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活动诱发的 K 瞬变清除和相关的胶质细胞肿胀与 AQP4 无关:使用 AQP4 同工型选择性抑制剂的研究。

Clearance of activity-evoked K transients and associated glia cell swelling occur independently of AQP4: A study with an isoform-selective AQP4 inhibitor.

机构信息

Department of Neuroscience, Faculty of Health and Medical Sciences, University of Copenhagen, Copenhagen, Denmark.

Department of Drug Design and Pharmacology, Faculty of Health and Medical Sciences, University of Copenhagen, Copenhagen, Denmark.

出版信息

Glia. 2021 Jan;69(1):28-41. doi: 10.1002/glia.23851. Epub 2020 Jun 7.

DOI:10.1002/glia.23851
PMID:32506554
Abstract

The mammalian brain consists of 80% water, which is continuously shifted between different compartments and cellular structures by mechanisms that are, to a large extent, unresolved. Aquaporin 4 (AQP4) is abundantly expressed in glia and ependymal cells of the mammalian brain and has been proposed to act as a gatekeeper for brain water dynamics, predominantly based on studies utilizing AQP4-deficient mice. However, these mice have a range of secondary effects due to the gene deletion. An efficient and selective AQP4 inhibitor has thus been sorely needed to validate the results obtained in the AQP4 mice to quantify the contribution of AQP4 to brain fluid dynamics. In AQP4-expressing Xenopus laevis oocytes monitored by a high-resolution volume recording system, we here demonstrate that the compound TGN-020 is such a selective AQP4 inhibitor. TGN-020 targets the tested species of AQP4 with an IC of ~3.5 μM, but displays no inhibitory effect on the other AQPs (AQP1-AQP9). With this tool, we employed rat hippocampal slices and ion-sensitive microelectrodes to determine the role of AQP4 in glia cell swelling following neuronal activity. TGN-020-mediated inhibition of AQP4 did not prevent stimulus-induced extracellular space shrinkage, nor did it slow clearance of the activity-evoked K transient. These data, obtained with a verified isoform-selective AQP4 inhibitor, indicate that AQP4 is not required for the astrocytic contribution to the K clearance or the associated extracellular space shrinkage.

摘要

哺乳动物的大脑由 80%的水组成,这些水通过多种机制在不同的隔室和细胞结构之间不断转移,但这些机制在很大程度上尚未得到解决。水通道蛋白 4(AQP4)在哺乳动物大脑的神经胶质细胞和室管膜细胞中大量表达,并被提议作为脑水动力学的“守门员”,这主要基于利用 AQP4 缺陷型小鼠进行的研究。然而,由于基因缺失,这些小鼠存在一系列的次要影响。因此,迫切需要一种高效且选择性的 AQP4 抑制剂来验证在 AQP4 小鼠中获得的结果,以量化 AQP4 对脑液动力学的贡献。在这里,我们使用高分辨率体积记录系统监测表达 AQP4 的非洲爪蟾卵母细胞,证明了化合物 TGN-020 是一种具有选择性的 AQP4 抑制剂。TGN-020 以约 3.5 μM 的 IC 靶向测试的 AQP4 物种,但对其他 AQP(AQP1-AQP9)没有抑制作用。有了这个工具,我们采用大鼠海马切片和离子敏感微电极来确定 AQP4 在神经元活动后神经胶质细胞肿胀中的作用。AQP4 的 TGN-020 介导的抑制作用并没有阻止刺激诱导的细胞外空间收缩,也没有减缓活性诱发的 K 瞬变的清除。这些使用经过验证的同工型选择性 AQP4 抑制剂获得的数据表明,AQP4 对于星形胶质细胞对 K 清除或相关细胞外空间收缩的贡献不是必需的。

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