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青蛙抽动肌纤维中缓慢钙电流的衰减受细胞内乙二醇双四乙酸(EGTA)的影响。

Decay of the slow calcium current in twitch muscle fibers of the frog is influenced by intracellular EGTA.

作者信息

Francini F, Stefani E

机构信息

Department of Physiology and Molecular Biophysics, Baylor College of Medicine, Houston, Texas 77030.

出版信息

J Gen Physiol. 1989 Nov;94(5):953-69. doi: 10.1085/jgp.94.5.953.

Abstract

The mechanism(s) of the decay of slow calcium current (ICa) in cut twitch skeletal muscle fibers of the frog were studied in voltage-clamp experiments using the double vaseline-gap technique. ICa decay followed a single exponential in 10 mM external Ca2+ and 20 mM internal EGTA solutions in all pulse protocols tested: single depolarizing pulses (activation protocol), two pulses (inactivation protocol), and during a long pulse preceded by a short prepulse (400 ms) to 80 mV (tail protocol). In single pulses the rate constant of ICa decay was approximately 0.75 s-1 at 0 mV and became faster with larger depolarizations. ICa had different amplitudes during the second pulses of the inactivation protocol (0 mV) and of the tail protocol (-20 to 40 mV) and had similar time constants of decay. The time constant of decay did not change significantly at each potential after replacing 10 mM Ca2+ with a Ca2+-buffered solution with malate. With 70 mM intracellular EGTA and 10 mM external Ca2+ solutions, ICa also decayed with a single-exponential curve, but it was about four times faster (approximately 3.5 s-1 at 0 mV pulse). In these solutions the rate constant showed a direct relationship with ICa amplitude at different potentials. With 70 mM EGTA, replacing the external 10 mM Ca2+ solution with the Ca2+-buffered solution caused the decay of ICa to become slower and to have the same relationship with membrane potential and ICa amplitude as in fibers with 20 mM EGTA internal solution. The mechanism of ICa decay depends on the intracellular EGTA concentration: (a) internal EGTA (both 20 and 70 mM) significantly reduces the voltage dependence of the inactivation process and (b) 70 mM EGTA dramatically increases the rate of tubular calcium depletion during the flow of ICa.

摘要

采用双凡士林间隙技术,通过电压钳实验研究了青蛙离体单收缩骨骼肌纤维中慢钙电流(ICa)衰减的机制。在所有测试的脉冲方案中:单去极化脉冲(激活方案)、双脉冲(失活方案)以及在由400 ms的短预脉冲(至80 mV)引发的长脉冲期间(尾电流方案),ICa衰减在10 mM细胞外Ca2+和20 mM细胞内EGTA溶液中呈单指数形式。在单脉冲中,ICa衰减的速率常数在0 mV时约为0.75 s-1,且随着去极化幅度增大而加快。在失活方案(0 mV)和尾电流方案(-20至40 mV)的第二个脉冲期间,ICa具有不同的幅度,但衰减时间常数相似。用苹果酸钙缓冲溶液替代10 mM Ca2+后,每个电位下的衰减时间常数无显著变化。在70 mM细胞内EGTA和10 mM细胞外Ca2+溶液中,ICa也呈单指数曲线衰减,但速度快约四倍(0 mV脉冲时约为3.5 s-1)。在这些溶液中,速率常数与不同电位下的ICa幅度呈直接关系。用70 mM EGTA,将细胞外10 mM Ca2+溶液替换为钙缓冲溶液会导致ICa衰减变慢,且与膜电位和ICa幅度的关系与细胞内溶液为20 mM EGTA的纤维相同。ICa衰减机制取决于细胞内EGTA浓度:(a)细胞内EGTA(20 mM和70 mM)均显著降低失活过程的电压依赖性;(b)70 mM EGTA显著增加ICa流动期间管状钙耗竭的速率。

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