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Active Site Architecture of Polymorphic Forms of Human Glutathione S-Transferase P1-1 Accounts For Their Enantioselectivity and Disparate Activity in the Glutathione Conjugation of 7-Beta,8-Alpha-Dihydroxy-9-Alpha,10-Alpha-Oxy-7,8,9,10-Tetrahydroben Zo(a)Pyrene

  1. Author:
    Hu, X.
    Odonnell, R.
    Srivastava, S. K.
    Xia, H.
    Zimniak, P.
    Nanduri, B.
    Bleicher, R. J.
    Awasthi, S.
    Awasthi, Y. C.
    Ji, X. H.
    Singh, S. V.

  2. Author Address

    Ji XH MERCY HOSP MERCY CANC INST CANC RES LAB PITTSBURGH, PA 15219 USA MERCY HOSP MERCY CANC INST CANC RES LAB PITTSBURGH, PA 15219 USA NCI FREDERICK CANC RES & DEV CTR ABL BASIC RES PROGRAM FREDERICK, MD 21702 USA UNIV ARKANSAS MED SCI HOSP DEPT MED LITTLE ROCK, AR 72205 USA UNIV ARKANSAS MED SCI HOSP DEPT BIOCHEM & MOL BIOL LITTLE ROCK, AR 72205 USA MCCLELLAN VA HOSP MED RES LITTLE ROCK, AR 72205 USA UNIV TEXAS MED BRANCH DEPT INTERNAL MED GALVESTON, TX 77555 USA UNIV TEXAS MED BRANCH DEPT HUMAN BIOL CHEM & GENET GALVESTON, TX 77555 USA
    1. Year: 1997
  2. Journal: Biochemical and Biophysical Research Communications
    1. 235
    2. 2
    3. Pages: 424-428
  4. Type of Article: Article
  1. Abstract:

    In this study, we demonstrate that the active site architecture of the human glutathione (GSH) S-transferase Pi (GSTP1-1) accounts for its enantioselectivity in the GSH conjugation of 7 beta,8 alpha-dihydroxy-9 alpha,10 alpha-oxy-7,8,9,10-tetrahydrobenzo(a) pyrene (anti-BPDE), the ultimate carcinogen of benzo(a)pyrene. Furthermore, we report that the two polymorphic forms of human GSTP1-1, differing in their primary structure by a single amino acid in position 104, have disparate activity toward (+)-anti-BPDE, which can also be rationalized in terms of their active site structures. When concentration of (+)-anti-BPDE, which among four BPDE isomers is the most potent carcinogen, was varied and GSH concentration was kept constant at 2 mM (saturating concentration), both forms of hGSTP1-1 [hGSTP1-1(V104) and hGSTP1-1(I104)] obeyed Michaelis-Menten kinetics. The V-max of GSH conjugation of (+)-anti-BPDE was approximately 3.4 fold higher for hGSTP1-1(V104) than for hGSTP1-1(I104). Adherence to Michaelis-Menten kinetics was also observed for both isoforms when (-)-anti-BPDE, which is a weak carcinogen, was used as the variable substrate. However, (-)-anti-BPDE was a relatively poor substrate for both isoforms as compared with (+)-anti-BPDE. Moreover, there were no significant differences between hGSTP1-1(V104) and hGSTP1-1(I104) in either V-max or K-m for (-)-anti-BPDE. The mechanism of differences in kinetic properties and enantioselectivity of hGSTP1-1 variants toward anti-BPDE was investigated by modeling of the two proteins with conjugation product molecules in their active sites. Molecular modeling studies revealed that the differences in catalytic properties of hGSTP1-1 variants as well as the enantioselectivity of hGSTP1-1 in the GSH conjugation of anti-BPDE can be rationalized in terms of the architecture of their active sites. Our results suggest that the population polymorphism of hGSTP1-1 variants with disparate enzyme activities may, at least in part, account for the differential susceptibility of individuals to carcinogens such as anti-BPDE and possibly other similar carcinogens. (C) 1997 Academic Press. [References: 23]

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