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. 2007;50(6):387-93.
doi: 10.1159/000110650. Epub 2007 Oct 31.

In vitro replication of hepatitis D virus using a new construct containing a cDNA dimer of HDV genome

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In vitro replication of hepatitis D virus using a new construct containing a cDNA dimer of HDV genome

Farida Behzadian et al. Intervirology. 2007.

Erratum in

  • Intervirology. 2008;51(3):202. Chahooki, Fatemeh Fotouhi [corrected to Fotouhi, Fatemeh]

Abstract

Background: There is no cell line susceptible to hepatitis D virus (HDV) infection and capable of stable replication of its genome. Different genetic-based approaches have been introduced to initiate HDV replication events so far.

Methods: In order to construct a replicative model for HDV made from a unique genome sequence, two monomeric units of HDV full-length cDNA were joined together through a four-step cloning scheme. The resulting vector (pcDNA3.1-D2) containing two tandem repeats of HDV cDNA under CMV promoter control was then used in transfection experiments into COS7 and HuH7 cell lines.

Results: HDV replication markers including expression of hepatitis delta antigen (HDAg), the only HDV-specific antigen, and synthesis of antigenomic RNA were shown in both transfected cell lines, indicating initiation of HDV genome replication.

Conclusions: Our results suggested that pcDNA3.1-D2, a vector containing a cDNA dimer of the HDV genome, originated from a unique full-length HDV molecule that is capable of replicating in cultured cells. This vector can be used conveniently for transfection experiments to study HDV molecular biology.

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