On the substrate specificity of cytochrome P450IIIA1

On the substrate specificity of cytochrome P450IIIA1

The instability of the solubilized/purified form, the lack of catalytic activity of the stabilized, macrolide-complexed form, and the compromised catalytic activity of the decomplexed form of steroid-inducible cytochrome P450IIIA1 motivated further investigations of the substrate specificity of this...

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Veröffentlicht in:Molecular pharmacology 1988-11, Vol.34 (5), p.628-637
Hauptverfasser: Namkung, M J, Yang, H L, Hulla, J E, Juchau, M R
Format: Artikel
Sprache:eng
Schlagworte:
2-Acetylaminofluorene - metabolism
Analytical, structural and metabolic biochemistry
Animals
Benzo(a)pyrene - metabolism
Biological and medical sciences
Cytochrome P-450 Enzyme System - analysis
cytochrome P450
Dealkylation
Dexamethasone - pharmacology
Enzyme Induction
Enzymes and enzyme inhibitors
Female
Fundamental and applied biological sciences. Psychology
Hydroxylation
Isoenzymes - analysis
Oxidoreductases
Pregnenolone - pharmacology
Rats
Rats, Inbred Strains
Substrate Specificity
Testosterone - metabolism
Troleandomycin - pharmacology
Warfarin - metabolism
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Zusammenfassung:The instability of the solubilized/purified form, the lack of catalytic activity of the stabilized, macrolide-complexed form, and the compromised catalytic activity of the decomplexed form of steroid-inducible cytochrome P450IIIA1 motivated further investigations of the substrate specificity of this isozyme. A major complementary goal was to identify reactions utilizable as sensitive, specific diagnostic probes for the detection and partial characterization of this isozyme in tissues for which isolation and purification are not practical (e.g., extrahepatic, embryonic tissues, etc.). The approach utilized a combination of a specific, purified inducer, specific inhibitors including triacetyloleandomycin and inhibitory antibodies, and diagnostic probe substrates including the phenoxazone ethers, testosterone, warfarin, 2-acetylaminofluorene, estradiol-17 beta and benzo[a]pyrene. The results obtained indicated that steroid-inducible, rat hepatic P450IIIA1 would catalyze minimal or no O-dealkylation of methoxy-, ethoxy- or pentoxyphenoxazone but catalyzed rapid O-debenzylation of benzyloxyphenoxazone. Hydroxylation of testosterone was specific for the beta face of the molecule at the 2-, 6-, 15- and 16-positions with no detectable conversion to androstenedione and minimal hydroxylation on the alpha face. Both the R- and S-enantiomers of warfarin were attacked at positions 9 and 10, and these reactions appeared to be specific to isozymes of the IIIA family. Aromatic hydroxylation of estradiol-17 beta was efficiently catalyzed, particularly at the 2-position. Hydroxylations of 2-acetylaminofluorene at positions 5 and 7 were catalyzed at relatively rapid rates, but N-hydroxylation of the same substrate was not catalyzed effectively. Hydroxylation of benzo[a]pyrene occurred preferentially at carbon 3 with much lesser activity at carbon 9 and little or no detectable attack at positions 7 or 1. The results indicated that the 2 beta- and 15 beta-hydroxylation of testosterone and the 10-hydroxylation of warfarin would serve as the most useful probes thus far available for detection of the presence of functional P450IIIA1 isozymes in tissues for which isolation and purification are impractical. The results also indicated a very broad, yet selective substrate specificity for the steroid-inducible P450IIIA1.
ISSN:0026-895X
1521-0111
DOI:10.1016/S0026-895X(25)09889-X