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兔心脏单个浦肯野细胞中的胞内钙离子瞬变及钙离子依赖的氯离子电流

[Ca2+]i transients and [Ca2+]i-dependent chloride current in single Purkinje cells from rabbit heart.

作者信息

Sipido K R, Callewaert G, Carmeliet E

机构信息

Laboratory of Physiology, Katholieke Universiteit Leuven, Belgium.

出版信息

J Physiol. 1993 Aug;468:641-67. doi: 10.1113/jphysiol.1993.sp019793.

DOI:10.1113/jphysiol.1993.sp019793
PMID:8254529
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1143848/
Abstract
  1. Single Purkinje cells, enzymatically isolated from rabbit ventricle, were studied under whole-cell voltage clamp and internally perfused with the fluorescent Ca2+ indicator, indo-1 (100 microM). 2. Fast [Ca2+]i transients were elicited by brief depolarizations from a holding voltage of -45 mV and by repolarization from very positive potentials. The peak [Ca2+]i-voltage relation was bell-shaped with a peak around +10 mV. 3. [Ca2+]i transients were completely blocked by the Ca2+ channel antagonist, nisoldipine (10 microM) and were very small when Ca2+ release from the sarcoplasmic reticulum (SR) was prevented by superfusion of cells by caffeine (1 mM) or ryanodine (10 microM). A fast application of caffeine induced a transient increase in [Ca2+]i. These results suggest [Ca2+]i transients are due to Ca(2+)-induced Ca2+ release from the SR. 4. Rate of decline of the [Ca2+]i transient was voltage dependent, suggesting contribution of the Na(+)-Ca2+ exchanger to Ca2+ efflux. At very positive potentials (> +60 mV), Ca2+ influx through the Na(+)-Ca2+ exchanger could be observed. 5. A transient outward current was observed at potentials positive to +10 mV, but only if depolarizing pulses were accompanied by a [Ca2+]i transient. 6. When the amplitude of the [Ca2+]i transient was changed by (1) changes in [Ca2+]o, (2) changes in frequency of depolarization or (3) conditioning prepulses, the amplitude of the outward current changed in the same direction. This suggests activation of the current is dependent on and graded by [Ca2+]i. 7. The outward current was observed in K(+)-free solutions, in the presence of Cs+ and TEA+, and was not blocked by 4-aminopyridine (10 mM). In contrast, DIDS (100 microM) decreased the outward current by 70 +/- 20% (mean +/- S.D., n = 9), without affecting [Ca2+]i. 8. When external Cl- was lowered, the amplitude of the outward current decreased; when internal Cl- was replaced by aspartate, it became apparent at more negative potentials. These interventions strongly suggest the current was carried by Cl-; it can therefore be referred to as a [Ca2+]i-activated Cl- current or ICl(Ca). 9. When ICl(Ca) was maximally activated during a conditioning step, steps to negative potentials revealed inward currents through ICl(Ca) (in symmetrical Cl- solutions). The fully activated I-V relation was linear. 10. ICl(Ca) could be activated at membrane potentials between -80 and +80 mV by a fast application of caffeine (10 mM), inducing Ca2+ release from the SR, demonstrating that ICl(Ca) does not require membrane depolarization or Ca2+ influx through the Ca2+ channel for its activation.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 从兔心室酶解分离出的单个浦肯野细胞,在全细胞电压钳制下进行研究,并向细胞内灌注荧光Ca2+指示剂indo-1(100微摩尔)。2. 通过从-45毫伏的钳制电压进行短暂去极化以及从非常正的电位进行复极化,引发快速的[Ca2+]i瞬变。[Ca2+]i峰值与电压的关系呈钟形,峰值约在+10毫伏。3. [Ca2+]i瞬变被Ca2+通道拮抗剂尼索地平(10微摩尔)完全阻断,并且当用咖啡因(1毫摩尔)或ryanodine(10微摩尔)对细胞进行灌流以阻止肌浆网(SR)释放Ca2+时,[Ca2+]i瞬变非常小。快速施加咖啡因会引起[Ca2+]i的短暂增加。这些结果表明[Ca2+]i瞬变是由于Ca(2+)诱导的Ca2+从SR释放所致。4. [Ca2+]i瞬变的下降速率是电压依赖性的,表明Na(+)-Ca2+交换体对Ca2+外流有贡献。在非常正的电位(>+60毫伏)时,可以观察到Ca2+通过Na(+)-Ca2+交换体流入。5. 在高于+10毫伏的电位下观察到一个短暂外向电流,但只有当去极化脉冲伴随着[Ca2+]i瞬变时才会出现。6. 当通过(1)改变[Ca2+]o、(2)改变去极化频率或(3)条件性预脉冲来改变[Ca2+]i瞬变的幅度时,外向电流的幅度会朝相同方向改变。这表明该电流的激活依赖于[Ca2+]i并与之成比例。7. 在无K+溶液中、存在Cs+和TEA+时观察到外向电流,并且不被4-氨基吡啶(10毫摩尔)阻断。相反,DIDS(100微摩尔)使外向电流降低了70±20%(平均值±标准差,n = 9),而不影响[Ca2+]i。8. 当降低细胞外Cl-时,外向电流的幅度减小;当用天冬氨酸替代细胞内Cl-时,在更负的电位下该电流变得明显。这些干预强烈表明该电流由Cl-携带;因此可以将其称为[Ca2+]i激活的Cl-电流或ICl(Ca)。9. 当在一个条件步骤中使ICl(Ca)最大程度激活时,向负电位的步骤显示出通过ICl(Ca)的内向电流(在对称Cl-溶液中)。完全激活的I-V关系是线性的。10. 通过快速施加咖啡因(10毫摩尔)诱导SR释放Ca2+,可以在-80至+80毫伏之间的膜电位激活ICl(Ca),这表明ICl(Ca)的激活不需要膜去极化或Ca2+通过Ca2+通道流入。(摘要截断于400字)

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