Investigation of the hepatotoxicity of flutamide: pro-survival/apoptotic and necrotic switch in primary rat hepatocytes characterized by metabolic and transcriptomic profiles in microfluidic liver biochips

Audrey Legendre; Sébastien Jacques; Florent Dumont; Jérôme Cotton; Patrick Paullier; Marie José Fleury; Eric Leclerc

doi:10.1016/j.tiv.2014.04.008

Investigation of the hepatotoxicity of flutamide: pro-survival/apoptotic and necrotic switch in primary rat hepatocytes characterized by metabolic and transcriptomic profiles in microfluidic liver biochips

Toxicol In Vitro. 2014 Aug;28(5):1075-87. doi: 10.1016/j.tiv.2014.04.008. Epub 2014 Apr 30.

Authors

Audrey Legendre¹, Sébastien Jacques², Florent Dumont², Jérôme Cotton³, Patrick Paullier¹, Marie José Fleury¹, Eric Leclerc⁴

Affiliations

¹ CNRS UMR 7338, Laboratoire de Biomécanique et Bio ingénierie, Université de Technologie de Compiègne, France.
² INSERM U1016 Plate-forme génomique institut Cochin, 22 rue Méchain, 75014 Paris, France.
³ Profilomic, 31 rue d'Aguesseau, 92100 Boulogne-Billancourt, France.
⁴ CNRS UMR 7338, Laboratoire de Biomécanique et Bio ingénierie, Université de Technologie de Compiègne, France. Electronic address: eric.leclerc@utc.fr.

PMID: 24793618
DOI: 10.1016/j.tiv.2014.04.008

Abstract

We investigated the effects of the liver damage induced by flutamide in primary rat hepatocytes using liver microfluidic biochips. Flutamide is a non-steroidal anti-androgenic drug. Two flutamide concentrations, 10 μM and 100 μM, were used to expose the hepatocytes for 24h under perfusion. Thanks to the maintenance of hepatocyte differentiation phenotype and to the biotransformation performance in the microfluidic cultures, the metabolic ratio analysis of hydroxyflutamide, flutamide-gluthatione and hydroxyflutamide-gluthatione productions demonstrated saturation of the drug's biotransformation process and the maintenance of a high level of flutamide at 100 μM when compared to 10 μM. A microarray analysis comparing flutamide (10 or 100 μM) with controls revealed a common response for both concentrations illustrated by modulating the expression of the mRNA of genes associated with mitochondrial perturbation, of the proliferator-activated receptors (Ppar) signaling, lipid and fatty acid metabolism, antioxidant defense, and cell death pathways, consistently with in vitro and in vivo reports. Additionally to literature reports, our integration of the transcriptomic profiles demonstrated a specific dose dependent response. We found at 10 μM a typical pro-survival/apoptosis network activation (through IGF/PDGFD upstream route and via a downstream up regulation in CREB5, BCL2, IKBKG routes in the PI3K/signaling). We also found a down regulation of mRNA levels in sugar and amino acid metabolism pathways. At 100 μM a typical necrosis switch was observed associated with a down regulation of the tight junctions' pathway, a cellular aggregation and a reduction of the cell viability. Altogether our data demonstrated the potential and the sensitivity of our liver microfluidic cultures to evaluate xenobiotic toxicity by improving in vitro analysis and reproducing both in vitro and in vivo results. Finally, we proposed two integrated synthetic networks to describe the response of rat hepatocytes to both exposure concentrations of flutamide.

Keywords: Flutamide; Hepatotoxicity; Metabolism; Microarray; Microfluidic biochips; Rat primary hepatocytes; Transcriptomic.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Androgen Antagonists / toxicity*
Animals
Bioreactors
Cells, Cultured
Cytochrome P-450 CYP1A1 / metabolism
Flutamide / toxicity*
Gene Expression Profiling
Hepatocytes / drug effects*
Hepatocytes / metabolism
Microarray Analysis
Microfluidic Analytical Techniques*
RNA, Messenger / metabolism
Rats

Substances

Androgen Antagonists
RNA, Messenger
Flutamide
Cytochrome P-450 CYP1A1