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J. Biol. Chem., Vol. 259, Issue 9, 5490-5494, 05, 1984
DA Otto
Following preincubation of isolated rat liver mitochondria in the absence
of substrate, the carnitine-independent oxidation of octanoate or butyrate
was markedly depressed when compared to rates observed with nonpreincubated
mitochondria. Carnitine addition prevented the inhibition of octanoate
oxidation but not that of butyrate. 2- Tetradecylglycidic acid or
Zwittergent 3-08 (Z3-08) completely blocked the effect of carnitine.
Replacement of ATP in the nonpreincubated incubation system with ADP
mimicked the effect of preincubation by inhibiting octanoate and butyrate
oxidation. This inhibition of octanoate oxidation was also prevented by
carnitine addition. There was a direct and causal relationship between the
ATP/ADP ratio of the total adenine nucleotide pool and the rate of
carnitine-independent octanoate oxidation in mitochondria. The depression
of octanoate oxidation was associated with a decrease in the
intramitochondrial AMP content and intra- and extramitochondrial ATP/ADP
ratios. In a cellular system, incubating isolated hepatocytes with fructose
or glycerol to lower the ATP/ADP ratio resulted in greater inhibition of
octanoate oxidation by 2-tetradecylglycidic acid. The data suggest that the
ATP/ADP ratio may have a role in determining the site of octanoate
activation and subsequent route of oxidation.
Relationship of the ATP/ADP ratio to the site of octanoate activation
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