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克隆的植物钾离子通道在非洲爪蟾卵母细胞中的表达:宏观电流分析

Expression of a cloned plant K+ channel in Xenopus oocytes: analysis of macroscopic currents.

作者信息

Véry A A, Gaymard F, Bosseux C, Sentenac H, Thibaud J B

机构信息

Laboratoire de Biochimie et Physiologie Végétales, URA 573 CNRS, ENSA.M-INRA, Montpellier, France.

出版信息

Plant J. 1995 Feb;7(2):321-32. doi: 10.1046/j.1365-313x.1995.7020321.x.

Abstract

The open reading frame from the Arabidopsis thaliana KAT1 cDNA was cloned in a transcription plasmid between the 3' and 5' untranslated regions of a beta-globin cDNA from Xenopus oocyte. The polyadenylated transcripts resulting from in vitro transcription gave rise to high levels of expression of KAT1 channel when injected in Xenopus oocytes. Upon hyperpolarization, a slow activating current could be recorded, inwardly- or outwardly-directed, depending on K+ external concentration. Predictions of the voltage-gated channel theory were shown to fit the data well. The equivalent gating charge and the half-activation potential ranged around 2 and -145 mV, respectively. KAT1 gating characteristics did not depend on K+ external concentration nor on external pH in the 5.0-7.5 range. KAT1 conductance was, however, increased (40%) when external pH was decreased from 6.5 to 5.0. The apparent affinity constant of KAT1 for K+ lay in the range 15-30 mM, at external pH 7.4. As for many K+ channels of animal cells, external caesium caused a voltage-dependent blockage of inward (but not outward) KAT1 current, whereas tetraethylammonium caused a voltage-independent block of both inward and outward KAT1 currents. In conclusion, high levels of expression made it possible to carry out the first quantitative analysis of KAT1 macroscopic currents. KAT1 channel was shown to display features similar to those of as yet uncloned inward-rectifying voltage-gated channels described in both plant cells (namely guard cells) and animal cells.

摘要

拟南芥KAT1 cDNA的开放阅读框被克隆到一个转录质粒中,该质粒位于非洲爪蟾卵母细胞β-珠蛋白cDNA的3'和5'非翻译区之间。体外转录产生的聚腺苷酸化转录本在注射到非洲爪蟾卵母细胞后能高水平表达KAT1通道。超极化时,可记录到一种缓慢激活的电流,其方向向内或向外,这取决于外部K+浓度。电压门控通道理论的预测结果与数据拟合良好。等效门控电荷和半激活电位分别约为2和-145 mV。KAT1的门控特性不依赖于外部K+浓度,也不依赖于5.0 - 7.5范围内的外部pH值。然而,当外部pH值从6.5降至5.0时,KAT1的电导增加了40%。在外部pH值为7.4时,KAT1对K+的表观亲和常数在15 - 30 mM范围内。与许多动物细胞的K+通道一样,外部铯会导致KAT1内向电流(但不是外向电流)的电压依赖性阻断,而四乙铵会导致KAT1内向和外向电流的电压非依赖性阻断。总之,高水平的表达使得对KAT1宏观电流进行首次定量分析成为可能。结果表明,KAT1通道具有与植物细胞(即保卫细胞)和动物细胞中描述的尚未克隆的内向整流电压门控通道相似的特征。

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