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低离子强度下轮藻中重水诱导的离子通道激活。

D2O-induced ion channel activation in Characeae at low ionic strength.

作者信息

Andjus P R, Kataev A A, Alexandrov A A, Vucelić D, Berestovsky G N

机构信息

Institute of Cell Biophysics, Russian Academy of Sciences, Puschino, Moscow region.

出版信息

J Membr Biol. 1994 Oct;142(1):43-53. doi: 10.1007/BF00233382.

Abstract

Effects of D2O were studied on internodal cells of the freshwater alga Nitellopsis obtusa under plasmalemma perfusion (tonoplast-free cells) with voltage clamp, and on Ca2+ channels isolated from the alga and reconstituted in bilayer lipid membranes (BLM). External application of artificial pond water (APW) with D2O as the solvent to the perfused plasmalemma preparation led to an abrupt drop of membrane resistance (Rm = 0.12 +/- 0.03 k omega.cm2), thus preventing further voltage clamping. APW with 25% D2O caused a two-step reduction of Rm: first, down to 2.0 +/- 0.8 k omega.cm2, and then further to 200 omega.cm2, in 2 min. It was shown that in the first stage, Ca2+ channels are activated, and then, Ca2+ ions entering through them activate the Cl- channels. The Ca2+ channels are activated irreversibly. If 100 mM CsCl was substituted for 200 mM sucrose (introduced for iso-osmoticity), no effect of D2O on Rm was observed. Intracellular H2O/D2O substitution also did not change Rm. In experiments on single Ca2+ channels in BLM H2O/D2O substitution in a solution containing 100 mM KCl (trans side) produced no effect on channel activity, while in 10 mM KCl, at negative voltage, the open channel probability sharply increased. This effect was irreversible. The single channel conductance was not altered after the H2O/D2O substitution. The discussion of the possible mechanism of D2O action on Ca2+ and Cl- channels was based on an osmotic-like stress effect and the phenomenon of higher D-bond energy compared to the H-bond.

摘要

在质膜灌流(无液泡膜细胞)条件下,利用电压钳研究了重水(D₂O)对淡水藻类钝节拟丽藻节间细胞的影响,以及对从该藻类分离并重构于双层脂质膜(BLM)中的Ca²⁺通道的影响。以D₂O为溶剂的人工池塘水(APW)外部施加于灌流的质膜制剂,导致膜电阻(Rm = 0.12 +/- 0.03 kΩ·cm²)突然下降,从而阻止了进一步的电压钳制。含25% D₂O的APW使Rm分两步降低:首先降至2.0 +/- 0.8 kΩ·cm²,然后在2分钟内进一步降至200 Ω·cm²。结果表明,在第一阶段,Ca²⁺通道被激活,然后,通过它们进入的Ca²⁺离子激活Cl⁻通道。Ca²⁺通道被不可逆地激活。如果用100 mM CsCl替代200 mM蔗糖(用于等渗),则未观察到D₂O对Rm的影响。细胞内H₂O/D₂O替代也未改变Rm。在BLM中对单个Ca²⁺通道进行的实验中,在含100 mM KCl(反侧)的溶液中进行H₂O/D₂O替代对通道活性无影响,而在10 mM KCl中,在负电压下,开放通道概率急剧增加。这种效应是不可逆的。H₂O/D₂O替代后单通道电导未改变。基于类似渗透的应力效应以及与氢键相比更高的D键能现象,对D₂O作用于Ca²⁺和Cl⁻通道的可能机制进行了讨论。

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