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用于RNA分析或流式细胞术的小鼠小胶质细胞的分离。

Isolation of murine microglial cells for RNA analysis or flow cytometry.

作者信息

Cardona Astrid E, Huang DeRen, Sasse Margaret E, Ransohoff Richard M

机构信息

Neuroinflammation Research Center, Department of Neurosciences, Lerner Research Institute, Cleveland Clinic, Cleveland, Ohio 44195, USA.

出版信息

Nat Protoc. 2006;1(4):1947-51. doi: 10.1038/nprot.2006.327.

Abstract

There is increasing interest in the isolation of adult microglia to study their functions at a morphological and molecular level during normal and neuroinflammatory conditions. Microglia have important roles in brain homeostasis, and in disease states they exert neuroprotective or neurodegenerative functions. To assay expression profiles or functions of microglia, we have developed a method to isolate microglial cells and infiltrating leukocytes from adult mouse brain. This protocol uses a digestion cocktail containing collagenase and dispase, and it involves separation over discontinuous percoll gradients. Isolated cells can be used for RNA analysis, including RNase protection analysis (RPA), quantitative RT-PCR, high-density microarray, proteomic or flow cytometric characterization of cell surface markers or adoptive transfer. Cell isolation can be completed in less than 4 h.

摘要

人们对分离成年小胶质细胞以研究其在正常和神经炎症状态下的形态和分子水平功能的兴趣日益浓厚。小胶质细胞在脑内稳态中发挥重要作用,在疾病状态下,它们具有神经保护或神经退行性变功能。为了分析小胶质细胞的表达谱或功能,我们开发了一种从成年小鼠脑内分离小胶质细胞和浸润白细胞的方法。该方案使用含有胶原酶和分散酶的消化混合液,并通过不连续的 Percoll 梯度进行分离。分离出的细胞可用于 RNA 分析,包括核糖核酸酶保护分析(RPA)、定量 RT-PCR、高密度微阵列、蛋白质组学分析或细胞表面标志物的流式细胞术表征,或用于过继转移。细胞分离可在不到 4 小时内完成。

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