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兔心脏浦肯野纤维中在无钠钙交换情况下瞬时内向电流的离子机制

Ionic mechanisms of transient inward current in the absence of Na(+)-Ca2+ exchange in rabbit cardiac Purkinje fibres.

作者信息

Han X, Ferrier G R

机构信息

Department of Pharmacology, Dalhousie University, Halifax, Nova Scotia, Canada.

出版信息

J Physiol. 1992 Oct;456:19-38. doi: 10.1113/jphysiol.1992.sp019324.

Abstract
  1. Membrane currents were measured with a two-microelectrode technique in voltage clamped rabbit cardiac Purkinje fibres under conditions known to cause intracellular calcium overload and to eliminate or minimize Na(+)-Ca2+ exchange. 2. Increasing [Ca2+]o from 2.5 to 5 mM or above and substituting external sodium with either sucrose, choline or Li+ induced an oscillatory transient inward current (TI) which peaked 200-300 ms after repolarization from a previous depolarizing pulse. The TI quickly disappeared upon return to normal Tyrode solution. Both the rate and configuration of action potentials of Purkinje fibres also returned to control upon return to Tyrode solution after 30 min of high Ca2+ exposure, if the Ca2+ concentration was 30 mM or less. 3. The TI in Na(+)-free solution was Ca2+ dependent. Either zero or low (2.5 mM) [Ca2+]o, or replacement of [Ca2+]o by BaCl prevented induction of the TI current upon repolarization from a previous depolarizing pulse. 4. In the presence of 30 mM-CaCl2 and with choline chloride as the substitute for NaCl, TI had a distinct reversal potential (Erev) of -25 mV. The time-to-peak TI, either inward or outward, did not shift significantly with change in voltage. Both inward and outward TI were simultaneously abolished by exposure to 1 microM-ryanodine, suggesting they were both activated by transient release of Ca2+ from the sarcoplasmic reticulum. The occurrence of TI in the absence of [Na+]o is not compatible with an electrogenic Na(+)-Ca2+ exchange mechanism. The existence of a clear-cut reversal potential suggests that an ionic channel may be responsible for the TI under these conditions. 5. Both the magnitude of peak TI and the Erev were affected by changes of CaCl2 concentration. (i) Under steady-state conditions, peak inward TI was significantly increased when the [Ca2+]o was elevated from 5 to 15 mM. The peak TI in the outward direction was significantly increased when [Ca2+]o was elevated from 15 to 30 mM; however, the difference in peak inward TI at 15 and 30 mM [Ca2+]o was small. (ii) Clear-cut reversals of TI were found at Ca2+ concentrations of 10 mM (Erev = -19.5 mV) or greater, and elevation of [Ca2+]o to 20, 30, 50 and 105 mM shifted the Erev to more negative potentials. (iii) In the presence of 5 mM [Ca2+]o the inward TI declined to zero at about -30 mV, and test voltages between -55 and +5 mV failed to reveal a distinct outward TI.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 在已知会导致细胞内钙超载并消除或最小化钠钙交换的条件下,采用双微电极技术在电压钳制的兔心脏浦肯野纤维中测量膜电流。2. 将细胞外钙浓度([Ca2+]o)从2.5 mM增加到5 mM或更高,并用蔗糖、胆碱或锂离子替代细胞外钠,会诱发一种振荡性瞬时内向电流(TI),该电流在先前去极化脉冲复极化后200 - 300毫秒达到峰值。回到正常台氏液后,TI迅速消失。如果钙浓度为30 mM或更低,在高钙暴露30分钟后回到台氏液时,浦肯野纤维动作电位的速率和形态也恢复到对照水平。3. 在无钠溶液中的TI依赖于钙。零或低(2.5 mM)的[Ca2+]o,或用BaCl2替代[Ca2+]o,可防止在先前去极化脉冲复极化时诱发TI电流。4. 在存在30 mM - CaCl2且用氯化胆碱替代NaCl的情况下,TI有一个明显的反转电位(Erev)为 - 25 mV。内向或外向TI的峰值时间不会随电压变化而显著改变。暴露于1 microM的ryanodine可同时消除内向和外向TI,表明它们均由肌浆网中钙的瞬时释放激活。在无[Na+]o时TI的出现与电致钠钙交换机制不相符。明确的反转电位表明在这些条件下离子通道可能是TI的原因。5. 峰值TI的大小和Erev均受CaCl2浓度变化的影响。(i)在稳态条件下,当[Ca2+]o从5 mM升高到15 mM时,内向峰值TI显著增加。当[Ca2+]o从15 mM升高到30 mM时,外向峰值TI显著增加;然而,15 mM和30 mM [Ca2+]o时内向峰值TI的差异较小。(ii)在钙浓度为10 mM(Erev = - 19.5 mV)或更高时发现TI有明确的反转,并且将[Ca2+]o升高到20、30、50和105 mM会使Erev向更负的电位移动。(iii)在存在5 mM [Ca2+]o时,内向TI在约 - 30 mV时降至零,并且在 - 55 mV至 + 5 mV之间的测试电压未能显示出明显的外向TI。(摘要截于400字)

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