Kinetic Modeling of {beta}-Chloroprene Metabolism: I. In vitro Rates in Liver and Lung Tissue Fractions from Mice, Rats, Hamsters, and Humans

doi:10.1093/toxsci/kfh092

ToxSci Advance Access originally published online on February 19, 2004

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Toxicological Sciences 79, 18-27 (2004)
Toxicological Sciences vol. 79 no. 1 © Society of Toxicology; all rights reserved.

Kinetic Modeling of ß-Chloroprene Metabolism: I. In vitro Rates in Liver and Lung Tissue Fractions from Mice, Rats, Hamsters, and Humans

Matthew W. Himmelstein¹, Steven C. Carpenter and Paul M. Hinderliter

E.I. du Pont de Nemours and Company, Haskell Laboratory for Health and Environmental Sciences, PO Box 50, 1090 Elkton Road, Newark, Delaware 19711

Received October 18, 2003; accepted January 26, 2004

Beta-chloroprene (2-chloro-1,3-butadiene, CD) is carcinogenicby inhalation exposure to B6C3F1 mice and Fischer F344 ratsbut not to Wistar rats or Syrian hamsters. The initial stepin metabolism is oxidation, forming a stable epoxide (1-chloroethenyl)oxirane(1-CEO), a genotoxicant that might be involved in rodent tumorigenicity.This study investigated the species-dependent in vitro kineticsof CD oxidation and subsequent 1-CEO metabolism by microsomalepoxide hydrolase and cytosolic glutathione S-transferases inliver and lung, tissues that are prone to tumor induction. Estimatesfor Vmax and Km for cytochrome P450-dependent oxidation of CDin liver microsomes ranged from 0.068 to 0.29 µ;mol/h/mgprotein and 0.53 to 1.33 µ;M, respectively. Oxidation(Vmax/Km) of CD in liver was slightly faster in the mouse andhamster than in rats or humans. In lung microsomes, Vmax/Kmwas much greater for mice compared with the other species. TheVmax and Km estimates for microsomal epoxide hydrolase activitytoward 1-CEO ranged from 0.11 to 3.66 µ;mol/h/mg proteinand 20.9 to 187.6 µ;M, respectively, across tissues andspecies. Hydrolysis (Vmax/Km) of 1-CEO in liver and lung microsomeswas faster for the human and hamster than for rat or mouse.The Vmax/Km in liver was 3 to 11 times greater than in lung.1-CEO formation from CD was measured in liver microsomes andwas estimated to be 2–5% of the total CD oxidation. GlutathioneS-transferase-mediated metabolism of 1-CEO in cytosolic tissuefractions was described as a pseudo-second order reaction; rateswere 0.0016–0.0068/h/mg cytosolic protein in liver and0.00056–0.0022 h/mg in lung. The observed differencesin metabolism are relevant to understanding species differencesin sensitivity to CD-induced liver and lung tumorigenicity.

Key Words: 2-chloro-1,3-butadiene; microsomes; cytosol; liver; lung; mouse; rat; hamster; human; in vitro kinetics.

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