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JBC, Vol. 250, Issue 17, 6640-6647, Sep, 1975
N. E. Garrett and H. S. Penefsky
Beef heart mitochondrial ATPase (F1) contained 2 mol of ADP and 1 mol of
ATP/mol of enzyme, which resisted removal by Sephadex chromatography with
dilute buffers or repeated precipitation with ammonium sulfate. The native
enzyme also contained two apparently equivalent binding sites, which
participated in readily reversible binding of adenyl-5'-ylimidodiphosphate
(AMP-P(NH)P), with a Kd of 1.3 mum. The failure of AMP-P(NH)P to compete
effectively with ADP for binding sites on F1 may be related to the failure
of the analog to inhibit oxidative phosphorylation. Virtually complete
removal of all adenine nucleotides from F1 occurred when the enzyme was
chromatographed on columns of Sephadex equilibrated with 50% glycerol. No
loss in ATPase activity was observed following removal of nucleotides from
the enzyme, which was then capable of binding more than 4 mol of ADP and
almost 5 mol of AMP-P(NH)P/mol of protein. Subsequent chromatography on
columns of Sephadex equilibrated with dilute buffers containing Mg2+
removed only 1.5 mol of ADP and no AMP-P(NH)P from the enzyme.
Reconstitution of F1 with ADP or with almost 5 mol of AMP-P(NH)P resulted
in preparations that exhibited an undiminished capacity to restore
oxidative phosphorylation in F1-deficient submitochondrial particles.
Interaction of adenine nucleotides with multiple binding sites on beef heart mitochondrial adenosine triphosphatase
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