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脑胶质细胞中不依赖水通道蛋白4的Kir4.1钾离子通道功能

Aquaporin-4 independent Kir4.1 K+ channel function in brain glial cells.

作者信息

Zhang Hua, Verkman A S

机构信息

Departments of Medicine and Physiology, Cardiovascular Research Institute, University of California, San Francisco, CA 94143-0521, USA.

出版信息

Mol Cell Neurosci. 2008 Jan;37(1):1-10. doi: 10.1016/j.mcn.2007.08.007. Epub 2007 Aug 15.

Abstract

Functional interaction of glial water channel aquaporin-4 (AQP4) and inwardly rectifying K+ channel Kir4.1 has been suggested from their apparent colocalization and biochemical interaction, and from the slowed glial cell K+ uptake in AQP4-deficient brain. Here, we report multiple lines of evidence against functionally significant AQP4-Kir4.1 interactions. Whole-cell patch-clamp of freshly isolated glial cells from brains of wild-type and AQP4 null mice showed no significant differences in membrane potential, barium-sensitive Kir4.1 K+ current or current-voltage curves. Single-channel patch-clamp showed no differences in Kir4.1 unitary conductance, voltage-dependent open probability or current-voltage relationship. Also, Kir4.1 protein expression and distribution were similar in wild-type and AQP4 null mouse brain and in the freshly isolated glial cells. Functional inhibition of Kir4.1 by barium or RNAi knock-down in primary glial cell cultures from mouse brain did not significantly alter AQP4 water permeability, as assayed by calcein fluorescence quenching following osmotic challenge. These studies provide direct evidence against functionally significant AQP4-Kir4.1 interactions in mouse glial cells, indicating the need to identify new mechanism(s) to account for altered seizure dynamics and extracellular space K+ buffering in AQP4 deficiency.

摘要

从胶质水通道水通道蛋白4(AQP4)和内向整流钾通道Kir4.1明显的共定位、生化相互作用以及AQP4缺陷型大脑中胶质细胞钾离子摄取减缓等方面,提示了它们之间存在功能相互作用。在此,我们报告了多条证据反对AQP4与Kir4.1之间存在功能上显著的相互作用。对野生型和AQP4基因敲除小鼠大脑中新鲜分离的胶质细胞进行全细胞膜片钳记录,结果显示膜电位、钡敏感的Kir4.1钾电流或电流-电压曲线均无显著差异。单通道膜片钳记录显示,Kir4.1的单位电导、电压依赖性开放概率或电流-电压关系也没有差异。此外,野生型和AQP4基因敲除小鼠大脑以及新鲜分离的胶质细胞中,Kir4.1蛋白的表达和分布相似。在用钡或RNA干扰敲低小鼠大脑原代胶质细胞培养物中的Kir4.1功能后,通过渗透压刺激后钙黄绿素荧光淬灭检测发现,AQP4的水通透性并未显著改变。这些研究提供了直接证据,反对小鼠胶质细胞中AQP4与Kir4.1之间存在功能上显著的相互作用,这表明需要确定新的机制来解释AQP4缺乏时癫痫发作动力学改变和细胞外空间钾离子缓冲的现象。

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