Cell Transplantation (Sep 2000)

Long-Term Culture of Glutamine Synthetase-Transfected HepG2 Cells in Circulatory Flow Bioreactor for Development of a Bioartificial Liver

  • Shin Enosawa,
  • Tomoyuki Miyashita,
  • Seiichi Suzuki,
  • Xiao-Kang Li,
  • Miyuki Tsunoda,
  • Hiroshi Amemiya,
  • Mitsugu Yamanaka,
  • Shinya Hiramatsu,
  • Naoko Tanimura,
  • Takeshi Omasa,
  • Kenichi Suga,
  • Toshiharu Matsumura

DOI
https://doi.org/10.1177/096368970000900520
Journal volume & issue
Vol. 9

Abstract

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Glutamine synthetase (GS) is involved in an accessory pathway of ammonia removal in mammals. To develop a bioartificial liver with a human cell line, GS gene was transfected into HepG2 cells, which had no ammonia removal activity. After culturing in the presence of methionine sulfoximine (MSX), a GS inhibitor, we obtained a MSX-resistant HepG2 subline (GS-HepG2), which had amplified GS gene; ammonia removal activity was estimated to be 1/7 of that of rat primary culture hepatocytes. The cells were cultured in a circulatory flow bioreactor for 109 days, while they multiplied from 5 × 10 7 to 4 × 10 9 cells. Three days after inoculation, the ammonia level of the culture medium was lowered to a level maintained thereafter, suggesting that using recombinant cell lines for bioartificial livers enables long-term repeated treatment for hepatic failure patient. Judging from the rate of decrease in the amount of the added ammonia, the ammonia removal capability of 4 × 10 9 GS-HepG2 cells was almost equivalent to 5 × 10 8 porcine hepatocytes inoculated into the circulatory flow bioreactor. Apart from their ammonia removal activity, GS-HepG2 cells eliminated human tumor necrosis factor-α (TNF-α). Cytokine removal therefore promises to be another useful property of bioreactor cells.