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大电导钙激活钾通道的 N 端同工型受辅助β1 亚基的差异调节。

N-terminal isoforms of the large-conductance Ca²⁺-activated K⁺ channel are differentially modulated by the auxiliary β1-subunit.

机构信息

From the Department of Obstetrics and Gynecology, Washington University in St. Louis School of Medicine, St. Louis, Missouri 63110 and.

出版信息

J Biol Chem. 2014 Apr 4;289(14):10095-103. doi: 10.1074/jbc.M113.521526. Epub 2014 Feb 25.

Abstract

The large-conductance Ca(2+)-activated K(+) (BK(Ca)) channel is essential for maintaining the membrane in a hyperpolarized state, thereby regulating neuronal excitability, smooth muscle contraction, and secretion. The BK(Ca) α-subunit has three predicted initiation codons that generate proteins with N-terminal ends starting with the amino acid sequences MANG, MSSN, or MDAL. Because the N-terminal region and first transmembrane domain of the α-subunit are required for modulation by auxiliary β1-subunits, we examined whether β1 differentially modulates the N-terminal BK(Ca) α-subunit isoforms. In the absence of β1, all isoforms had similar single-channel conductances and voltage-dependent activation. However, whereas β1 did not modulate the voltage-activation curve of MSSN, β1 induced a significant leftward shift of the voltage activation curves of both the MDAL and MANG isoforms. These shifts, of which the MDAL was larger, occurred at both 10 μM and 100 μM Ca(2+). The β1-subunit increased the open dwell times of all three isoforms and decreased the closed dwell times of MANG and MDAL but increased the closed dwell times of MSSN. The distinct modulation of voltage activation by the β1-subunit may be due to the differential effect of β1 on burst duration and interburst intervals observed among these isoforms. Additionally, we observed that the related β2-subunit induced comparable leftward shifts in the voltage-activation curves of all three isoforms, indicating that the differential modulation of these isoforms was specific to β1. These findings suggest that the relative expression of the N-terminal isoforms can fine-tune BK(Ca) channel activity in cells, highlighting a novel mechanism of BK(Ca) channel regulation.

摘要

大电导钙激活钾(BK(Ca)) 通道对于维持膜的超极化状态至关重要,从而调节神经元兴奋性、平滑肌收缩和分泌。BK(Ca)α 亚基有三个预测的起始密码子,产生以 MANG、MSSN 或 MDAL 氨基酸序列开头的 N 端蛋白。由于 α 亚基的 N 端区域和第一跨膜域对于辅助β1 亚基的调节是必需的,我们研究了β1 是否差异调节 N 端 BK(Ca)α 亚基同工型。在没有β1 的情况下,所有同工型的单通道电导和电压依赖性激活都相似。然而,β1 不调节 MSSN 的电压激活曲线,而β1 诱导 MDAL 和 MANG 同工型的电压激活曲线都发生明显的左移。这些移位,MDAL 更大,发生在 10 μM 和 100 μM Ca(2+) 时。β1 亚基增加了所有三种同工型的开放停留时间,并减少了 MANG 和 MDAL 的关闭停留时间,但增加了 MSSN 的关闭停留时间。β1 亚基对电压激活的差异调节可能是由于β1 对这些同工型中观察到的爆发持续时间和爆发间隔的差异影响。此外,我们观察到相关的β2 亚基诱导所有三种同工型的电压激活曲线发生类似的左移,表明这些同工型的差异调节是特异性的β1。这些发现表明,N 端同工型的相对表达可以微调细胞中 BK(Ca) 通道的活性,突出了 BK(Ca) 通道调节的新机制。

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