Home
About Us
FAQs
Alternatives A to Z
Research Resources
Education Resources
Calendar
Publications
Links
Altweb Newsletter
Español

Project Team
Sponsors

Print this page / Imprima esta página

SEARCH

MEETINGS

Alternatives and 3Rs Workshop
January 28-29, 2008
Santa Monica, CA
Details forthcoming

ICCVAM's 10-Year Anniversary Symposium
February 5, 2008
Bethesda, MD

Workshop on Acute Chemical Safety Testing (NICEATM/ICCVAM)
February 6-8, 2008
Bethesda, MD

Shaping the Future of Research: Bringing Together IACUCs, IBCs & IRBs
February 14-15, 2008
Tempe, Arizona

PRIM&R: 2008 Annual Institutional Animal Care & Use Committee (IACUC) Conference
March 25-28, 2008
Atlanta, GA

MORE MEETINGS...

 

 

 

ALTEX :: Alternatives to Animal Experiments

2007, VOLUME 1

Use of a standardised and validated long-term human hepatocyte culture system for repetitive analyses of drugs: Repeated administrations of acetaminophen reduces albumin and urea secretion

Anett Ullrich¹, Christine Berg¹, Jan G. Hengstler² and Dieter Runge¹

¹PRIMACYT Cell Culture Technology GmbH, FRG, Schwerin; ²Center for Toxicology, University Leipzig, FRG, Leipzig, Germany

SUMMARY

Human hepatocytes are the in vitro system of choice to study drug-induced processes in man. Here, we present HEPAC2: a standardised and validated culture system in which human hepatocytes are maintained in HHMM (Human Hepatocyte Maintenance Medium) with HGF (hepatocyte growth factor) and EGF (epidermal growth factor). Cellular viability and hepatocellular functions were monitored daily. Albumin and urea production remained on a relatively constant level for up to 2-3 weeks. Based on this, a standard protocol was established that allows repeated exposure of hepatocytes to study drug metabolism. We used acetaminophen (AAP) to assay the feasibility of this system. Hepatocytes were exposed to AAP (100-2815 mg/l) for 24 h. Subsequently, the culture medium was replaced by medium without AAP and the same exposure scenario was repeated at intervals of 4 days. High doses of AAP (2815 mg/l) diminished urea production by 15-30% and albumin secretion by 70-80%. These effects were reversible. After removal of AAP, secretion of urea and albumin returned to control levels. AAP hepatotoxicity is caused by its biotransformation to the reactive metabolite N-acetyl-p-benzoquinoneimine (NAPQI) mediated by CYP2E1 and CYP1A2. The AAP activating enzymes were active for at least 21 days and their activity was maintained during at least four repeated cycles of exposure to AAP. In conclusion, these data demonstrate the suitability of our long-term culture system to serve as a tool for repetitive screening of drug-mediated changes of hepatocellular functions. This culture technique may help to overcome the sparse availability of human hepatocytes for testing drugmediated responses in man.

Keywords: human hepatocytes, long-term cultures, acetaminophen, repetitive cycles of drug administration