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本文引用的文献

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Calcium tolerant ventricular myocytes prepared by preincubation in a "KB medium".通过在“KB培养基”中预孵育制备的耐钙心室肌细胞。
Pflugers Arch. 1982 Oct;395(1):6-18. doi: 10.1007/BF00584963.
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Pharmacological dissection of charge movement in frog skeletal muscle fibers.蛙骨骼肌纤维中电荷移动的药理学剖析
Biophys J. 1982 Jul;39(1):119-22. doi: 10.1016/S0006-3495(82)84498-6.
3
The effects of tetracaine on the membrane currents and contraction of frog atrial muscle.丁卡因对蛙心房肌膜电流和收缩的影响。
J Physiol. 1981 Aug;317:475-86. doi: 10.1113/jphysiol.1981.sp013837.
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Dielectric components of charge movements in skeletal muscle.骨骼肌中电荷运动的介电成分。
J Physiol. 1981;313:187-205. doi: 10.1113/jphysiol.1981.sp013658.
5
The shortening of the action potential by DNP in guinea-pig ventricular myocytes is mediated by an increase of a time-independent K conductance.二硝基酚(DNP)使豚鼠心室肌细胞动作电位缩短是由一种非时间依赖性钾电导增加介导的。
Pflugers Arch. 1983 Jun 1;397(4):251-9. doi: 10.1007/BF00580257.
6
Delayed rectification in the cardiac Purkinje fiber is not activated by intracellular calcium.心脏浦肯野纤维中的延迟整流不受细胞内钙的激活。
Biophys J. 1984 Apr;45(4):837-9. doi: 10.1016/S0006-3495(84)84227-7.
7
Effects of tetracaine on charge movements and calcium signals in frog skeletal muscle fibers.丁卡因对青蛙骨骼肌纤维电荷移动和钙信号的影响。
Proc Natl Acad Sci U S A. 1983 Mar;80(5):1477-81. doi: 10.1073/pnas.80.5.1477.
8
A transient outward current related to calcium release and development of tension in elephant seal atrial fibres.与海象心房纤维中钙释放及张力发展相关的瞬时外向电流。
J Physiol. 1984 Dec;357:267-92. doi: 10.1113/jphysiol.1984.sp015500.
9
Maximal upstroke velocity as an index of available sodium conductance. Comparison of maximal upstroke velocity and voltage clamp measurements of sodium current in rabbit Purkinje fibers.最大上升速度作为可用钠电导的指标。兔浦肯野纤维中最大上升速度与钠电流电压钳测量值的比较。
Circ Res. 1984 Jun;54(6):636-51. doi: 10.1161/01.res.54.6.636.
10
Single channel analysis of the inward rectifier K current in the rabbit ventricular cells.兔心室肌细胞内向整流钾电流的单通道分析
Jpn J Physiol. 1983;33(6):1039-56. doi: 10.2170/jjphysiol.33.1039.

丁卡因对单个豚鼠心室肌细胞的电生理效应。

Electrophysiological effects of tetracaine in single guinea-pig ventricular myocytes.

作者信息

Carmeliet E, Morad M, Van der Heyden G, Vereecke J

出版信息

J Physiol. 1986 Jul;376:143-61. doi: 10.1113/jphysiol.1986.sp016146.

DOI:10.1113/jphysiol.1986.sp016146
PMID:2432230
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1182791/
Abstract

The effect of tetracaine on the ionic current in enzymatically dissociated single guinea-pig ventricular cells was studied using a two micro-electrode voltage-clamp technique. The myocytes were pre-incubated with Cs+ and the experiments were performed at room temperature in order to reduce the contribution of the delayed outward current. Tetracaine decreased the maximum rate of rise of the action potential with a dissociation constant (KD) strongly dependent on the holding potential (0.77 microM at -80 mV, and 6.2 microM at -95 mV). Application of 20 microM-tetracaine resulted in about a 50% reduction of the inwardly rectifying K+ current, while ten times higher concentrations were required to suppress the delayed K+ current. The inactivation time course of the Ca2+ current could be fitted with two exponentials, with time constants tau f = 15 ms and tau s = 150 ms at around 0 mV. Tetracaine decreased the amplitude of the Ca2+ current and speeded its decay. This effect was found to be primarily due to a marked inhibition of the amplitude of the slowly inactivating component (apparent KD = 80 microM, nH = 2). The drug had little effect on the time constants of the two components of Ca2+ channel inactivation. When Sr2+ or Ba2+ were the charge carriers, inactivation of the Ca2+ channel was again fitted with a fast and a slow exponential. In addition, a maintained (or very slowly inactivating) component was present. Tetracaine not only suppressed the amplitudes of the slowly inactivating and the maintained components, but also decreased the time constant of the slowly inactivating component. The results are consistent with a direct effect of tetracaine on the high threshold Ca2+ channel and do not support indirect effects of the drug secondary to suppression of Ca2+ release from internal stores.

摘要

采用双微电极电压钳技术研究了丁卡因对酶解分离的单个豚鼠心室肌细胞离子电流的影响。心肌细胞用Cs+预孵育,并在室温下进行实验,以减少延迟外向电流的影响。丁卡因降低动作电位的最大上升速率,其解离常数(KD)强烈依赖于钳制电位(-80 mV时为0.77 μM,-95 mV时为6.2 μM)。应用20 μM丁卡因导致内向整流K+电流降低约50%,而抑制延迟K+电流则需要高10倍的浓度。Ca2+电流的失活时间进程可用两个指数拟合,在约0 mV时,时间常数τf = 15 ms,τs = 150 ms。丁卡因降低Ca2+电流的幅度并加速其衰减。发现这种作用主要是由于对缓慢失活成分的幅度有明显抑制(表观KD = 80 μM,nH = 2)。该药物对Ca2+通道失活的两个成分的时间常数影响很小。当Sr2+或Ba2+作为载流子时,Ca2+通道的失活再次可用一个快指数和一个慢指数拟合。此外,还存在一个持续(或非常缓慢失活)的成分。丁卡因不仅抑制缓慢失活成分和持续成分的幅度,还降低缓慢失活成分的时间常数。结果与丁卡因对高阈值Ca2+通道的直接作用一致,不支持该药物继发于抑制细胞内钙库释放Ca2+的间接作用。