Expression of Recombinant HBV Pol Proteins in HepG2 Cells

  • Cho, Ginam (School of Biological Science, Seoul National University) ;
  • Na, Seun-Gon (School of Biological Science, Seoul National University) ;
  • Suh, Se-Won (Department of Chemistry, Seoul National University) ;
  • Jung, Gu-Hung (School of Biological Science, Seoul National University)
  • Received : 2000.06.15
  • Accepted : 2000.10.10
  • Published : 2000.11.30

Abstract

In this study HepG2 cells were used to express and purify HBV pol proteins. In order to facilitate purification of HBV pol proteins, HBV pol and its deletion mutants were fused to MBP (Maltose Binding Protein). As a result we successfully expressed and partially purified both wild type and mutant recombinant HBV pol proteins by using an amylose resin and anti-MBP antibody. In the case of wild type, the anti-MBP antibody detected three bands. One was full-length and the others were generated by proteolysis of the terminal domain region. The expressed MBP/POL proteins were localized both in the cytoplasm and in the perinuclear region. The purified proteins had polymerase activity toward an exogenous homo-polymer template. The MBP/POL protein also had DNA synthesis activity in vivo, since the MBP/POL expression construct was able to complement a HBV polymerase mutant in trans.

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