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首页> 外文期刊>The Journal of general physiology >Perchlorate enhances transmission in skeletal muscle excitation-contraction coupling.
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Perchlorate enhances transmission in skeletal muscle excitation-contraction coupling.

机译:高氯酸盐增强骨骼肌兴奋-收缩耦合的传递。

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The effects of the anion perchlorate (present extracellularly at 8 mM) were studied on functional skeletal muscle fibers from Rana pipiens, voltage-clamped in a Vaseline gap chamber. Established methods were used to monitor intramembranous charge movement and flux of Ca release from the sarcoplasmic reticulum (SR) during pulse depolarization. Saponin permeabilization of the end portions of the fiber segment (Irving, M., J. Maylie, N. L. Sizto, and W. K. Chandler. 1987. Journal of General Physiology. 89:1-41) substantially reduced the amount of charge moving during conventional control pulses, thus minimizing a technical error that plagued our previous studies. Perchlorate prolonged the ON time course of charge movement, especially at low and intermediate voltages. The OFFs were also made slower, the time constant increasing twofold. The hump kinetic component was exaggerated by ClO4- or was made to appear in fibers that did not have it in reference conditions. ClO4- had essentially no kinetic ON effects at high voltages ( or = 10 mV). ClO4- changed the voltage distribution of mobile charge. In single Boltzmann fits, the midpoint potential V was shifted -20 mV and the steepness parameter K was reduced by 4.7 mV (or 1.78-fold), but the maximum charge was unchanged (n = 9). Total Ca content in the SR, estimated using the method of Schneider et al. (Schneider, M. F., B. J. Simon, and G. Szucs. 1987. Journal of Physiology. 392:167-192) for correcting for depletion, stayed constant over tens of minutes in reference conditions but decayed in ClO4- at an average rate of 0.3 mumol/liter myoplasmic water per s. ClO4- changed the kinetics of release flux, reducing the fractional inactivation of release after the peak. ClO4- shifted the voltage dependence of Ca release flux. In particular, the threshold voltage for Ca release was shifted by about -20 mV, and the activation of the steady component of release flux was shifted by 20 mV in the negative direction. The shift of release activation was greater than that of mobile charge. Thus the threshold charge, defined as the minimum charge moved for eliciting a detectable Ca transient, was reduced from 6 nC/microF (0.55, n = 7) to 3.4 (0.53). The average of the paired differences was 2.8 (0.33, P 0.01). The effects of ClO4- were then studied in fibers in modified functional situations. Depletion of Ca in the SR, achieved by high frequency pulsing in the presence of intracellular BAPTA and EGTA, simplified but did not eliminate the effects of ClO4-.(ABSTRACT TRUNCATED AT 400 WORDS)
机译:研究了高氯酸根阴离子(在细胞外以8 mM存在)对来自Rana pipiens的功能性骨骼肌纤维的影响,该纤维被钳位在Vaseline间隙室中。已建立的方法用于监测脉冲去极化过程中膜内电荷的运动以及从肌浆网(SR)释放的Ca的通量。纤维段末端的皂苷透化(Irving,M.,J. Maylie,NL Sizto,and WK Chandler。1987. General Physiology。89:1-41)大大减少了常规控制过程中电荷的移动量。脉冲,从而将困扰我们先前研究的技术错误降至最低。高氯酸盐延长了电荷运动的导通时间,特别是在中低压时。 OFFs也变慢了,时间常数增加了两倍。驼峰动力学成分被ClO4-夸大,或使其出现在参考条件下没有的纤维中。 ClO4-在高电压(>或= 10 mV)下基本上没有动力学导通效应。 ClO4-改变了移动电荷的电压分布。在单次Boltzmann拟合中,中点电势V偏移了-20 mV,陡度参数K降低了4.7 mV(或1.78倍),但是最大电荷不变(n = 9)。 SR中的总Ca含量,使用Schneider等人的方法估算。 (Schneider,MF,BJ Simon和G. Szucs。1987.生理学杂志。392:167-192)用于校正耗竭,在参考条件下在数十分钟内保持恒定,但在ClO4-中的衰减平均为0.3摩尔/升肌质水/秒。 ClO 4改变了释放通量的动力学,减少了峰后释放的部分失活。 ClO4-改变了Ca释放通量的电压依赖性。特别是,Ca释放的​​阈值电压偏移了大约-20 mV,释放通量的稳定成分的激活在负方向上偏移了> 20 mV。释放激活的移动大于移动充电的移动。因此,阈值电荷(定义为引起可检测的Ca瞬变的最小电荷移动)从6 nC / microF(0.55,n = 7)降低到3.4(0.53)。配对差异的平均值为2.8(0.33,P <0.01)。然后研究了改性功能条件下纤维对ClO4-的影响。在细胞内BAPTA和EGTA存在下通过高频脉冲实现的SR中Ca的消耗得以简化,但并没有消除ClO4-的作用。(摘要截断为400字)

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