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J. Biol. Chem., Vol. 255, Issue 9, 3994-4000, May, 1980
RP Casey, M Thelen and A Azzi
We have investigated the covalent binding of dicyclohexylcarbodiimide
(DCCD) to cytochrome c oxidase in relation to its inhibition of
ferrocytochrome c-induced H+ translocation by the enzyme reconstituted in
lipid vesicles. DCCD bound to the reconstituted oxidase in a time- and
concentration-dependent manner which appeared to correlate with its
inhibition of H+ translocation. In both reconstituted vesicles and intact
beef heart mitochondria, the DCCD-binding site was located in subunit III
of the oxidase. The apolar nature of DCCD and relatively minor effects of
the hydrophilic carbodiimide, 1-ethyl-(3-
dimethylaminopropyl)-carbodiimide, on H+ translocation by the oxidase
indicate that the site of action of DCCD is hydrophobic. DCCD also bound to
isolated cytochrome c oxidase, though in this case subunits III and IV were
labeled. The maximal overall stoichiometries of DCCD molecules bound per
cytochrome c oxidase molecule were 1 and 1.6 for the reconstituted and
isolated enzymes, respectively. These findings point to subunit III of
cytochrome c oxidase having an important role in H+ translocation by the
enzyme and indicate that DCCD may prove a useful tool in elucidating the
mechanism of H+ pumping.
Dicyclohexylcarbodiimide binds specifically and covalently to cytochrome c oxidase while inhibiting its H+-translocating activity
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