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Calcium-activated force responses in fast- and slow-twitch skinned muscle fibres of the rat at different temperatures.大鼠不同温度下快肌和慢肌去皮肤肌纤维的钙激活力反应
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A Ca-dependent Cl- conductance in cultured mouse spinal neurones.培养的小鼠脊髓神经元中的一种钙依赖性氯电导。
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A transient calcium-dependent chloride current in the immature Xenopus oocyte.非洲爪蟾未成熟卵母细胞中的一种瞬时钙依赖性氯电流。
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8
A patch-clamp study of bovine chromaffin cells and of their sensitivity to acetylcholine.一项关于牛嗜铬细胞及其对乙酰胆碱敏感性的膜片钳研究。
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Properties of single calcium-activated potassium channels in cultured rat muscle.培养的大鼠肌肉中单个钙激活钾通道的特性
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10
Calcium-mediated inactivation of the calcium conductance in caesium-loaded giant neurones of Aplysia californica.钙介导的加州海兔铯负载巨神经元中钙电导的失活
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发育中的雏鸡骨骼肌中一种钙和电压依赖性氯电流。

A calcium- and voltage-dependent chloride current in developing chick skeletal muscle.

作者信息

Hume R I, Thomas S A

机构信息

Department of Biology, University of Michigan, Ann Arbor 48109.

出版信息

J Physiol. 1989 Oct;417:241-61. doi: 10.1113/jphysiol.1989.sp017799.

DOI:10.1113/jphysiol.1989.sp017799
PMID:2482883
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1189264/
Abstract
  1. Depolarization of embryonic chick myotubes from negative potentials elicits a rapid spike followed by a long-duration after-potential. The ionic basis of the long-duration after-potential was examined by making intracellular recordings from cultured myotubes, and by making whole-cell patch-clamp recordings from myoblasts and myoballs. 2. The peak potential of the long-duration after-potential varied with the chloride gradient, suggesting that a conductance increase to chloride is involved in generating the after-potential. However, a calcium current was also implicated, since lowering the extracellular calcium or replacing extracellular calcium with cobalt abolished the after-potential. 3. When extracellular calcium was replaced with strontium or barium, short-duration spikes similar to calcium spikes were observed, but only strontium was able to support activation of long-duration after-potentials. Intracellular injection of calcium or strontium into myotubes bathed in calcium-free extracellular solutions restored the ability of depolarization to evoke an after-potential. Intracellular injection of magnesium, barium, nickel or cobalt did not restore this ability. These experiments strongly suggested that the long-duration after-potential was due to a calcium- and voltage-activated chloride current. 4. Whole-cell voltage-clamp recordings from myoballs and myoblasts showed that a large chloride conductance could be activated by depolarization when the internal free calcium concentration was buffered at levels greater than 10(-7) M. At 2.5 x 10(-7) M-calcium, the voltage dependence of activation was steepest in the range of -30 to -20 mV and the activation kinetics varied with the membrane potential. The time to half-maximal activation ranged from 0.1 s at positive potentials to greater than 1 s at more negative potentials. The time constant for deactivation was approximately 1 s at -50 mV. No inactivation was observed. 5. The selectivity of the chloride current was measured by substituting other anions for chloride. The following permeability series was found: I- greater than NO3- greater than Br- greater than Cl- greater than acetate greater than F- greater than SO4- = glucuronate. Thus anion permeability decreased as the hydration radius increased. 6. Measurements of the resting potential of developing myoblasts and myotubes under 'physiological' conditions (37 degrees C, bicarbonate buffer) suggest that the after-potential acts to depolarize these cells 10-20 mV above their resting potential (approximately -60 mV) for several seconds. 7. We discuss the possibility that the long-duration after-potential may be involved in triggering myoblast fusion and in the generation of bursts of spontaneous contractions in developing myotubes.
摘要
  1. 胚胎期鸡肌管从负电位去极化会引发一个快速的尖峰,随后是一个持续时间较长的后电位。通过对培养的肌管进行细胞内记录,以及对成肌细胞和肌球进行全细胞膜片钳记录,研究了持续时间较长的后电位的离子基础。2. 持续时间较长的后电位的峰值电位随氯离子梯度而变化,这表明氯离子电导增加参与了后电位的产生。然而,钙电流也与之有关,因为降低细胞外钙或用钴替代细胞外钙会消除后电位。3. 当用锶或钡替代细胞外钙时,观察到类似于钙尖峰的短持续时间尖峰,但只有锶能够支持持续时间较长的后电位的激活。在无钙的细胞外溶液中培养的肌管内注射钙或锶,恢复了去极化引发后电位的能力。向肌管内注射镁、钡、镍或钴不能恢复这种能力。这些实验强烈表明,持续时间较长的后电位是由钙和电压激活的氯电流引起的。4. 对肌球和成肌细胞进行的全细胞膜片钳记录表明,当内部游离钙浓度缓冲在大于10^(-7) M的水平时,去极化可激活较大的氯电导。在2.5×10^(-7) M钙浓度下,激活的电压依赖性在-30至-20 mV范围内最陡峭,且激活动力学随膜电位而变化。半最大激活时间从正电位时的0.1秒到更负电位时的大于1秒不等。在-50 mV时失活时间常数约为1秒。未观察到失活现象。5. 通过用其他阴离子替代氯离子来测量氯电流的选择性。发现了以下通透性序列:I^(-)>NO3^(-)>Br^(-)>Cl^(-)>醋酸根>F^(-)>SO4^(2-) = 葡萄糖醛酸根。因此,阴离子通透性随水化半径增加而降低。6. 在“生理”条件(37℃,碳酸氢盐缓冲液)下对发育中的成肌细胞和肌管静息电位的测量表明,后电位的作用是使这些细胞在其静息电位(约-60 mV)之上去极化10 - 20 mV达数秒。7. 我们讨论了持续时间较长的后电位可能参与触发成肌细胞融合以及发育中的肌管中自发收缩爆发产生的可能性。