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草履虫中的单基因突变会增加一种钙依赖性钾电流。

A calcium-dependent potassium current is increased by a single-gene mutation in Paramecium.

作者信息

Hennessey T M, Kung C

机构信息

Laboratory of Molecular Biology, University of Wisconsin-Madison 53706.

出版信息

J Membr Biol. 1987;98(2):145-55. doi: 10.1007/BF01872127.

Abstract

The membrane currents of wild type Paramecium tetraurelia and the behavioral mutant teaA were analyzed under voltage clamp. The teaA mutant was shown to have a greatly increased outward current which was blocked completely by the combined use of internally delivered Cs+ and external TEA+. This, along with previous work (Satow, Y., Kung, C., 1976, J. Exp. Biol. 65:51-63) identified this as a K+ current. It was further found to be a calcium-activated K+ current since this increased outward K+ current cannot be elicited when the internal calcium is buffered with injected EGTA. The mutation pwB, which blocks the inward calcium current, also blocks this increased outward K+ current in teaA. This shows that this mutant current is activated by calcium through the normal depolarization-sensitive calcium channel. While tail current decay kinetic analysis showed that the apparent inactivation rates for this calcium-dependent K+ current are the same for mutant and wild type, the teaA current activates extremely rapidly. It is fully activated within 2 msec. This early activation of such a large outward current causes a characteristic reduction in the amplitude of the action potential of the teaA mutant. The teaA mutation had no effect on any of the other electrophysiological parameters examined. The phenotype of the teaA mutant is therefore a general decrease in responsiveness to depolarizing stimuli because of a rapidly activating calcium-dependent K+ current which prematurely repolarizes the action potential.

摘要

在电压钳制条件下分析了野生型四膜虫和行为突变体teaA的膜电流。结果显示,teaA突变体的外向电流大幅增加,而胞内注入Cs⁺和胞外加入TEA⁺联合使用时可完全阻断该电流。结合之前的研究工作(Satow, Y., Kung, C., 1976, J. Exp. Biol. 65:51 - 63),确定这是一种K⁺电流。进一步研究发现它是一种钙激活的K⁺电流,因为当用注入的EGTA缓冲胞内钙时,这种增加的外向K⁺电流无法被诱发。阻断内向钙电流的突变体pwB,也能阻断teaA中这种增加的外向K⁺电流。这表明该突变体电流是通过正常的去极化敏感钙通道被钙激活的。虽然尾电流衰减动力学分析表明,这种钙依赖性K⁺电流在突变体和野生型中的表观失活速率相同,但teaA电流激活极快。在2毫秒内即可完全激活。如此大的外向电流的早期激活导致teaA突变体动作电位幅度出现特征性降低。teaA突变对所检测的任何其他电生理参数均无影响。因此,teaA突变体的表型是对去极化刺激的反应性普遍降低,原因是一种快速激活的钙依赖性K⁺电流使动作电位过早复极化。

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