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本文引用的文献

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INFLUENCE OF LITHIUM IONS ON THE TRANSMEMBRANE POTENTIAL AND CATION CONTENT OF CARDIAC CELLS.锂离子对心肌细胞跨膜电位及阳离子含量的影响
J Gen Physiol. 1964 Jan;47(3):501-30. doi: 10.1085/jgp.47.3.501.
2
Activity-dependent changes of slow inward current in ventricular heart muscle.心室肌慢内向电流的活动依赖性变化。
Pflugers Arch. 1981 Oct;391(4):277-83. doi: 10.1007/BF00581507.
3
Relation between intracellular Na ion activity and tension of sheep cardiac Purkinje fibers exposed to dihydro-ouabain.暴露于二氢哇巴因的绵羊心脏浦肯野纤维细胞内钠离子活性与张力之间的关系
Biophys J. 1980 Feb;29(2):315-30. doi: 10.1016/S0006-3495(80)85135-6.
4
Existence of two transient outward currents in sheep cardiac Purkinje fibers.绵羊心脏浦肯野纤维中两种瞬时外向电流的存在。
Pflugers Arch. 1982 Feb;392(4):352-9. doi: 10.1007/BF00581631.
5
Kinetics of sodium ion induced calcium ion release in calcium ion loaded cardiac sarcolemmal vesicles: determination of initial velocities by stopped-flow spectrophotometry.钠离子诱导钙离子从钙离子负载的心肌肌膜囊泡中释放的动力学:通过停流分光光度法测定初始速度。
Biochemistry. 1982 Apr 13;21(8):1914-8. doi: 10.1021/bi00537a033.
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Inward current channels activated by intracellular Ca in cultured cardiac cells.培养心肌细胞中由细胞内钙激活的内向电流通道。
Nature. 1981 Dec 24;294(5843):752-4. doi: 10.1038/294752a0.
7
The slow inward current, isi, in the rabbit sino-atrial node investigated by voltage clamp and computer simulation.通过电压钳和计算机模拟研究了家兔窦房结中的缓慢内向电流isi。
Proc R Soc Lond B Biol Sci. 1984 Sep 22;222(1228):305-28. doi: 10.1098/rspb.1984.0066.
8
The dependence of slow inward current in Purkinje fibres on the extracellular calcium-concentration.浦肯野纤维中缓慢内向电流对细胞外钙浓度的依赖性。
J Physiol. 1967 Sep;192(2):479-92. doi: 10.1113/jphysiol.1967.sp008310.
9
The slow repolarization phase of the action potential in rat heart.大鼠心脏动作电位的缓慢复极化阶段。
J Physiol. 1985 Mar;360:13-25. doi: 10.1113/jphysiol.1985.sp015601.
10
Calcium channels: molecular pharmacology, structure and regulation.钙通道:分子药理学、结构与调控
J Membr Biol. 1988 Sep;104(2):81-105. doi: 10.1007/BF01870922.

犬心室肌慢内向电流的收缩相关成分及其与Na(+)-Ca2+交换的关系。

A contraction-related component of slow inward current in dog ventricular muscle and its relation to Na(+)-Ca2+ exchange.

作者信息

Simurda J, Simurdová M, Bravený P, Sumbera J

机构信息

Department of Physiology, Masaryk University, Brno, Czechoslovakia.

出版信息

J Physiol. 1992 Oct;456:49-70. doi: 10.1113/jphysiol.1992.sp019326.

DOI:10.1113/jphysiol.1992.sp019326
PMID:1293284
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1175671/
Abstract
  1. The slow inward current component related to contraction (Isic) was studied in voltage clamp experiments on canine ventricular trabeculae at 30 degrees C with the aims of (a) estimating its relation to electrogenic Na(+)-Ca2+ exchange and (b) comparing it with similar currents as reported in cardiac myocytes. 2. Isic may be recorded under conditions of augmented contractility in response to depolarizing pulses below the threshold of the classic slow inward current (presumably mediated by L-type Ca2+ channels). In responses to identical depolarizing clamp pulses the peak value of Isic is directly related to the amplitude of contraction (Fmax). Isic peaks about 60 ms after the onset of depolarization and declines with a half-time of about 110 ms. 3. The voltage threshold of Isic activation is the same as the threshold of contraction. The positive inotropic clamp preconditions shift both thresholds to more negative values of membrane voltage, i.e. below the threshold of the classic slow inward current. 4. Isic may also be recorded as a slowly decaying inwardly directed current 'tail' after depolarizing pulses. In this representation the peak value of Isic changes with duration of the depolarizing pulses, again in parallel with Fmax. In response to pulses shorter than 100 ms both variables increase with depolarization time. If initial conditions remain constant, further prolongation of the pulse does not significantly influence either one (tail currents follow a common envelope). 5. Isic differs from classic slow inward current by: (a) its direct relation to contraction, (b) the slower decay of the current tail on repolarization, (c) slower restitution corresponding to the mechanical restitution, (d) its relative insensitivity to Ca(2+)-blocking agents (the decrease of Isic is secondary to the negative inotropic of Ca(2+)-blocking agents (the decrease of Isic is secondary to the negative inotropic effect) and (e) its disappearance after Sr2+ substitution for Ca2+. 6. The manifestations of Isic in multicellular preparations do not differ significantly from those reported in isolated myocytes (in contrast to calcium current). 7. The analysis of the correlation between Isic and Fmax transients during trains of identical test depolarizing pulses at variable extra- and intracellular ionic concentrations (changes of [Ca2+]o, 50% Li+ substitution for Na+, strophanthidin) indicate that the observed effects conform to the predictions based on a quantitative model of Na(+)-Ca2+ exchange. 8. It is concluded that Isic is activated by a transient increase of [Ca2+]i, in consequence of the release from the reticular stores.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 在30℃下对犬心室肌小梁进行电压钳实验,研究与收缩相关的缓慢内向电流成分(Isic),目的是:(a)评估其与电致Na(+)-Ca2+交换的关系;(b)将其与心肌细胞中报道的类似电流进行比较。2. 在经典缓慢内向电流(可能由L型Ca2+通道介导)阈值以下的去极化脉冲作用下,可在收缩增强的条件下记录到Isic。对于相同的去极化钳制脉冲,Isic的峰值与收缩幅度(Fmax)直接相关。Isic在去极化开始后约60毫秒达到峰值,并以约110毫秒的半衰期下降。3. Isic激活的电压阈值与收缩阈值相同。正性肌力钳制预处理使两个阈值都移向膜电压更负的值,即低于经典缓慢内向电流的阈值。4. 在去极化脉冲后,Isic也可记录为缓慢衰减的内向电流“尾”。在这种表现形式中,Isic的峰值随去极化脉冲的持续时间而变化,同样与Fmax平行。对于短于100毫秒的脉冲,两个变量都随去极化时间增加。如果初始条件保持不变,脉冲的进一步延长对两者均无显著影响(尾电流遵循共同的包络线)。5. Isic与经典缓慢内向电流的不同之处在于:(a)它与收缩直接相关;(b)复极化时电流尾的衰减较慢;(c)与机械恢复相对应的较慢恢复;(d)它对Ca(2+)阻断剂相对不敏感(Isic的降低继发于Ca(2+)阻断剂的负性肌力作用);(e)用Sr2+替代Ca2+后它消失。6. Isic在多细胞制剂中的表现与在分离的心肌细胞中报道的表现没有显著差异(与钙电流相反)。7. 在细胞外和细胞内离子浓度可变([Ca2+]o变化、50% Li+替代Na+、毒毛花苷)的相同测试去极化脉冲序列期间分析Isic和Fmax瞬变之间的相关性,表明观察到的效应符合基于Na(+)-Ca2+交换定量模型的预测。8. 得出结论,Isic由肌浆网释放导致的[Ca2+]i瞬时增加激活。(摘要截短于400字)