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Permeant Ion-Dependent Changes in Gating of Kir2.1 Inward Rectifier Potassium Channels

机译:Kir2.1内向整流器钾离子通道门控中离子的离子依赖性变化

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摘要

We studied the effect of monovalent thallium ion (Tl+) on the gating of single Kir2.1 channels, which open and close spontaneously at a constant membrane potential. In cell-attached recordings of single-channel inward current, changing the external permeant ion from K+ to Tl+ decreases the mean open-time by ∼20-fold. Furthermore, the channel resides predominantly at a subconductance level, which results from a slow decay (τ = 2.7 ms at −100 mV) from the fully open level immediately following channel opening. Mutation of a pore-lining cysteine (C169) to valine abolishes the slow decay and subconductance level, and single-channel recordings from channels formed by tandem tetramers containing one to three C169V mutant subunits indicate that Tl+ must interact with at least three C169 residues to induce these effects. However, the C169V mutation does not alter the single-channel closing kinetics of Tl+ current. These results suggest that Tl+ ions change the conformation of the ion conduction pathway during permeation and alter gating by two distinct mechanisms. First, they interact with the thiolate groups of C169 lining the cavity to induce conformational changes of the ion passageway, and thereby produce a slow decay of single-channel current and a dominant subconductance state. Second, they interact more strongly than K+ with the main chain carbonyl oxygens lining the selectivity filter to destabilize the open state of the channel and, thus, alter the open/close kinetics of gating. In addition to altering gating, Tl+ greatly diminishes Ba2+ block. The unblocking rate of Ba2+ is increased by >22-fold when the external permeant ion is switched from K+ to Tl+ regardless of the direction of Ba2+ exit. This effect cannot be explained solely by ion–ion interactions, but is consistent with the notion that Tl+ induces conformational changes in the selectivity filter.
机译:我们研究了单价th离子(Tl + )对单个Kir2.1通道的门控的影响,该通道在恒定的膜电位下自发打开和关闭。在单通道流入电流的细胞附着记录中,将外部渗透离子从K + 更改为Tl + 可使平均打开时间减少约20倍。此外,通道主要位于亚导水平,这是由于紧随通道打开之后的完全断开水平的缓慢衰减(τ= 2.7 ms,-100 mV)引起的。将有孔的半胱氨酸(C169)突变为缬氨酸消除了缓慢的衰变和亚电导水平,并且由包含一到三个C169V突变亚基的串联四聚体形成的通道的单通道记录表明,Tl + 必须与至少三个C169残基相互作用以诱导这些作用。但是,C169V突变不会改变Tl + 电流的单通道闭合动力学。这些结果表明,Tl + 离子在渗透过程中改变了离子传导途径的构象,并通过两种不同的机制改变了门控。首先,它们与衬在空腔内的C169的硫醇盐基相互作用,诱导离子通道的构象变化,从而产生缓慢的单通道电流衰减和主要的亚电导状态。其次,它们与K + 相互作用更强,与选择性过滤器衬里的主链羰基氧相互作用来破坏通道的打开状态,从而改变门控的打开/关闭动力学。除了改变选通之外,Tl + 大大减小了Ba 2 + 块。当外部渗透离子从K + 切换为Tl + 时,Ba 2 + 的解封速率增加> 22倍Ba 2 + 的出口方向。这种作用不能仅通过离子-离子相互作用来解释,而是与Tl + 引起选择性滤光片中构象变化的观点一致。

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