Metabolism of Chrysene and Phenanthrene to Bay-Region Diol Epoxides by Rat Liver Enzymes

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Metabolism of Chrysene and Phenanthrene to Bay-Region Diol Epoxides by Rat Liver Enzymes

M. NORDQVIST ¹, D. R. THAKKER ¹, K. P. VYAS ¹, H. YAGI ¹, W. LEVIN ¹, D. E. RYAN ¹, P. E. THOMAS ¹, A. H. CONNEY ¹, and D. M. JERINA ¹

¹ Laboratory of Bioorganic Chemistry, National Institute of Arthritis, Metabolism and Digestive Diseases, National Institutes of Health, Bethesda, Maryland 20205, and Department of Biochemistry and Drug Metabolism, Hoffman-La Roche Inc., Nutley, New Jersey 07110

Liver microsomal metabolism of the weak carcinogen chryseneand the noncarcinogen phenanthrene are compared. In general,chrysene is a rather poor substrate whereas phenanthrene isa relatively good substrate for the cytochrome P-450-dependentmonooxygenase system. With microsomes from 3-methylcholanthrene-treatedrats, phenanthrene was metabolized at a rate of 7.6 nmoles/min/nmoleof cytochrome P-450 as compared with a rate of only 1.5 withchrysene as substrate. Dihydrodiols were major metabolites forboth substrates, accounting for 92%-96% of the metabolism ofphenanthrene and 65%-76% of the metabolism of chrysene withmicrosomes from control and treated rats. The K-region 9,10-dihydrodiolis the major metabolite of phenanthrene, whereas the benzo-ring1,2- and 3,4-dihydrodiols dominate the metabolism of chrysene fromwhich very little K-region dihydrodiol was formed. For bothhydrocarbons, microsomes from 3-methylcholanthrene-treated ratsproduced the (-)-[1R,2R]-dihydrodiol, which hasa bay-region double bond, with $ge$ 80% enantiomeric purity. Withmicrosomes from phenobarbital-treated rats, the chrysene 1,2-dihydrodiolwas only 10% enantiomerically pure. The (-)-[3R,4R]-dihydrodiolswere the major enantiomers of phenanthrene and chrysene, whereasthe (-)-[9S,1OS]-dihydriol predominated at the K-regionof phenanthrene. Metabolism of the metabolically formed (-)-[1R,2R]-dihydrodiolsof phenanthrene and chrysene by microsomes from 3-methylcholanthrene-treatedrats resulted in the predominant formation in each case of abay-region 1,2-diol-3,4-epoxide in which the benzylic hydroxylgroup and oxirane oxygen are trans to each other (isomer-2).The respective 1,2-dihydrodiols were metabolized at the samerate as was chrysene. Thus, as had previously been observedfor the metabolism of benzo[a]pyrene and benzo[a]anthracene,liver microsomal enzymes display high stereoselectivity in theirformation of predominantly one of four possible stereoisomersof their respective bay-region diol epoxides. These diol epoxidesfrom the four hydrocarbons are superimposable when their bay-regionsare aligned.

Submitted on July 14, 1980
Accepted on September 3, 1980

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