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Calcium transients and intramembrane charge movement in skeletal muscle fibres.骨骼肌纤维中的钙瞬变和膜内电荷移动。
Nature. 1979 May 31;279(5712):391-6. doi: 10.1038/279391a0.
2
Some factors influencing the contractility of a non-conducting fiber preparation.一些影响非传导性纤维制剂收缩性的因素。
Biochim Biophys Acta. 1950 Jan;4(1-3):58-67. doi: 10.1016/0006-3002(50)90009-6.
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ELECTROCHEMICAL COUPLING IN POTENTIATION OF MUSCULAR CONTRACTION.肌肉收缩增强中的电化学偶联
Science. 1964 Feb 7;143(3606):577-9. doi: 10.1126/science.143.3606.577.
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Activation of the contractile mechanism in striated muscle.横纹肌收缩机制的激活。
Acta Physiol Scand. 1958 Oct 28;44(1):55-66. doi: 10.1111/j.1748-1716.1958.tb01608.x.
5
Stoichiometry of the reactions of calcium with the metallochromic indicator dyes antipyrylazo III and arsenazo III.钙与金属显色指示剂染料安替比拉宗III和偶氮胂III反应的化学计量学
Biophys J. 1981 Dec;36(3):607-21. doi: 10.1016/S0006-3495(81)84755-8.
6
Action of caffeine in excitation-contraction coupling of frog skeletal muscle fibres.咖啡因对青蛙骨骼肌纤维兴奋-收缩偶联的作用。
J Physiol. 1982 Apr;325:195-211. doi: 10.1113/jphysiol.1982.sp014145.
7
Membrane charge moved at contraction thresholds in skeletal muscle fibres.在骨骼肌纤维的收缩阈值处,膜电荷发生移动。
J Physiol. 1981 May;314:595-633. doi: 10.1113/jphysiol.1981.sp013726.
8
Membrane charge movement in contracting and non-contracting skeletal muscle fibres.收缩和非收缩骨骼肌纤维中的膜电荷移动
J Physiol. 1981 May;314:565-93. doi: 10.1113/jphysiol.1981.sp013725.
9
The control of contraction activation by the membrane potential.膜电位对收缩激活的控制。
Experientia. 1981 Jun;37(6):580-1. doi: 10.1007/BF01990061.
10
Comparison of birefringence signals and calcium transients in voltage-clamped cut skeletal muscle fibres of the frog.青蛙电压钳制离体骨骼肌纤维中双折射信号与钙瞬变的比较
J Physiol. 1983 Aug;341:579-93. doi: 10.1113/jphysiol.1983.sp014825.

咖啡因对青蛙离体骨骼肌纤维膜内电荷移动和钙瞬变的影响。

Effect of caffeine on intramembrane charge movement and calcium transients in cut skeletal muscle fibres of the frog.

作者信息

Kovács L, Szücs G

出版信息

J Physiol. 1983 Aug;341:559-78. doi: 10.1113/jphysiol.1983.sp014824.

DOI:10.1113/jphysiol.1983.sp014824
PMID:6604806
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1195575/
Abstract
  1. The authors have studied the effect of caffeine in subthreshold concentration (0.5 mmol l(-1) at 2-4 degrees C) on the contraction threshold, on intramembrane charge movement and calcium transients in voltage-clamped frog skeletal muscle fibres.2. The single-gap technique (Kovács & Schneider, 1978) was used for the voltage clamping of terminated segments of cut fibres. Ionic conductances were minimized by using caesium glutamate at the open end pool and tetraethylammonium sulphate and tetrodotoxin at the closed end pool.3. Myoplasmic calcium transients evoked by depolarizing pulses were recorded by measuring the changes in absorbance of the fibres at 720 nm after the intracellular application of Antipyrylazo III dye.4. The strength-duration curve for contraction threshold was shifted towards more negative membrane potentials in the presence of caffeine. Shift was more definite at shorter pulse durations than at the rheobase.5. The total amount of charge moving during the depolarizing pulses at different membrane potentials was not changed by caffeine treatment, whereas the threshold amounts of charge moved during the critical periods of the contraction threshold decreased at different voltages (by about 23%).6. In the presence of caffeine, calcium transients accompanying long (100 ms) depolarizing pulses showed increased voltage-dependent peak amplitudes, rising phases and rate coefficients referring to calcium release, but a decreased voltage-dependent re-uptake rate either during or after the pulse.7. Calcium transients evoked by depolarizing pulses along the strength-duration curve for contraction threshold gave the same peak amplitudes (ranging from 0.9 to 2.8 mumol l(-1) free myoplasmic calcium on different fibres), but membrane-potential-dependent latency times and rising phases. The rate coefficients for declining phase did not depend on the preceding pulse voltage.8. On applying caffeine, the calcium transients related to the contraction threshold also had equal but smaller peak amplitudes, shorter latency times and the same magnitude of voltage-independent rate coefficients for the declining phase as in the control solution.9. The twitch potentiating effect of caffeine can be explained by its facilitating calcium release from the sarcoplasmic reticulum, while the re-uptake rate is not modified. The apparent inhibition of re-uptake can be related to the enhanced release of calcium due to caffeine effect. Due to the sensitizing effect of caffeine on the sarcoplasmic reticulum membrane, smaller amounts of charge are needed to reach the contraction threshold than without caffeine.
摘要
  1. 作者研究了阈下浓度(2-4摄氏度时为0.5 mmol l(-1))的咖啡因对收缩阈值、膜内电荷移动以及电压钳制的青蛙骨骼肌纤维中钙瞬变的影响。

  2. 采用单间隙技术(Kovács和Schneider,1978年)对切断纤维的末端节段进行电压钳制。通过在开放端池使用谷氨酸铯,在封闭端池使用硫酸四乙铵和河豚毒素,使离子电导最小化。

  3. 通过在细胞内施加安替比拉佐III染料后测量纤维在720 nm处吸光度的变化,记录去极化脉冲诱发的肌浆钙瞬变。

  4. 在咖啡因存在的情况下,收缩阈值的强度-时间曲线向更负的膜电位方向移动。在较短脉冲持续时间下的移动比在基强度时更明显。

  5. 咖啡因处理并未改变在不同膜电位下去极化脉冲期间移动的总电荷量,而在收缩阈值的关键时期移动的阈值电荷量在不同电压下减少(约23%)。

  6. 在咖啡因存在的情况下,伴随长(100 ms)去极化脉冲的钙瞬变显示出电压依赖性峰值幅度、上升相以及与钙释放相关的速率系数增加,但在脉冲期间或之后电压依赖性再摄取速率降低。

  7. 沿着收缩阈值的强度-时间曲线的去极化脉冲诱发的钙瞬变具有相同的峰值幅度(不同纤维上自由肌浆钙的范围为0.9至2.8 mumol l(-1)),但具有膜电位依赖性的潜伏期和上升相。下降相的速率系数不取决于先前的脉冲电压。

  8. 施加咖啡因时,与收缩阈值相关的钙瞬变也具有相等但较小的峰值幅度、较短的潜伏期以及与对照溶液中下降相相同大小的电压非依赖性速率系数。

  9. 咖啡因的抽搐增强作用可以通过其促进肌浆网释放钙来解释,而再摄取速率未改变。再摄取的明显抑制可能与咖啡因作用导致的钙释放增强有关。由于咖啡因对肌浆网膜的致敏作用,与无咖啡因时相比,达到收缩阈值所需的电荷量更少。