Metal-directed affinity labeling of zinc(II), cobalt(II) and cadmium(II) horse liver alcohol dehydrogenases |
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| Authors: | Knut H. Dahl John S. McKinley-McKee |
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| Affiliation: | Department of Biochemistry, University of Oslo Norway |
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| Abstract: | The active site metal in horse liver alcohol dehydrogenase has been studied by metal-directed affinity labeling of the native zinc(II) enzyme and that substituted with cobalt(II) or cadmium(II). Reversible binding of bromoimidazolyl propionic acid to the cobalt enzyme blueshifts the visible absorption band originating from the catalytic cobalt atom at 655 to 630 nm. Binding of imidazole to the cobalt(II) enzyme redshifts the 655 nm band to 667 nm. Addition of bromoimidazolyl propionic acid blueshifts this 667 nm band back to 630 nm. This proves direct binding of the label to the active site metal in competition with imidazole. The affinity of the label for the reversible binding site in the three enzymes follows the order Zn ? Cd ? Co. After reversible complex formation, bromoimidazolyl propionic acid alkylates cysteine-46, one of the protein ligands to the active site metal. The nucleophilic reactivity of this metal-mercaptide bond in each reversible complex follows the order Co ? Zn ? Cd. |
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| Keywords: | Since this work only deals with the native zinc(II) and the fully substituted cobalt(II) or cadmium(II) enzymes, the terms zinc, cadmium, and cobalt enzyme refer to liver alcohol dehydrogenase with this metal in both the catalytic and the noncatalytic metal binding sites. Pipes, 1,4-piperazinediehthansulfonic acid Address reprint requests to Knut H. Dahl, Department of Biochemistry, University of Oslo, P.B. 1041, Blindern, Oslo 3, Norway. |
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