A Na+-activated K+ current (IK,Na) is present in guinea-pig but not rat ventricular myocytes

被引:0
|
作者
C. Lawrence
G. C. Rodrigo
机构
[1] Department of Physiology,
[2] School of Medical Sciences,undefined
[3] University of Otago,undefined
[4] Dunedin,undefined
[5] New Zealand e-mail: glenn.rodrigo@stonebow.otago.ac.nz Fax: +64-34797323,undefined
来源
Pflügers Archiv | 1999年 / 437卷
关键词
Key words Cardiac myocyte; Ca2+ channels; Ca2+ paradox; Intracellular sodium; K+ current; Membrane potential;
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摘要
 The effects of removing extracellular Ca2+ and Mg2+ on the membrane potential, membrane current and intracellular Na+ activity (aiNa) were investigated in guinea-pig and rat ventricular myocytes. Membrane potential was recorded with a patch pipette and whole-cell membrane currents using a single-electrode voltage clamp. Both guinea-pig and rat cells depolarize when the bathing Ca2+ and Mg2+ are removed and the steady-state aiNa increases rapidly from a resting value of 6.4± 0.6 mM to 33±3.8 mM in guinea-pig (n=9) and from 8.9±0.8 mM to 29.3±3.0 mM (n=5) in rat ventricular myocytes. Guinea-pig myocytes partially repolarized when, in addition to removal of the bathing Ca2+ and Mg2+, K+ was also removed, however rat cells remained depolarized. A large diltiazem-sensitive inward current was recorded in guinea-pig and rat myocytes, voltage-clamped at –20 mV, when the bathing divalent cations were removed. When the bathing K+ was removed after Ca2+ and Mg2+ depletion, a large outward K+ current developed in guinea-pig, but not in rat myocytes. This current had a reversal potential of –80±0.7 mV and was not inhibited by high Mg2+ or glybenclamide indicating that it is not due to activation of non-selective cation or adenosine triphosphate (ATP)-sensitive K channels. The current was not activated when Li+ replaced the bathing Na+ and was blocked by R-56865, suggesting that it was due to the activation of KNa channels.
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页码:831 / 838
页数:7
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