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咖啡因会减缓电压钳制的骨骼肌纤维中钙释放的关闭过程。

Caffeine slows turn-off of calcium release in voltage clamped skeletal muscle fibers.

作者信息

Simon B J, Klein M G, Schneider M F

机构信息

Department of Biological Chemistry, University of Maryland School of Medicine, Baltimore 21201.

出版信息

Biophys J. 1989 Apr;55(4):793-7. doi: 10.1016/S0006-3495(89)82878-4.

Abstract

Myoplasmic free calcium transients delta [Ca2+] were monitored with the calcium indicators antipyrylazo III and fura-2 in voltage clamped cut frog skeletal muscle fibers, in the presence and absence of 0.5 mM caffeine. Without caffeine delta [Ca2+] began to decline within a few milliseconds of fiber repolarization for pulses of all durations. In caffeine delta [Ca2+] continued to rise for 10-60 ms after 10 or 20 ms depolarizing pulses, indicating that the release of calcium from the sarcoplasmic reticulum (SR) continued well after repolarization of transverse tubular (TT) membranes in the presence of caffeine. Caffeine also increased the peak amplitude of delta [Ca2+] for all pulses and slowed the decline of delta [Ca2+] after pulses of all durations. The rate of calcium release from the SR calculated from delta [Ca2+] showed that for 10 ms pulses in caffeine release did not turn off abruptly on repolarization but instead declined to zero with a time constant essentially the same as the time constant for inactivation of SR calcium release during depolarizing pulses in the presence or absence of caffeine. The observed loss of TT membrane potential control of SR calcium release in the presence of caffeine suggests the appearance of a significant component of cytosolic Ca2+-induced calcium release in caffeine.

摘要

在电压钳制的离体青蛙骨骼肌纤维中,使用钙指示剂安替比拉宗III和fura-2监测肌质游离钙瞬变δ[Ca2+],实验分别在存在和不存在0.5 mM咖啡因的情况下进行。在没有咖啡因时,对于所有持续时间的脉冲,δ[Ca2+]在纤维复极化后的几毫秒内就开始下降。在存在咖啡因的情况下,对于10或20 ms的去极化脉冲,δ[Ca2+]在复极化后还会持续上升10 - 60 ms,这表明在咖啡因存在时,横管(TT)膜复极化后,肌浆网(SR)中的钙释放仍会持续很长时间。咖啡因还增加了所有脉冲下δ[Ca2+]的峰值幅度,并减缓了所有持续时间脉冲后δ[Ca2+]的下降。根据δ[Ca2+]计算得出的SR钙释放速率表明,对于咖啡因存在下的10 ms脉冲,复极化时释放不会突然停止,而是以与有无咖啡因时去极化脉冲期间SR钙释放失活时间常数基本相同的时间常数下降至零。在咖啡因存在下观察到的TT膜电位对SR钙释放控制的丧失表明,咖啡因中出现了显著的胞质Ca2+诱导钙释放成分。

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