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水通道蛋白-4 通道对海马体中 K+缓冲和缝隙连接偶联的影响。

Impact of aquaporin-4 channels on K+ buffering and gap junction coupling in the hippocampus.

机构信息

Institute of Cellular Neurosciences, University of Bonn, Bonn, Germany.

出版信息

Glia. 2011 Jun;59(6):973-80. doi: 10.1002/glia.21169. Epub 2011 Mar 28.

DOI:10.1002/glia.21169
PMID:21446052
Abstract

Aquaporin-4 (AQP4) is the main water channel in the brain and primarily localized to astrocytes where the channels are thought to contribute to water and K(+) homeostasis. The close apposition of AQP4 and inward rectifier K(+) channels (Kir4.1) led to the hypothesis of direct functional interactions between both channels. We investigated the impact of AQP4 on stimulus-induced alterations of the extracellular K(+) concentration (K(+)) in murine hippocampal slices. Recordings with K(+)-selective microelectrodes combined with field potential analyses were compared in wild type (wt) and AQP4 knockout (AQP4(-/-)) mice. Astrocyte gap junction coupling was assessed with tracer filling during patch clamp recording. Antidromic fiber stimulation in the alveus evoked smaller increases and slower recovery of K(+) in the stratum pyramidale of AQP4(-/-) mice indicating reduced glial swelling and a larger extracellular space when compared with control tissue. Moreover, the data hint at an impairment of the glial Na(+)/K(+) ATPase in AQP4-deficient astrocytes. In a next step, we investigated the laminar profile of K(+) by moving the recording electrode from the stratum pyramidale toward the hippocampal fissure. At distances beyond 300 μm from the pyramidal layer, the stimulation-induced, normalized increases of K(+) in AQP4(-/-) mice exceeded the corresponding values of wt mice, indicating facilitated spatial buffering. Astrocytes in AQP4(-/-) mice also displayed enhanced tracer coupling, which might underlie the improved spatial re- distribution of K(+) in the hippocampus. These findings highlight the role of AQP4 channels in the regulation of K(+) homeostasis.

摘要

水通道蛋白-4(AQP4)是大脑中的主要水通道,主要定位于星形胶质细胞,通道被认为有助于水和 K+稳态。AQP4 与内向整流钾通道(Kir4.1)的紧密附着导致了这两种通道之间存在直接功能相互作用的假说。我们研究了 AQP4 对小鼠海马切片中刺激诱导的细胞外 K+浓度 ([K+](o))变化的影响。使用 K+选择性微电极进行记录,并结合场电位分析,在野生型(wt)和 AQP4 敲除(AQP4(-/-))小鼠中进行了比较。在膜片钳记录期间用示踪剂填充评估星形胶质细胞缝隙连接偶联。在齿状回内的逆行纤维刺激下,AQP4(-/-)小鼠的 [K+](o)增加幅度较小且恢复较慢,表明与对照组织相比,星形胶质细胞肿胀减少,细胞外空间增大。此外,数据提示 AQP4 缺陷星形胶质细胞中的胶质 Na+/K+ATP 酶受损。在下一步中,我们通过将记录电极从锥体层移向海马裂来研究 [K+](o)的层状分布。在距离锥体层 300 μm 以外的距离处,AQP4(-/-)小鼠刺激诱导的、标准化的 [K+](o)增加超过了 wt 小鼠的对应值,表明空间缓冲作用增强。AQP4(-/-)小鼠的星形胶质细胞也显示出增强的示踪剂偶联,这可能是海马中 [K+](o)的空间再分布得到改善的原因。这些发现强调了 AQP4 通道在 K+稳态调节中的作用。

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