首页> 美国卫生研究院文献>Biophysical Journal >Hydrophobic mutations alter the movement of Mg2+ in the pore of voltage-gated potassium channels.
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Hydrophobic mutations alter the movement of Mg2+ in the pore of voltage-gated potassium channels.

机译:疏水性突变会改变电压门控钾通道孔中Mg2 +的运动。

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摘要

The permeation pathways of the voltage-gated K+ channels Kv3.1 and ShakerB delta 6-46 (ShB delta) were studied using Mg2+ block. Internal Mg2+ blocked both channels in a voltage-dependent manner, and block was partially relieved by external K+, consistent with Mg2+ binding within the pore. The kinetics of Mg2+ block was much faster for Kv3.1 than for ShB delta. Fast block of Kv3.1 was transferred to ShB delta with transplantation of the P-region, but not of S6. The difference in the P-region, causing the change in Mg2+ binding kinetics, was attributed to ShB delta (V443) and its analog Kv3.1(L401), because in both channels leucine at this position gave fast block, whereas valine gave slow block. For Kv3.1 the major determinant of the voltage dependence of Mg2+ binding resided primarily in the off rate, whereas for Kv3.1(L401V) the voltage dependence resided primarily in the on rate, consistent with a change in the rate-limiting barrier for Mg2+ binding. Our data suggest that hydrophobic residues at positions 401 of Kv3.1 and 443 of ShB delta act as barriers to the movement of Mg2+ in the pore.
机译:使用Mg2 +阻滞研究了电压门控K +通道Kv3.1和ShakerB delta 6-46(ShB delta)的渗透途径。内部Mg2 +以电压依赖的方式阻断了两个通道,并且外部K +解除了部分阻断,这与孔中Mg2 +的结合相一致。 Kv3.1的Mg2 +阻滞动力学比ShBδ快得多。 Kv3.1的快速阻滞通过P区移植而不是S6移植到ShB delta。 P区域的差异导致Mg2 +结合动力学的变化,归因于ShB delta(V443)及其类似物Kv3.1(L401),因为在这两个通道中,亮氨酸在此位置均提供快速阻滞,而缬氨酸则提供缓慢的阻滞。块。对于Kv3.1,Mg2 +结合的电压依赖性的主要决定因素主要在于截止速率,而对于Kv3.1(L401V),电压依赖性主要取决于导通速率,这与限制速率的限制有关。 Mg2 +结合。我们的数据表明,Kv3.1的401位和ShB delta的443位的疏水残基充当Mg2 +在孔中运动的障碍。

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