用玻璃闪烁探测器测量单根肌纤维中的钙通量。

Calcium fluxes in single muscle fibres measured with a glass scintillator probe.

作者信息

Ashley C C, Lea T J

出版信息

J Physiol. 1978 Sep;282:307-31. doi: 10.1113/jphysiol.1978.sp012465.

DOI:10.1113/jphysiol.1978.sp012465

PMID:102762

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1282741/

Abstract

An intracellular glass scintillator (Caldwell & Lea, 1973) has been used to obtain a continuous record of the influx of 45Ca into single muscle fibres of the barnacle, Balanus nubilus. 2. In the presence of intracellular EGTA (final concentration greater than 3 mM/kg), the scintillator detected an initial fast phase to the influx (half-time = 18.3 min, compartment size = 4.1% fibre volume) followed by a slow, linear phase which gave a value for the Ca influx of 1.2 p-mole . cm-2 . sec-1. The efflux of 45Ca was also measured with the scintillator by transferring a 45Ca-loaded fibre into 45Ca-free saline. Two exponential phases of efflux were detected with half-times of 16.2 and 500 min. 3. The characterisitics of the fast phase of the influx and efflux are similar to those of the influx of the impermeant sucrose and inulin, suggesting that the fast phase represents exchange with the extracellular 'cleft space'. This phase was insensitive to external La3+ (2 mM). 4. The slow phase is considered to represent the flux of Ca across the surface membrane. It was inhibited by external La3+ (2 mM) and stimulated by replacing external Na+ with Li+. 5. When EGTA-injected fibres were depolarized using an axial, intracellular electrode the Ca influx, measured from the slow phase, was increased. At higher concentrations of intracellular EGTA (6--22 mM/kg), the extra Ca influx due to a rectangular, depolarizing current pulse was proportional to the number of Ca spikes it produced. A single Ca spike gave an extra Ca influx of 19--48 p-mole . cm-2. External D600 (5 x 10(-4)M) inhibited both Ca spike and the extra Ca influx. 6. At lower intracellular EGTA concentrations (3.6--11 mM/kg), a 50 mV depolarization of 250 msec duration gave a mean extra Ca influx of 80 p-mole . cm-2. The upper value was 145 p-mole . cm-2 and this would increase the total internal Ca by 4.1 micrometer/kg. It is calculated that if all this extra Ca was bound to the myofibrillar sites for tension, it would only produce 6.2% of the force expected for a similar depolarization in a fibre with no intracellular EGTA.

摘要

一种细胞内玻璃闪烁体（考德威尔和利，1973年）已被用于获取45Ca流入藤壶（Balanus nubilus）单根肌纤维的连续记录。2. 在细胞内乙二醇双乙胺醚（EGTA）存在的情况下（终浓度大于3 mM/kg），闪烁体检测到流入的初始快速阶段（半衰期 = 18.3分钟，区室大小 = 纤维体积的4.1%），随后是缓慢的线性阶段，该阶段得出的Ca流入值为1.2皮摩尔·厘米-2·秒-1。通过将负载45Ca的纤维转移到不含45Ca的盐溶液中，也用闪烁体测量了45Ca的流出。检测到两个指数衰减阶段的流出，半衰期分别为16.2和500分钟。3. 流入和流出的快速阶段的特征与非渗透性蔗糖和菊粉的流入特征相似，这表明快速阶段代表与细胞外“裂隙空间”的交换。该阶段对外部La3+（2 mM）不敏感。4. 缓慢阶段被认为代表Ca穿过表面膜的通量。它受到外部La3+（2 mM）的抑制，并通过用Li+替代外部Na+而受到刺激。5. 当使用轴向细胞内电极使注入EGTA的纤维去极化时，从缓慢阶段测量的Ca流入增加。在较高浓度的细胞内EGTA（6 - 22 mM/kg）下，由于矩形去极化电流脉冲导致的额外Ca流入与它产生的Ca尖峰数量成正比。单个Ca尖峰产生的额外Ca流入为19 - 48皮摩尔·厘米-2。外部D600（5×10(-4)M）抑制Ca尖峰和额外的Ca流入。6. 在较低的细胞内EGTA浓度（3.6 - 11 mM/kg）下，持续250毫秒的50 mV去极化产生的平均额外Ca流入为80皮摩尔·厘米-2。上限值为145皮摩尔·厘米-2，这将使细胞内总Ca增加4.1微米/千克。据计算，如果所有这些额外的Ca都与肌原纤维的张力位点结合，它只会产生在没有细胞内EGTA的纤维中类似去极化预期力的6.2%。