Elimination of the slow gating of ClC-0 chloride channel by a point mutation

被引:78
作者
Lin, YW [1 ]
Lin, CW [1 ]
Chen, TY [1 ]
机构
[1] Natl Yang Ming Univ, Dept Physiol, Taipei 11221, Taiwan
关键词
ClC-0; slow gating; Zn2+ inhibition; cysteine mutagenesis;
D O I
10.1085/jgp.114.1.1
中图分类号
Q4 [生理学];
学科分类号
071003 ;
摘要
The inactivation of the CIC-0 chloride channel is very temperature sensitive and is greatly facilitated by the binding of a zinc ion (Zn2+) from the extracellular side, leading to a Zn2+-induced current inhibition. To further explore the I elation of Zn2+ inhibition and the CIC-0 inactivation, Tie mutated all 12 cysteine amino acids in the channel and assayed the effect of Zn2+ on these mutants. With this approach, we found that C212 appears to be important for the sensitivity of the Zn2+ inhibition. Upon mutating C212 to serine or alanine, the inactivation of the channel in macroscopic current recordings disappears and the channel does not show detectable inactivation events at the single-channel level. At the same time, the channel's sensitivity to Zn2+ inhibition is also greatly reduced. The other two cysteine mutants, C213G and C480S, as well as a previously identified mutant, S123T, also affect the inactivation of the channel to some degree, but the temperature-dependent inactivation process is still present, likewise the high sensitivity of the Zn2+ inhibition. These results further support the assertion that the inhibition of Zn2+ on CIC-0 is indeed due to an effect on the inactivation of the channel. The absence of inactivation in C212S mutants may provide a better defined system to study the fast gating and the ion permeation of CIC-0.
引用
收藏
页码:1 / 12
页数:12
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