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通过免疫淘选从啮齿动物大脑中纯化内皮细胞。

Purification of endothelial cells from rodent brain by immunopanning.

作者信息

Zhou Lu, Sohet Fabien, Daneman Richard

机构信息

Department of Neurobiology, Stanford University School of Medicine, Stanford, California 94305-5125;

出版信息

Cold Spring Harb Protoc. 2014 Jan 1;2014(1):65-77. doi: 10.1101/pdb.prot074963.

Abstract

This protocol describes the use of immunopanning to purify endothelial cells from the rodent brain. Immunopanning permits the prospective isolation of endothelial cells from nervous tissue by relying on the binding of the endothelial cells to an anti-CD31 antibody adhered to a Petri dish. The cells are viable at the end of this gentle procedure, and they can be analyzed acutely for gene expression or cultured alone or in coculture with other central nervous system (CNS) cell types, including CNS pericytes and CNS astrocytes. This procedure can be used to isolate endothelial cells from either rat or mouse. We have suggested specific antibodies that work for each species. Note that endothelial cells from rats and mice have different morphologies; in general, rat CNS endothelial cells are longer and thinner than mouse CNS endothelial cells. This procedure can also be used to purify endothelial cells from different regions of the CNS, including brain and optic nerve. Dissociation procedures must be optimized for each tissue.

摘要

本方案描述了使用免疫淘选法从啮齿动物大脑中纯化内皮细胞的方法。免疫淘选法通过依赖内皮细胞与粘附在培养皿上的抗CD31抗体的结合,实现从神经组织中前瞻性地分离内皮细胞。在这个温和的操作结束时,细胞仍保持活力,可对其进行急性基因表达分析,或单独培养,或与其他中枢神经系统(CNS)细胞类型(包括CNS周细胞和CNS星形胶质细胞)共培养。此方法可用于从大鼠或小鼠中分离内皮细胞。我们推荐了适用于每个物种的特异性抗体。请注意,大鼠和小鼠的内皮细胞形态不同;一般来说,大鼠CNS内皮细胞比小鼠CNS内皮细胞更长更细。此方法也可用于从CNS的不同区域(包括脑和视神经)纯化内皮细胞。必须针对每个组织优化解离程序。

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