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Circulation Research. 1995;76:790-801

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(Circulation Research. 1995;76:790-801.)
© 1995 American Heart Association, Inc.


Articles

Effects of Action Potential Duration on Excitation-Contraction Coupling in Rat Ventricular Myocytes

Action Potential Voltage-Clamp Measurements

R. A. Bouchard, R. B. Clark, W. R. Giles

From the Departments of Medical Physiology and Medicine, The University of Calgary, Alberta, Canada.

Correspondence to W.R. Giles, 3330 Hospital Dr NW, Calgary, Alberta, Canada T2N 4N1.

Abstract Although each of the fundamental processes involved in excitation-contraction coupling in mammalian heart has been identified, many quantitative details remain unclear. The initial goal of our experiments was to measure both the transmembrane Ca2+ current, which triggers contraction, and the Ca2+ extrusion due to Na+-Ca2+ exchange in a single ventricular myocyte. An action potential waveform was used as the command for the voltage-clamp circuit, and the membrane potential, membrane current, [Ca2+]i, and contraction (unloaded cell shortening) were monitored simultaneously. Ca2+-dependent membrane current during an action potential consists of two components: (1) Ca2+ influx through L-type Ca2+ channels (ICa-L) during the plateau of the action potential and (2) a slow inward tail current that develops during repolarization negative to {approx}-25 mV and continues during diastole. This slow inward tail current can be abolished completely by replacement of extracellular Na+ with Li+, suggesting that it is due to electrogenic Na+-Ca2+ exchange. In agreement with this, the net charge movement corresponding to the inward component of the Ca2+-dependent current (ICa-L) was approximately twice that during the slow inward tail current, a finding that is predicted by a scheme in which the Ca2+ that enters during ICa is extruded during diastole by a 3 Na+–1 Ca2+ electrogenic exchanger. Action potential duration is known to be a significant inotropic variable, but the quantitative relation between changes in Ca2+ current, action potential duration, and developed tension has not been described in a single myocyte. We used the action potential voltage-clamp technique on ventricular myocytes loaded with indo 1 or rhod 2, both Ca2+ indicators, to study the relation between action potential duration, ICa-L, and cell shortening (inotropic effect). A rapid change from a "short" to a "long" action potential command waveform resulted in an immediate decrease in peak ICa-L and a marked slowing of its decline (inactivation). Prolongation of the action potential also resulted in slowly developing increases in the magnitude of Ca2+ transients (145±2%) and unloaded cell shortening (4.0±0.4 to 7.6±0.4 µm). The time-dependent nature of these effects suggests that a change in Ca2+ content (loading) of the sarcoplasmic reticulum is responsible. Measurement of [Ca2+]i by use of rhod 2 showed that changes in the rate of rise of the [Ca2+]i transient (which in rat ventricle is due to the rate of Ca2+ release from the sarcoplasmic reticulum) were closely correlated with changes in the magnitude and the time course of ICa-L. These findings demonstrate that Ca2+ release from the sarcoplasmic reticulum can be modulated by the action potential waveform as a result of changes in ICa-L.


Key Words: action potential duration • action potential clamp • excitation-contraction coupling • Ca2+ current • Na+-Ca2+ exchange • intracellular Ca2+




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