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Evidence for two K+ currents activated upon hyperpolarization ofParamecium tetraurelia
Authors:Robin R. Preston  Yoshiro Saimi  Ching Kung
Affiliation:(1) Laboratory of Molecular Biology, University of Wisconsin-Madison, 53706 Madison, Wisconsin;(2) Department of Genetics, University of Wisconsin-Madison, 53706 Madison, Wisconsin
Abstract:Summary Hyperpolarization of voltage-clampedParamecium tetraurelia in K+ solutions elicits a complex of Ca2+ and K+ currents. The tail current that accompanies a return to holding potential (–40 mV) contains two K+ components. The tail current elicited by a step to –110 mV of ge50-msec duration contains fast-decaying (tauap3.5 msec) and slow-decaying (tauap20 msec) components. The reversal potential of both components shifts by 55–57 mV/10-fold change in external [K+], suggesting that they represent pure K+ currents. The dependence of the relative amplitudes of the two tail currents on duration of hyperpolarization suggests that the slow K+ current activates slowly and is sustained, whereas the fast current activates rapidly during hyperpolarization and then rapidly inactivates. Iontophoretic injection of a Ca2+ chelator, EGTA, specifically reduces slow tail-current amplitude without affecting the fast tail component. Both K+ currents are inhibited by extracellular TEA+ in a concentration-dependent, noncooperative manner, whereas the fast K+ current alone is inhibited by 0.7mm quinidine.
Keywords:inward rectification  voltage-dependent K+ current  Ca2+-dependent K+ current  Paramecium
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