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对照小鼠和mdx小鼠骨骼肌中延迟整流电流的膜片钳研究

A patch-clamp study of delayed rectifier currents in skeletal muscle of control and mdx mice.

作者信息

Hocherman S D, Bezanilla F

机构信息

Department of Physiology, UCLA School of Medicine 90024, USA.

出版信息

J Physiol. 1996 May 15;493 ( Pt 1)(Pt 1):113-28. doi: 10.1113/jphysiol.1996.sp021368.

Abstract
  1. Potassium currents were measured in the extensor digitorum longus muscle of normal and mdx mice, which lack the protein dystrophin, using the cell-attached and inside-out patch clamp techniques, in the presence of asymmetrical K+ concentrations (3 mM in the pipette, 160 mM in the bath). 2. In cell-attached patches, the delayed rectifier was the most commonly found potassium channel, with a density of roughly 8 channels microns-2. Outward macroscopic currents were activated in macropatches depolarized to potentials positive to -60 mV. The probability of opening reached half-maximal values around -40 mV for control patches and -31 mV for patches from mdx mice. 3. Tail currents were linear in the range between -60 and +20 mV, reversing close to -100 mV. The single channel current at 0 mV, estimated from non-stationary analysis of variance, was used in conjunction with the slope of the linear part of the tail current to calculate the single channel conductance, yielding a value of 19 +/- 1 pS. 4. At 0 mV, the delayed rectifier inactivated with two time constants, of 70 +/- 20 ms and 600 +/- 200 ms. Prepulses of 500 ms duration to different potentials produced incomplete inactivation with inactivation reaching 50% of its maximum at -50 mV. 5. Single channel activity was recorded using small pipettes. Both single channel conductance and kinetic behaviour were in agreement with the macroscopic current data. 6. In excised patches, the delayed rectifier current ran down, unmasking other K+ channels. A Ca(2+)-dependent K+ channel of 186 pS (BK-like channel) was found frequently in patches bathed in solutions containing appropriate concentrations of calcium, especially at stronger depolarizations. A K+ channel of 63 pS was unmasked in control excised patches bathed in solutions devoid of ATP. This channel was not observed in patches excised from mdx fibers.
摘要
  1. 采用细胞贴附式和内面向外式膜片钳技术,在不对称钾离子浓度(电极内3 mM,浴槽内160 mM)条件下,测量正常小鼠和缺乏抗肌萎缩蛋白的mdx小鼠的趾长伸肌中的钾电流。2. 在细胞贴附式膜片中,延迟整流钾通道是最常见的钾通道,密度约为8个通道/μm²。在去极化至高于 -60 mV的大膜片中可激活外向宏观电流。对照膜片在约 -40 mV时开放概率达到最大值的一半,mdx小鼠膜片则在约 -31 mV时达到。3. 尾电流在 -60至 +20 mV范围内呈线性,反转电位接近 -100 mV。通过非平稳方差分析估计的0 mV时的单通道电流,与尾电流线性部分的斜率一起用于计算单通道电导,得出值为19±1 pS。4. 在0 mV时,延迟整流钾通道以70±20 ms和600±200 ms两个时间常数失活。持续500 ms的不同电位预脉冲产生不完全失活,在 -50 mV时失活达到最大值的50%。5. 使用小电极记录单通道活动。单通道电导和动力学行为均与宏观电流数据一致。6. 在切除的膜片中,延迟整流钾电流衰减,从而揭示出其他钾通道。在含有适当浓度钙的溶液中浸泡的膜片中,经常发现一个186 pS的钙依赖性钾通道(类大电导钙激活钾通道),尤其是在更强的去极化时。在不含ATP的溶液中浸泡的对照切除膜片中,一个63 pS的钾通道被揭示出来。在从mdx纤维切除的膜片中未观察到该通道。

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