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通过皮质表面光漂白对脑细胞外间隙扩散进行体内测量。

In vivo measurement of brain extracellular space diffusion by cortical surface photobleaching.

作者信息

Binder Devin K, Papadopoulos Marios C, Haggie Peter M, Verkman A S

机构信息

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

出版信息

J Neurosci. 2004 Sep 15;24(37):8049-56. doi: 10.1523/JNEUROSCI.2294-04.2004.

Abstract

Molecular diffusion in the brain extracellular space (ECS) is an important determinant of neural function. We developed a brain surface photobleaching method to measure the diffusion of fluorescently labeled macromolecules in the ECS of the cerebral cortex. The ECS in mouse brain was labeled by exposure of the intact dura to fluorescein-dextrans (M(r) 4, 70, and 500 kDa). Fluorescein-dextran diffusion, detected by fluorescence recovery after laser-induced cortical photobleaching using confocal optics, was slowed approximately threefold in the brain ECS relative to solution. Cytotoxic brain edema (produced by water intoxication) or seizure activity (produced by convulsants) slowed diffusion by >10-fold and created dead-space microdomains in which free diffusion was prevented. The hindrance to diffusion was greater for the larger fluorescein-dextrans. Interestingly, slowed ECS diffusion preceded electroencephalographic seizure activity. In contrast to the slowed diffusion produced by brain edema and seizure activity, diffusion in the ECS was faster in mice lacking aquaporin-4 (AQP4), an astroglial water channel that facilitates fluid movement between cells and the ECS. Our results establish a minimally invasive method to quantify diffusion in the brain ECS in vivo, revealing stimulus-induced changes in molecular diffusion in the ECS with unprecedented spatial and temporal resolution. The in vivo mouse data provide evidence for: (1) dead-space ECS microdomains after brain swelling; (2) slowed molecular diffusion in the ECS as an early predictor of impending seizure activity; and (3) a novel role for AQP4 as a regulator of brain ECS.

摘要

分子在脑细胞外间隙(ECS)中的扩散是神经功能的一个重要决定因素。我们开发了一种脑表面光漂白方法,用于测量荧光标记的大分子在大脑皮质ECS中的扩散。通过将完整的硬脑膜暴露于荧光素-葡聚糖(分子量分别为4、70和500 kDa)来标记小鼠脑内的ECS。利用共聚焦光学系统,通过激光诱导皮质光漂白后的荧光恢复来检测荧光素-葡聚糖的扩散,结果表明,相对于溶液,大脑ECS中的荧光素-葡聚糖扩散速度减慢了约三倍。细胞毒性脑水肿(由水中毒引起)或癫痫活动(由惊厥剂引起)使扩散速度减慢了10倍以上,并产生了阻止自由扩散的死腔微区。对于较大的荧光素-葡聚糖,扩散的阻碍更大。有趣的是,ECS扩散减慢先于脑电图癫痫活动。与脑水肿和癫痫活动引起的扩散减慢相反,在缺乏水通道蛋白4(AQP4)的小鼠中,ECS中的扩散更快,AQP4是一种星形胶质细胞水通道,有助于细胞与ECS之间的液体流动。我们的研究结果建立了一种微创方法来定量体内大脑ECS中的扩散,以前所未有的空间和时间分辨率揭示了刺激诱导的ECS中分子扩散的变化。体内小鼠数据为以下方面提供了证据:(1)脑肿胀后ECS中的死腔微区;(2)ECS中分子扩散减慢作为即将发生癫痫活动的早期预测指标;(3)AQP4作为大脑ECS调节剂的新作用。

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