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视网膜Müller细胞中水通道蛋白4水通道与Kir4.1钾通道之间不存在功能相互作用的证据。

Evidence against functional interaction between aquaporin-4 water channels and Kir4.1 potassium channels in retinal Müller cells.

作者信息

Ruiz-Ederra Javier, Zhang Hua, Verkman A S

机构信息

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

出版信息

J Biol Chem. 2007 Jul 27;282(30):21866-72. doi: 10.1074/jbc.M703236200. Epub 2007 May 24.

DOI:10.1074/jbc.M703236200
PMID:17525153
Abstract

Indirect evidence suggests that the Müller/glial cell water channel aquaporin-4 (AQP4) modulates K(+) channel function of the closely associated Kir4.1 protein. We used patch clamp to compare Kir4.1 K(+) channel function in freshly isolated Müller cells from retinas of wild-type (+/+) and AQP4 knock-out (-/-) mice. Immunocytochemistry showed a comparable Kir4.1 protein expression pattern in Müller cells from +/+ and -/- retinas, with greatest expression at their end feet. Osmotic water permeability was >4-fold reduced in -/- than in +/+ Müller cells. Resting membrane potential did not differ significantly in +/+ versus -/- Müller cells (-64 +/- 1 versus -64 +/- 1 mV, S.E., n = 24). Whole-cell K(+) currents recorded with a micropipette inserted into the cell soma were Ba(2+)-sensitive and showed no significant differences in magnitude in +/+ versus -/- Müller cells (1.3 +/- 0.1 versus 1.2 +/- 0.1 nA at -160 mV) or in inwardly rectifying current-voltage relationships. Spatially resolved K(+) currents generated by pulsed K(+) injections along Müller cell bodies were also comparable in +/+ versus -/- Müller cells. Single-channel cell-attached patch clamp showed comparable unitary conductance, current-voltage data, and open probability in +/+ versus -/- Müller cells. Thus, contrary to the generally accepted view, our results provide direct evidence against functionally significant AQP4 modulation of Müller cell Kir4.1 K(+) channel function.

摘要

间接证据表明,米勒细胞/神经胶质细胞水通道水通道蛋白4(AQP4)可调节紧密相关的Kir4.1蛋白的钾离子通道功能。我们使用膜片钳技术比较了野生型(+/+)和AQP4基因敲除型(-/-)小鼠视网膜新鲜分离的米勒细胞中Kir4.1钾离子通道的功能。免疫细胞化学显示,+/+和-/-视网膜的米勒细胞中Kir4.1蛋白表达模式相似,在其终足处表达最高。-/-米勒细胞的渗透水通透性比+/+米勒细胞降低了4倍以上。+/+和-/-米勒细胞的静息膜电位无显著差异(-64±1mV对-64±1mV,标准误,n = 24)。用微电极插入细胞体记录的全细胞钾电流对钡离子敏感,在+/+和-/-米勒细胞中,其大小无显著差异(在-160mV时为1.3±0.1nA对1.2±0.1nA),内向整流电流-电压关系也无显著差异。沿米勒细胞体进行脉冲钾离子注射产生的空间分辨钾电流在+/+和-/-米勒细胞中也相似。单通道细胞贴附式膜片钳显示,+/+和-/-米勒细胞的单位电导、电流-电压数据和开放概率相似。因此,与普遍接受的观点相反,我们的结果提供了直接证据,反对AQP4对米勒细胞Kir4.1钾离子通道功能进行功能上显著的调节。

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