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FM 染料通过钙库操纵型钙通道进入细胞,并改变培养星形胶质细胞的钙信号。

FM dyes enter via a store-operated calcium channel and modify calcium signaling of cultured astrocytes.

机构信息

Institut National de la Santé et de la Recherche Médicale, INSERM U603, Centre National de la Recherche Scientifique, UMR 8154, Laboratoire de Neurophysiologie & Nouvelles Microscopies, Université Paris Descartes, 45 Rue des Saints Pères, F-75006 Paris, France.

出版信息

Proc Natl Acad Sci U S A. 2009 Dec 22;106(51):21960-5. doi: 10.1073/pnas.0909109106. Epub 2009 Dec 9.

Abstract

The amphiphilic fluorescent styryl pyridinium dyes FM1-43 and FM4-64 are used to probe activity-dependent synaptic vesicle cycling in neurons. Cultured astrocytes can internalize FM1-43 and FM4-64 inside vesicles but their uptake is insensitive to the elevation of cytosolic calcium (Ca(2+)) concentration and the underlying mechanism remains unclear. Here we used total internal reflection fluorescence microscopy and pharmacological tools to study the mechanisms of FM4-64 uptake into cultured astrocytes from mouse neocortex. Our data show that: (i) endocytosis is not a major route for FM4-64 uptake into astrocytes; (ii) FM4-64 enters astrocytes through an aqueous pore and strongly affects Ca(2+) homeostasis; (iii) partitioning of FM4-64 into the outer leaflet of the plasma membrane results in a facilitation of store-operated Ca(2+) entry (SOCE) channel gating; (iv) FM4-64 permeates and competes with Ca(2+) for entry through a SOCE channel; (v) intracellular FM4-64 mobilizes Ca(2+) from the endoplasmic reticulum stores, conveying a positive feedback to activate SOCE and to sustain dye uptake into astrocytes. Our study demonstrates that FM dyes are not markers of cycling vesicles in astrocytes and calls for a careful interpretation of FM fluorescence.

摘要

两亲性荧光苯乙烯吡啶鎓染料 FM1-43 和 FM4-64 被用于探测神经元中依赖活动的突触囊泡循环。培养的星形胶质细胞可以将 FM1-43 和 FM4-64 内化到囊泡内,但它们的摄取对细胞质钙离子(Ca(2+))浓度的升高不敏感,其潜在机制尚不清楚。在这里,我们使用全内反射荧光显微镜和药理学工具来研究 FM4-64 从培养的来自小鼠新皮质的星形胶质细胞摄取的机制。我们的数据表明:(i)内吞作用不是 FM4-64 进入星形胶质细胞的主要途径;(ii)FM4-64 通过水孔进入星形胶质细胞,并强烈影响 Ca(2+) 稳态;(iii)FM4-64 分配到质膜的外叶导致易化储存操作的 Ca(2+) 内流(SOCE)通道门控;(iv)FM4-64 通过 SOCE 通道渗透并与 Ca(2+) 竞争进入;(v)细胞内的 FM4-64 从内质网库中动员 Ca(2+),对激活 SOCE 和维持染料进入星形胶质细胞的摄取产生正向反馈。我们的研究表明,FM 染料不是星形胶质细胞中循环囊泡的标志物,并呼吁对 FM 荧光进行仔细解释。

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