Visualization of Gap Junction-Mediated Astrocyte Coupling in Acute Mouse Brain Slices

急性小鼠脑切片中间隙连接介导的星形胶质细胞偶联的可视化

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作者:Nine F Kompier, Gabrielle Siemonsmeier, Niklas Meyer, Helmut Kettenmann, Fritz G Rathjen

Abstract

Gap junctions are transmembrane protein channels that enable the exchange of small molecules such as ions, second messengers, and metabolites between adjacent cells. Gap junctions are found in various mammalian organs, including skin, endothelium, liver, pancreas, muscle, and central nervous system (CNS). In the CNS, they mediate coupling between neural cells including glial cells, and the resulting panglial networks are vital for brain homeostasis. Tracers of sufficiently small molecular mass can diffuse across gap junctions and are used to visualize the extent of cell-to-cell coupling in situ by delivering them to a single cell through sharp electrodes or patch-clamp micropipettes. Here, we describe a protocol for pre-labeling and identification of astrocytes in acute mouse forebrain slices using Sulforhodamine 101 (SR101). Fluorescent cells can then be targeted for whole-cell patch-clamp, which allows for further confirmation of astroglial identity by assessing their electrophysiological properties, as well as for passive dialysis with a tracer such as biocytin. Slices can then be subjected to chemical fixation and immunostaining to detect dye-coupled networks. This protocol provides a method for the identification of astrocytes in live tissue through SR101 labeling. Alternatively, transgenic reporter mice can also be used to identify astrocytes. While we illustrate the use of this protocol for the study of glial networks in the mouse brain, the general principles are applicable to other species, tissues, and cell types. Key features • Pre-labeling of live astrocytes in acute adult mouse brain slices using the dye Sulforhodamine 101. • Dialysis of biocytin into individual astrocytes using whole-cell patch-clamp electrophysiology. • Staining of biocytin by streptavidin and immunostaining of GFAP, imaging, and analysis of dye-coupled astrocytic networks. • Can be used for other glial cell types and might be adapted to other tissues and species.

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