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大鼠感觉神经元中的钙诱导钙释放

Calcium-induced calcium release in rat sensory neurons.

作者信息

Shmigol A, Verkhratsky A, Isenberg G

机构信息

Bogomoletz Institute of Physiology, Kiev-24, Ukraine.

出版信息

J Physiol. 1995 Dec 15;489 ( Pt 3)(Pt 3):627-36. doi: 10.1113/jphysiol.1995.sp021078.

DOI:10.1113/jphysiol.1995.sp021078
PMID:8788929
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1156834/
Abstract
  1. In isolated dorsal root ganglion cells (DRG neurons), changes in the concentration of global cytosolic Ca2+ (delta [Ca2+]c) were measured by the fluorescence of K5-indo-1. Depolarizations from -60 to 0 mV (500 ms) and Ca2+ influx through Ca2+ channels (ICa) increased [Ca2+]c by 480 +/- 113 nM, the peak occurring 542 +/- 76 ms (mean +/- S.E.M.) after repolarization. 2. Ryanodine (10 microM) reduced depolarization-induced delta [Ca2+]c by up to 80% and blocked delta [Ca2+]c induced by 20 mM caffeine. 3. Peak delta [Ca2+]c and peak ICa followed a similar bell-shaped voltage dependence. Removal of extracellular Ca2+ abolished depolarization-induced delta [Ca2+]c; its elevation from 2 to 8 mM increased peak ICa by 30% and delta [Ca2+]c by 108%. 4. Ca2+ influx at 0 mV was graded by pulse durations between 20 and 500 ms. Up to 200 ms, delta [Ca2+]c increased linearly with Ca2+ influx. Depolarizations longer than 200 ms induced a supralinear increase in delta [Ca2+]c that was abolished by caffeine (20 mM). 5. The supralinear increase in delta [Ca2+]c and the caffeine-induced delta [Ca2+]c were measured only in thirteen of nineteen DRG neurons; in the other six of nineteen cells both properties were absent. The results suggest that Ca(2+)-induced Ca2+ release (CICR) is expressed differently in different populations of DRG neurons. 6. A single action potential did not significantly increase [Ca2+]c. Trains of stimuli (20 Hz) induced delta [Ca2+]c that linearly increased with the number of action potentials. Delta [Ca2+]c due to 100 action potentials had a significant ryanodine-sensitive component. 7. It is discussed that CICR can contribute to the depolarization-induced [Ca2+]c, provided the Ca2+ influx lasts for a certain minimum period of time.
摘要
  1. 在分离的背根神经节细胞(DRG神经元)中,通过K5-indo-1的荧光测量细胞溶质中全局Ca2+浓度的变化(δ[Ca2+]c)。从-60 mV到0 mV的去极化(500毫秒)以及通过Ca2+通道(ICa)的Ca2+内流使[Ca2+]c增加了480±113 nM,峰值出现在复极化后542±76毫秒(平均值±标准误)。2. 10 μM的ryanodine可使去极化诱导的δ[Ca2+]c降低多达80%,并阻断20 mM咖啡因诱导的δ[Ca2+]c。3. 峰值δ[Ca2+]c和峰值ICa呈现相似的钟形电压依赖性。去除细胞外Ca2+可消除去极化诱导的δ[Ca2+]c;将其浓度从2 mM提高到8 mM可使峰值ICa增加30%,δ[Ca2+]c增加108%。4. 在0 mV时的Ca2+内流由20至500毫秒的脉冲持续时间分级。在200毫秒以内,δ[Ca2+]c随Ca2+内流呈线性增加。持续时间超过200毫秒的去极化诱导δ[Ca2+]c超线性增加,这一增加被20 mM咖啡因消除。5. 在19个DRG神经元中,只有13个测量到了δ[Ca2+]c的超线性增加和咖啡因诱导的δ[Ca2+]c;在另外6个细胞中,这两种特性均不存在。结果表明,Ca(2+)诱导的Ca2+释放(CICR)在不同群体的DRG神经元中表现不同。6. 单个动作电位并未显著增加[Ca2+]c。刺激串(20 Hz)诱导的δ[Ca2+]c随动作电位数量呈线性增加。由100个动作电位引起的δ[Ca2+]c具有显著的ryanodine敏感成分。7. 讨论了只要Ca2+内流持续一定最短时间,CICR就可能对去极化诱导的[Ca2+]c有贡献。

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