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本文引用的文献

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Regulation of Shaker K+ channel inactivation gating by the cAMP-dependent protein kinase.
Neuron. 1994 May;12(5):1097-109. doi: 10.1016/0896-6273(94)90317-4.
2
Inactivation properties of voltage-gated K+ channels altered by presence of beta-subunit.β亚基的存在改变电压门控钾离子通道的失活特性。
Nature. 1994 May 26;369(6478):289-94. doi: 10.1038/369289a0.
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Statistical analysis of single sodium channels. Effects of N-bromoacetamide.单钠通道的统计分析。N-溴乙酰胺的作用。
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Effect of N-bromoacetamide on single sodium channel currents in excised membrane patches.N-溴乙酰胺对膜片钳单钠通道电流的影响。
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6
Genetic modification of potassium channels in Drosophila Shaker mutants.果蝇Shaker突变体中钾通道的基因改造。
Nature. 1981;293(5829):228-30. doi: 10.1038/293228a0.
7
Different modes of Ca channel gating behaviour favoured by dihydropyridine Ca agonists and antagonists.二氢吡啶类钙激动剂和拮抗剂所青睐的不同钙通道门控行为模式。
Nature. 1984;311(5986):538-44. doi: 10.1038/311538a0.
8
A new preparation for recording single-channel currents from skeletal muscle.一种用于记录骨骼肌单通道电流的新制剂。
Proc R Soc Lond B Biol Sci. 1984 Jun 22;221(1225):455-64. doi: 10.1098/rspb.1984.0044.
9
Slow changes in potassium permeability in skeletal muscle.骨骼肌中钾通透性的缓慢变化。
J Physiol. 1970 Jul;208(3):645-68. doi: 10.1113/jphysiol.1970.sp009140.
10
Voltage clamp experiments in striated muscle fibres.横纹肌纤维的电压钳实验。
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体外分化的非洲爪蟾肌细胞中钾通道的可转换失活模式。

Convertible modes of inactivation of potassium channels in Xenopus myocytes differentiating in vitro.

作者信息

Ernsberger U, Spitzer N C

机构信息

Department of Biology, University of California, San Diego, La Jolla 92093-0357, USA.

出版信息

J Physiol. 1995 Apr 15;484 ( Pt 2)(Pt 2):313-29. doi: 10.1113/jphysiol.1995.sp020667.

DOI:10.1113/jphysiol.1995.sp020667
PMID:7602528
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1157896/
Abstract
  1. Voltage-dependent inactivating single-channel potassium currents were recorded in cell-attached and inside-out patches from embryonic Xenopus myocytes differentiating in culture. 2. Channels with rapid inactivation (time constants < 25 ms) and with slow inactivation (time constants > 80 ms) recorded after one day in vitro appear to belong to two functionally different classes. Rapidly and slowly inactivating channels show steady-state inactivation with potentials of half-inactivation of -74 +/- 7 and -44 +/- 9 mV. They exhibit voltage-dependent activation, with times to half-maximal activation of 0.79 +/- 0.09 and 1.17 +/- 0.22 ms when stepped from -120 to +40 mV. Rapidly inactivating channels also have a lower open probability than slowly inactivating ones. The channels have similar conductances of 23 +/- 6 and 17 +/- 4 pS and extrapolated reversal potentials close to the potassium equilibrium potential. 3. In cell-attached patches, inactivation behaviours of channels with rapid or slow inactivation do not change during recording. After patch excision, rapidly inactivating channels usually switch to a slow inactivation mode. Slowly inactivating channels derived from rapidly inactivating channels after patch excision retain their conductance and extrapolated reversal potential, but are not distinguishable from native slowly inactivating channels with respect to steady-state inactivation, activation and inactivation times, as well as open probabilities. 4. The change in inactivation behaviour of rapidly inactivating channels after patch excision is reversed by application of reduced dithiothreitol (DTT). In contrast, channels with slow inactivation in the cell-attached mode do not change in to rapidly inactivating channels after application of DTT in the excised configuration, suggesting that these channels belong to a structurally different class. 5. Frequent observation of superposing channel openings indicates clustering of inactivating potassium channels in the myocyte membrane, since many patches lack channel activity. Clustering does not depend on the presence of differentiating neurones. 6. Channels with rapid inactivation increase 6-fold in density during the first day in culture in the presence of neurones; channel density decreases in their absence. Channels with slow inactivation increase 2-fold in density in the presence or absence of differentiating neurones during this period. 7. Channels with rapid or slow inactivation in cell-attached membrane belong to functionally distinct classes that are developmentally regulated differently. Reversible changes from rapid to slow inactivation mode after patch excision suggest that the channels may be structurally related.
摘要
  1. 在体外培养分化的非洲爪蟾胚胎肌细胞的细胞贴附式和内面向外膜片中记录了电压依赖性失活单通道钾电流。2. 体外培养一天后记录到的快速失活(时间常数<25毫秒)和缓慢失活(时间常数>80毫秒)的通道似乎属于两个功能不同的类别。快速失活和缓慢失活通道的稳态失活半失活电位分别为-74±7和-44±9毫伏。它们表现出电压依赖性激活,从-120毫伏跃升至+40毫伏时,达到最大激活一半的时间分别为0.79±0.09和1.17±0.22毫秒。快速失活通道的开放概率也低于缓慢失活通道。这些通道的电导相似,分别为23±6和17±4皮安,外推反转电位接近钾平衡电位。3. 在细胞贴附式膜片中,快速或缓慢失活通道的失活行为在记录过程中不变。膜片切除后,快速失活通道通常转变为缓慢失活模式。膜片切除后从快速失活通道衍生而来的缓慢失活通道保留其电导和外推反转电位,但在稳态失活、激活和失活时间以及开放概率方面与天然缓慢失活通道无法区分。4. 膜片切除后快速失活通道失活行为的变化可通过应用还原型二硫苏糖醇(DTT)逆转。相反,细胞贴附模式下缓慢失活的通道在切除配置中应用DTT后不会转变为快速失活通道,这表明这些通道属于结构不同的类别。5. 频繁观察到叠加的通道开放表明失活钾通道在肌细胞膜中聚集,因为许多膜片缺乏通道活性。聚集不依赖于分化神经元的存在。6. 在有神经元存在的情况下,快速失活通道在培养的第一天密度增加6倍;在没有神经元的情况下通道密度降低。在此期间,无论有无分化神经元,缓慢失活通道的密度均增加2倍。7. 细胞贴附膜片中快速或缓慢失活的通道属于功能不同的类别,在发育过程中受到不同的调节。膜片切除后从快速失活模式到缓慢失活模式的可逆变化表明这些通道可能在结构上相关。