Genetic Modification of Hepatocytes towards Hepatocyte Transplantation and Liver Tissue Engineering

Hiroyuki Kuge; Kazuo Ohashi; Takashi Yokoyama; Hiromichi Kanehiro; Michiyoshi Hisanaga; Fumikazu Koyama; Ginny L. Bumgardner; Ken-Ichiro Kosai; Yoshiyuki Nakajima

doi:10.3727/000000006783982214

Cell Transplantation (Jan 2006)

Genetic Modification of Hepatocytes towards Hepatocyte Transplantation and Liver Tissue Engineering

Hiroyuki Kuge,
Kazuo Ohashi,
Takashi Yokoyama,
Hiromichi Kanehiro,
Michiyoshi Hisanaga,
Fumikazu Koyama,
Ginny L. Bumgardner,
Ken-Ichiro Kosai,
Yoshiyuki Nakajima

Affiliations

Hiroyuki Kuge: Department of Surgery, Nara Medical University, Nara, Japan
Kazuo Ohashi: Department of Surgery, Nara Medical University, Nara, Japan
Takashi Yokoyama: Department of Surgery, Nara Medical University, Nara, Japan
Hiromichi Kanehiro: Department of Surgery, Nara Medical University, Nara, Japan
Michiyoshi Hisanaga: Department of Surgery, Nara Medical University, Nara, Japan
Fumikazu Koyama: Department of Surgery, Nara Medical University, Nara, Japan
Ginny L. Bumgardner: Department of Surgery, Ohio State University Medical Center, Columbus, OH, USA
Ken-Ichiro Kosai: Division of Gene Therapy and Regenerative Medicine, Cognitive and Molecular Research Institute for Brain Diseases, Kurume University, Kurume, Japan
Yoshiyuki Nakajima: Department of Surgery, Nara Medical University, Nara, Japan

DOI: https://doi.org/10.3727/000000006783982214
Journal volume & issue: Vol. 15

Abstract

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Cell-based therapies, including liver tissue engineering following hepatocyte transplantation, have therapeutic potential for several types of liver diseases. Modifications in the methodology to manipulate the donor hepatocytes in a more simple and timely manner prior to transplantation would enhance the therapeutic efficacy of this procedure. Conventional approach for vector-mediated gene transduction to the isolated hepatocytes has been performed under primary culture conditions that routinely require several days to complete. In our study, we have established a clinically feasible approach that requires only 1 h of infection time with an adenoviral vector system that results in an extremely efficient transduction efficiency (>80%). To optimize transduction efficiency and sustain normal cellular function, we determined that the isolated hepatocytes should be maintained in UW solution as a suspension medium and infected with adenoviral vectors (Ad) for no more than 1 h at a MOI of 1. To establish if the isolated hepatocytes could be used as a source for cell-based therapies, we transplanted the Ad-transduced hepatocytes into the liver or under the kidney capsule. When the cells were transplanted into the liver, Ad-transduced hepatocytes cultured in suspension conditions were found to have a significantly higher survival rate (p < 0.01) than Ad-transduced hepatocytes cultured under standard conditions. We also confirmed that these Ad-transduced hepatocytes have ability to survive long term and were able to engineer a biologically active hepatic tissue under the kidney capsule. Finally, we obtained high level of transduction into canine, porcine, and human isolated hepatocytes in a suspension solution mixed with Ad. In conclusion, the present studies demonstrate that isolated hepatocytes could be genetically modified using Ad when kept in a suspension solution. For this reason, this cell-modified technique could be used for the treatment of liver-targeted diseases and/or disorders.

Published in Cell Transplantation

ISSN: 0963-6897 (Print); 1555-3892 (Online)
Publisher: SAGE Publishing
Country of publisher: United States
LCC subjects: Medicine
Website: http://journals.sagepub.com/home/cll

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