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钙激活钾通道在腮腺细胞:BK 通道超极化激活的功能基础。

Ca2+-activated K channels in parotid acinar cells: The functional basis for the hyperpolarized activation of BK channels.

机构信息

Department of Pharmacology and Physiology, University of Rochester School of Medicine and Dentistry, Rochester, NY, USA.

出版信息

Channels (Austin). 2010 Jul-Aug;4(4):278-88. doi: 10.4161/chan.4.4.12197. Epub 2010 Jul 28.

Abstract

Fluid secretion relies on a close interplay between Ca(2+)-activated Cl and K channels. Salivary acinar cells contain both large conductance, BK, and intermediate conductance, IK1, K channels. Physiological fluid secretion occurs with only modest (<500 nM) increases in intracellular Ca(2+) levels but BK channels in many cell types and in heterologous expression systems require very high concentrations for significant activation. We report here our efforts to understand this apparent contradiction. We determined the Ca(2+) dependence of IK1 and BK channels in mouse parotid acinar cells. IK1 channels activated with an apparent Ca(2+) affinity of about 350 nM and a Hill coefficient near 3. Native parotid BK channels activated at similar Ca(2+) levels unlike the BK channels in other cell types. Since the parotid BK channel is encoded by an uncommon splice variant, we examined this clone in a heterologous expression system. In contrast to the native parotid channel, activation of this expressed "parSlo" channel required very high levels of Ca(2+). In order to understand the functional basis for the special properties of the native channels, we analyzed the parotid BK channel in the context of the Horrigan-Aldrich model of BK channel gating. We found that the shifted activation of parotid BK channels resulted from a hyperpolarizing shift of the voltage dependence of voltage sensor activation and channel opening and included a large change in the coupling of these two processes.

摘要

液体分泌依赖于 Ca(2+)激活的 Cl 和 K 通道之间的紧密相互作用。唾液腺泡细胞包含大电导、BK 和中等电导、IK1、K 通道。生理液体分泌发生在细胞内 Ca(2+)水平仅适度增加(<500 nM)的情况下,但在许多细胞类型和异源表达系统中,BK 通道需要非常高的浓度才能显著激活。我们在这里报告了我们理解这一明显矛盾的努力。我们确定了小鼠腮腺腺泡细胞中 IK1 和 BK 通道的 Ca(2+)依赖性。IK1 通道以约 350 nM 的表观 Ca(2+)亲和力和接近 3 的 Hill 系数激活。天然腮腺 BK 通道在类似的 Ca(2+)水平下激活,与其他细胞类型中的 BK 通道不同。由于腮腺 BK 通道由一种罕见的剪接变体编码,我们在异源表达系统中研究了这个克隆。与天然腮腺通道相反,这种表达的“parSlo”通道的激活需要非常高的 Ca(2+)水平。为了理解天然通道特殊性质的功能基础,我们在 Horrigan-Aldrich 模型的背景下分析了腮腺 BK 通道的门控。我们发现,腮腺 BK 通道的激活移位是由于电压传感器激活和通道打开的电压依赖性的超极化移位引起的,并且包括这两个过程的耦合的很大变化。

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