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  ESTABLISHMENT OF IMMORTALIZED HUMAN HEPATIC STELLATE SCAVENGER CELLS TO DEVELOP BIOARTIFICIAL LIVERS

Watanabe, T., Shibata, N., Westerman, K. A., Okitsu, T., Allain, J. E., Sakaguchi, M., Totsugawa, T., Maruyama, M., Matsumura, T., Noguchi, H., Yamamoto, S., Hikida, M., Ohmori, A., Reth, M., Weber, A., Tanaka, N., Leboulch, P., & Kobayashi, N. (2003). ESTABLISHMENT OF IMMORTALIZED HUMAN HEPATIC STELLATE SCAVENGER CELLS TO DEVELOP BIOARTIFICIAL LIVERS. Transplantation, 75(11), 1873-1880.

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資料種別: 学術論文

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 作成者:
Watanabe, Takamasa, 著者
Shibata, Norikuni, 著者
Westerman, Karen A., 著者
Okitsu, Teru, 著者
Allain, Jean E., 著者
Sakaguchi, Masakiyo, 著者
Totsugawa, Toshinori, 著者
Maruyama, Masanobu, 著者
Matsumura, Toshihisa, 著者
Noguchi, Hirofumi, 著者
Yamamoto, Shinichiro, 著者
Hikida, Masaki, 著者
Ohmori, Akira, 著者
Reth, Michael1, 著者           
Weber, Anne, 著者
Tanaka, Noriaki, 著者
Leboulch, Philippe, 著者
Kobayashi, Naoya, 著者
所属:
1Research Group and Chair of Molecular Immunology of the University of Freiburg, Max Planck Institute of Immunobiology and Epigenetics, Max Planck Society, ou_2243645              

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 要旨: BACKGROUND: Maintenance of liver-specific functions has been shown to be stabilized by co-cultivation of hepatocytes with hepatic stellate cells (HSC). Because the limited lifespan of human HSC is a major hurdle to their use, the authors report here the amplification of human HSC populations in vitro by retroviral transfer of human telomerase reverse transcriptase (hTERT). METHODS: Human HSC strain LI 90 cells were transduced with a retroviral vector SSR#197 expressing hTERT and green fluorescent protein (GFP) cDNA flanked by a pair of loxP. TWNT-1, one of SSR#197-immortalized HSC, was characterized. Differentiated liver functions were evaluated in an immortalized human hepatocyte NKNT-3-TWNT-1 co-culture system. RESULTS: TWNT-1 cells showed differential functions of HSC, including uptake of acetylated low-density lipoproteins and synthesis of collagen type I and hepatocyte growth factor. Efficient excision of the retrovirally transferred hTERT and GFP cDNAs was achieved by TAT-mediated expression of the Cre recombinase and subsequent GFP-negative cell sorting. When co-cultured with TWNT-1 cells, NKNT-3 increased protein expression of the detoxifying cytochrome P450-associated protein isoenzymes 3A4 and 2C9 and urea synthesis. CONCLUSIONS: TWNT-1 cells could be valuable in the study of integrated liver functions and contribute to the optimization of liver cell therapies and bioartificial livers.

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言語: eng - English
 日付: 2003-06-15
 出版の状態: 出版
 ページ: -
 出版情報: -
 目次: -
 査読: -
 識別子(DOI, ISBNなど): eDoc: 127841
ISI: 000183684900016
 学位: -

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出版物 1

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出版物名: Transplantation
種別: 学術雑誌
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出版社, 出版地: -
ページ: - 巻号: 75 (11) 通巻号: - 開始・終了ページ: 1873 - 1880 識別子(ISBN, ISSN, DOIなど): ISSN: 0041-1337