complete genomes is necessary. A method for completely in vitro amplification of full-length HBV genomes starting from serum RC-DNA is described. This uses in vitro completion/ligation of plus-strand HBV RC-DNA and amplification using Rolling-Circle Amplification, eventually followed by a genomic PCR. The method can amplify complete HBV genomes from sera with viral loads ranging from >1.0E+8 IU/ml down to 1.0E+3 IU/ml. The method can be applied to archived sera that have undergone long-term storage or to archived DNA serum extracts. The genomes can easily be cloned. HBV genotypes A-G can all be amplified with no apparent problems. A recombinant subgenotype A3/genotype E genome was identified and fully sequenced.Entities:
Keywords: HBV; HBV genotypes; Recombinant genomes; Rolling-Circle Amplification (RCA); Serum relaxed-circular DNA
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Year: 2013 PMID: 23928222 DOI: 10.1016/j.jviromet.2013.07.045
Source DB: PubMed Journal: J Virol Methods ISSN: 0166-0934 Impact factor: 2.014