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单个哺乳动物骨骼肌纤维中的钙瞬变

Calcium transients in single mammalian skeletal muscle fibres.

作者信息

Delbono O, Stefani E

机构信息

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

出版信息

J Physiol. 1993 Apr;463:689-707. doi: 10.1113/jphysiol.1993.sp019617.

Abstract
  1. We studied the transient changes in myoplasmic Ca2+ concentration under current- and voltage-clamp (double Vaseline-gap technique) in cut fibres of rat extensor digitorum longus muscle using mag-fura-2 (furaptra) as Ca2+ indicator, at 3.6-3.8 microns sarcomere length and 17 degrees C. Mag-fura-5 and fura-2 were also used in order to characterize some aspects of the Ca2+ transients. 2. The peak [Ca2+] in response to a single action potential was 4.6 +/- 0.4 microM (n = 5). The time to peak of the Ca2+ transient was 4.6 +/- 0.42 ms, with half-width of 8.2 +/- 1.5 ms, time constant of the rising phase 1.15 +/- 0.25 ms, time constant of the decaying phase 3.26 +/- 0.65 ms, and delay between action potential and Ca2+ transient 2.0 +/- 0.2 ms. 3. Ca2+ transients were studied under voltage-clamp conditions at different voltages and pulse durations. The rising phase showed a complex temporal course with a fast initial increase and a second component. Both components were separated by a plateau or a brief decrease of the Ca2+ concentration. The peak Ca2+ transient was 10.5 +/- 1.3 microM (n = 22). 4. After interrupting the pulse, Ca2+ concentration decayed exponentially. The time constant of decay of the Ca2+ transient increased with the pulse voltage and duration, reaching a maximum value at potentials more positive than +10 mV and pulses longer than 200 ms. An analysis of the decaying phases of the Ca2+ transients suggests that only the removal process operates after fibre repolarization. 5. The rate of Ca2+ release from the sarcoplasmic reticulum was calculated using the Melzer, Ríos & Schneider model. The value of 17.2 +/- 3.1 micronM ms-1 (n = 10) estimated in these calculations was intermediate between those obtained by other authors from cut frog muscles (10 microM ms-1) and intact frog fibres (100 microM ms-1) using antipyrylazo III (AP III) as the Ca2+ indicator.
摘要
  1. 我们在3.6 - 3.8微米肌节长度和17摄氏度条件下,采用双凡士林间隙技术,运用mag - fura - 2(furaptra)作为钙离子指示剂,在大鼠趾长伸肌的离体纤维上,通过电流钳和电压钳研究了肌质钙离子浓度的瞬态变化。为了表征钙离子瞬变的某些方面,还使用了Mag - fura - 5和fura - 2。2. 单个动作电位引起的钙离子浓度峰值为4.6±0.4微摩尔/升(n = 5)。钙离子瞬变的峰值时间为4.6±0.42毫秒,半高宽为8.2±1.5毫秒,上升相时间常数为1.15±0.25毫秒,衰减相时间常数为3.26±0.65毫秒,动作电位与钙离子瞬变之间的延迟为2.0±0.2毫秒。3. 在不同电压和脉冲持续时间的电压钳条件下研究了钙离子瞬变。上升相呈现出复杂的时间进程,有一个快速的初始增加和第二个成分。两个成分之间由钙离子浓度的平台期或短暂下降隔开。钙离子瞬变的峰值为10.5±1.3微摩尔/升(n = 22)。4. 中断脉冲后,钙离子浓度呈指数衰减。钙离子瞬变的衰减时间常数随脉冲电压和持续时间增加,在电位高于 +10毫伏且脉冲长于200毫秒时达到最大值。对钙离子瞬变衰减相的分析表明,纤维复极化后只有清除过程起作用。5. 使用梅尔泽、里奥斯和施耐德模型计算了肌浆网钙离子释放速率。这些计算中估计的值为17.2±3.1微摩尔/升·毫秒(n = 10),介于其他作者使用安替比拉佐III(AP III)作为钙离子指示剂从离体青蛙肌肉(10微摩尔/升·毫秒)和完整青蛙纤维(100微摩尔/升·毫秒)获得的值之间。
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0280/1175366/49617eaf2972/jphysiol00419-0683-a.jpg

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