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Research ArticleArticle

Comparative Analysis and Functional Characterization of HC-AFW1 Hepatocarcinoma Cells: CYP Expression and Induction by Nuclear Receptor Agonists

Albert Braeuning, Maria Thomas, Ute Hofmann, Silvia Vetter, Eva Zeller, Barbara Petzuch, Janina Johanning, Werner Schroth, Thomas S. Weiss, Ulrich M. Zanger and Michael Schwarz
Drug Metabolism and Disposition August 26, 2015, dmd.115.064667; DOI: https://doi.org/10.1124/dmd.115.064667
Albert Braeuning
1 Federal Institute for Risk Assessment;
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  • For correspondence: albert.braeuning@bfr.bund.de
Maria Thomas
2 Dr.-Margarethe-Fischer-Bosch-Institute for Clinical Pharmacology;
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Ute Hofmann
2 Dr.-Margarethe-Fischer-Bosch-Institute for Clinical Pharmacology;
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Silvia Vetter
3 University of Tuebingen;
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Eva Zeller
3 University of Tuebingen;
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Barbara Petzuch
3 University of Tuebingen;
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Janina Johanning
2 Dr.-Margarethe-Fischer-Bosch-Institute for Clinical Pharmacology;
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Werner Schroth
2 Dr.-Margarethe-Fischer-Bosch-Institute for Clinical Pharmacology;
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Thomas S. Weiss
4 Regensburg University Hospital
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Ulrich M. Zanger
2 Dr.-Margarethe-Fischer-Bosch-Institute for Clinical Pharmacology;
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Michael Schwarz
3 University of Tuebingen;
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Abstract

Enzymatic conversion of most xenobiotic compounds is accomplished by hepatocytes in the liver, which are also an important target for the manifestation of the toxic effects of foreign compounds. Most cell lines derived from hepatocytes lack important toxifying or detoxifying enzymes or are defective in signaling pathways which regulate expression and activity of these enzymes. On the other hand, the use of primary human hepatocytes is complicated by scarce availability of cells and high inter-donor variability. Thus, analyses of drug metabolism and hepatotoxicity in vitro are a difficult task. The cell line HC-AFW1 was isolated from a pediatric hepatocellular carcinoma and so far has been used for tumorigenicity and chemotherapy resistance studies. Here, a comprehensive characterization of xenobiotic metabolism in HC-AFW1 cells is presented along with studies on the functionality of the most important transcriptional regulators of drug-metabolizing enzymes. Results from HC-AFW1 cells were compared to commercially available HepaRG cells and to cultured primary human hepatocytes. Data show that the nuclear receptors and xenosensors AHR (aryl hydrocarbon receptor), CAR (constitutive androstane receptor), PXR (pregnane-X-receptor), NRF2 (nuclear factor (erythroid-derived 2)-like 2), and PPARα (peroxisome proliferator-activated receptor α) are functional in HC-AFW1 cells, comparable to HepaRG and primary cells. HC-AFW1 cells possess considerable activities of different cytochrome P450 (CYP) enzymes, which, however, are lower than corresponding enzyme activities in HepaRG cells or primary hepatocytes. In summary, HC-AFW1 are a new promising tool for studying the mechanisms of the regulation of drug metabolism in human liver cells in vitro.

  • cytochrome P450
  • enzyme induction
  • liver physiology/models
  • nuclear receptors
  • The American Society for Pharmacology and Experimental Therapeutics
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Drug Metabolism and Disposition: 51 (6)
Drug Metabolism and Disposition
Vol. 51, Issue 6
1 Jun 2023
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Research ArticleArticle

Comparative Analysis and Functional Characterization of HC-AFW1 Hepatocarcinoma Cells: CYP Expression and Induction by Nuclear Receptor Agonists

Albert Braeuning, Maria Thomas, Ute Hofmann, Silvia Vetter, Eva Zeller, Barbara Petzuch, Janina Johanning, Werner Schroth, Thomas S. Weiss, Ulrich M. Zanger and Michael Schwarz
Drug Metabolism and Disposition August 26, 2015, dmd.115.064667; DOI: https://doi.org/10.1124/dmd.115.064667

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Research ArticleArticle

Comparative Analysis and Functional Characterization of HC-AFW1 Hepatocarcinoma Cells: CYP Expression and Induction by Nuclear Receptor Agonists

Albert Braeuning, Maria Thomas, Ute Hofmann, Silvia Vetter, Eva Zeller, Barbara Petzuch, Janina Johanning, Werner Schroth, Thomas S. Weiss, Ulrich M. Zanger and Michael Schwarz
Drug Metabolism and Disposition August 26, 2015, dmd.115.064667; DOI: https://doi.org/10.1124/dmd.115.064667
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