4.6 Article

Free [ADP] and aerobic muscle work follow at least second order kinetics in rat gastrocnemius in vivo

Journal

JOURNAL OF BIOLOGICAL CHEMISTRY
Volume 275, Issue 9, Pages 6129-6134

Publisher

AMER SOC BIOCHEMISTRY MOLECULAR BIOLOGY INC
DOI: 10.1074/jbc.275.9.6129

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The relationship between free cytosolic [ADP] land [P-i]) and steady-state aerobic muscle work in rat gastrocnemius muscle in vivo using P-31 NMR was investigated. Anesthetized rats were ventilated and placed in a custom-built cradle fitted with a force transducer that could be placed into a 7-tesla NMR magnet. Muscle work was induced by supramaximal sciatic nerve stimulation that activated all fibers, Muscles were stimulated at 0.1, 0.2, 0.3, 0.4, 0.5, 0.8, 1.0, and 2.0 Hz until twitch force, phosphocreatine, and P-i were unchanged between two consecutive spectra acquired in 4-min blocks (8-12 min), Parallel bench experiments were performed to measure total tissue glycogen, lactate, total creatine, and pyruvate in freeze-clamped muscles after 10 min of stimulation at each frequency. Up to 0.5 Hz, there was no significant change in muscle glycogen, lactate, and the lactate/pyruvate ratios between 8-12 min. At 0.8 Hz, there was a 17% fall in glycogen and a 65% rise in the muscle lactate with a concomitant fall in pH, Above this frequency, glycogen fell rapidly, lactate continued to rise, and ATP and pH declined. On the basis of these force and metabolic measurements, we estimated the maximal mitochondrial capacity (V-max) to be 0.8 Hz. Free [ADP] was then calculated at each submaximal workload from measuring all the reactants of the creatine kinase equilibrium after adjusting the K'(CK) to the muscle temp (30 degrees C), pH, and pMg, We show that ADP (and P-i) and tension-time integral follow a Pill relationship with at least a second order function. The K-0.5 values for free [ADP] and [P-i] were 48 mu M and 9 mM, respectively. Our data did not fit any form of the Michaelis-Menten equation. We therefore conclude that free cytosolic [ADP] and [P-i] could potentially control steady-state oxidative phosphorylation in skeletal muscle in vitro.

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