The functions of key residues in the inhibitor, substrate and cofactor sites of human 3beta-hydroxysteroid dehydrogenase type 1 are validated by mutagenesis

The functions of key residues in the inhibitor, substrate and cofactor sites of human 3beta-hydroxysteroid dehydrogenase type 1 are validated by mutagenesis

In postmenopausal women, human 3beta-hydroxysteroid dehydrogenase type 1 (3beta-HSD1) is a critical enzyme in the conversion of DHEA to estradiol in breast tumors, while 3beta-HSD2 participates in the production of cortisol and aldosterone in the human adrenal gland. The goals of this project are to...

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Veröffentlicht in:The Journal of steroid biochemistry and molecular biology 2010-06, Vol.120 (4-5), p.192
Hauptverfasser: Thomas, James L, Mack, Vance L, Sun, Jingping, Terrell, J Ross, Bucholtz, Kevin M
Format: Artikel
Sprache:eng
Schlagworte:
3-Hydroxysteroid Dehydrogenases - antagonists & inhibitors
3-Hydroxysteroid Dehydrogenases - chemistry
3-Hydroxysteroid Dehydrogenases - genetics
3-Hydroxysteroid Dehydrogenases - metabolism
Amino Acids - chemistry
Amino Acids - genetics
Amino Acids - metabolism
Binding Sites
Breast Neoplasms - drug therapy
Dehydroepiandrosterone - chemistry
Dehydroepiandrosterone - metabolism
Dihydrotestosterone - analogs & derivatives
Dihydrotestosterone - chemistry
Dihydrotestosterone - metabolism
Female
Humans
Kinetics
Models, Molecular
Mutagenesis, Site-Directed
Protein Binding
Protein Conformation
Substrate Specificity
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Zusammenfassung:In postmenopausal women, human 3beta-hydroxysteroid dehydrogenase type 1 (3beta-HSD1) is a critical enzyme in the conversion of DHEA to estradiol in breast tumors, while 3beta-HSD2 participates in the production of cortisol and aldosterone in the human adrenal gland. The goals of this project are to determine if Arg195 in 3beta-HSD1 vs. Pro195 in 3beta-HSD2 in the substrate/inhibitor binding site is a critical structural difference responsible for the higher affinity of 3beta-HSD1 for inhibitor and substrate steroids compared to 3beta-HSD2 and whether Asp61, Glu192 and Thr8 are fingerprint residues for cofactor and substrate binding using site-directed mutagenesis. The R195P-1 mutant of 3beta-HSD1 and the P195R-2 mutant of 3beta-HSD2 have been created, expressed, purified and characterized kinetically. Dixon analyses of the inhibition of the R195P-1 mutant, P195R-2 mutant, wild-type 3beta-HSD1 and wild-type 3beta-HSD2 by trilostane has produced kinetic profiles that show inhibition of 3beta-HSD1 by trilostane (K(i)=0.10microM, competitive) with a 16-fold lower K(i) and different mode than measured for 3beta-HSD2 (K(i)=1.60microM, noncompetitive). The R195P-1 mutation shifts the high-affinity, competitive inhibition profile of 3beta-HSD1 to a low-affinity (trilostane K(i)=2.56microM), noncompetitive inhibition profile similar to that of 3beta-HSD2 containing Pro195. The P195R-2 mutation shifts the low-affinity, noncompetitive inhibition profile of 3beta-HSD2 to a high-affinity (trilostane K(i)=0.19microM), competitive inhibition profile similar to that of 3beta-HSD1 containing Arg195. Michaelis-Menten kinetics for DHEA, 16beta-hydroxy-DHEA and 16alpha-hydroxy-DHEA substrate utilization by the R195P-1 and P195R-2 enzymes provide further validation for higher affinity binding due to Arg195 in 3beta-HSD1. Comparisons of the Michaelis-Menten values of cofactor and substrate for the targeted mutants of 3beta-HSD1 (D61N, D61V, E192A, T8A) clarify the functions of these residues as well.
ISSN:1879-1220
DOI:10.1016/j.jsbmb.2010.04.015