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用于钙成像的急性脑室下区切片的制备。

Preparation of acute subventricular zone slices for calcium imaging.

作者信息

Lacar Benjamin, Young Stephanie Z, Platel Jean-Claude, Bordey Angélique

机构信息

Department of Neurosurgery and Cellular & Molecular Physiology, Yale University School of Medicine, CT, USA.

出版信息

J Vis Exp. 2012 Sep 19(67):e4071. doi: 10.3791/4071.

Abstract

The subventricular zone (SVZ) is one of the two neurogenic zones in the postnatal brain. The SVZ contains densely packed cells, including neural progenitor cells with astrocytic features (called SVZ astrocytes), neuroblasts, and intermediate progenitor cells. Neuroblasts born in the SVZ tangentially migrate a great distance to the olfactory bulb, where they differentiate into interneurons. Intercellular signaling through adhesion molecules and diffusible signals play important roles in controlling neurogenesis. Many of these signals trigger intercellular calcium activity that transmits information inside and between cells. Calcium activity is thus reflective of the activity of extracellular signals and is an optimal way to understand functional intercellular signaling among SVZ cells. Calcium activity has been studied in many other regions and cell types, including mature astrocytes and neurons. However, the traditional method to load cells with calcium indicator dye (i.e. bath loading) was not efficient at loading all SVZ cell types. Indeed, the cellular density in the SVZ precludes dye diffusion inside the tissue. In addition, preparing sagittal slices will better preserve the three-dimensional arrangement of SVZ cells, particularly the stream of neuroblast migration on the rostral-caudal axis. Here, we describe methods to prepare sagittal sections containing the SVZ, the loading of SVZ cells with calcium indicator dye, and the acquisition of calcium activity with time-lapse movies. We used Fluo-4 AM dye for loading SVZ astrocytes using pressure application inside the tissue. Calcium activity was recorded using a scanning confocal microscope allowing a precise resolution for distinguishing individual cells. Our approach is applicable to other neurogenic zones including the adult hippocampal subgranular zone and embryonic neurogenic zones. In addition, other types of dyes can be applied using the described method.

摘要

室下区(SVZ)是出生后大脑中的两个神经发生区之一。SVZ包含紧密排列的细胞,包括具有星形胶质细胞特征的神经祖细胞(称为SVZ星形胶质细胞)、神经母细胞和中间祖细胞。在SVZ产生的神经母细胞沿切线方向远距离迁移至嗅球,在那里它们分化为中间神经元。通过黏附分子和可扩散信号进行的细胞间信号传导在控制神经发生中起重要作用。这些信号中的许多会触发细胞间钙活性,从而在细胞内和细胞间传递信息。因此,钙活性反映了细胞外信号的活性,是了解SVZ细胞间功能信号传导的最佳方式。钙活性已在许多其他区域和细胞类型中进行了研究,包括成熟的星形胶质细胞和神经元。然而,用钙指示剂染料加载细胞的传统方法(即浴加载)在加载所有SVZ细胞类型时效率不高。实际上,SVZ中的细胞密度会阻止染料在组织内扩散。此外,制备矢状切片将更好地保留SVZ细胞的三维排列,特别是神经母细胞在头尾轴上的迁移流。在这里,我们描述了制备包含SVZ的矢状切片、用钙指示剂染料加载SVZ细胞以及通过延时电影获取钙活性的方法。我们使用Fluo-4 AM染料通过在组织内施加压力来加载SVZ星形胶质细胞。使用扫描共聚焦显微镜记录钙活性,该显微镜具有精确的分辨率以区分单个细胞。我们的方法适用于其他神经发生区,包括成年海马颗粒下区和胚胎神经发生区。此外,可以使用所述方法应用其他类型的染料。

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