Abstract
Inactivation of the membrane-bound ATPase by tight ADP binding was studied under nonenergized conditions. The energy state of the system was controlled either by omitting MgCl2, preventing ATP hydrolysis, or by addition of an uncoupler which dissipates the {Mathematical expression}. In the absence of Mg2+, ATP prevents the inactivation of the enzyme by ADP, in a competitive manner. This effect of ATP resembles that of GDP with Mg2+ present. In the presence of nigericin, Mg2+, and ATP, inactivation occurs after a 10-15-sec interval, during which the enzyme is able to hydrolyze ATP at a relatively rapid rate. The degree of inactivation is proportional to the level of bound ADP detected. This behavior is different from that of the coupled ATPase (no uncoupler added), where inactivation is attained only upon exhaustion of the ATP by its hydrolysis, despite the finding that ADP binds tightly to the active ATPase at all stages of the reaction. Higher levels of tightly bound ADP were detected in the presence of an uncoupler. We suggest that the interval during which the enzyme becomes inactive is that required for the enzyme to generate and bind ADP, and to change from the active to the inactive conformation. These results support the mechanism suggested previously for the modulation of the ATPase by tight nucleotide binding.
Original language | English |
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Pages (from-to) | 467-478 |
Journal | Journal of Bioenergetics and Biomembranes |
Volume | 14 |
Issue number | 5-6 |
DOIs | |
State | Published - 1 Dec 1982 |
Keywords
- ATP hydrolysis
- ATP synthetase
- ATPase
- Chloroplasts
- P-ATP exchange
- enzyme modulation
- nigericin
- tightly bound ADP
- tightly bound nucleotides
- uncoupler
ASJC Scopus subject areas
- Physiology
- Cell Biology