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体外和体内神经干细胞增殖的评估。

Evaluation of proliferation of neural stem cells in vitro and in vivo.

作者信息

Morte Maria Inês, Carreira Bruno P, Machado Vanessa, Carmo Anália, Nunes-Correia Isabel, Carvalho Caetana M, Araújo Inês M

机构信息

Centre for Neuroscience and Cell Biology, University of Coimbra, Coimbra, Portugal.

出版信息

Curr Protoc Stem Cell Biol. 2013;Chapter 2:Unit 2D.14. doi: 10.1002/9780470151808.sc02d14s24.

DOI:10.1002/9780470151808.sc02d14s24
PMID:23404673
Abstract

This unit describes two basic protocols for the detection of the proliferation of neural stem cells (NSC). The first one addresses cell proliferation in cultures, starting with primary cell cultures isolated from the mouse subventricular zone (SVZ), in which SVZ-derived NSC are kept in culture as neurospheres. By using this culture system, we are able to study different stages of adult neurogenesis, such as proliferation, differentiation, migration, and survival. Thus, in the first basic protocol, we describe two different techniques to evaluate cell proliferation based on EdU incorporation: (a) immunocytochemistry and (b) flow cytometry. EdU, a new thymidine analog, which is detected by a reproducible and sensitive method based on click chemistry, does not require DNA denaturation, as is the case with BrdU. Thus, co-labeling of EdU with other specific antibodies of extracellular or intracellular targets, as well as other DNA dyes, is possible. In the second basic protocol, we describe an in vivo assay to evaluate proliferation of NSC in the dentate gyrus of hippocampus of adult mice, by both BrdU and EdU detection. With this approach, it is also possible to study different stages of adult neurogenesis, by co-labeling thymidine analogs with other specific markers, such as doublecortin (DCX) or neuronal nuclei protein (NeuN).

摘要

本单元描述了检测神经干细胞(NSC)增殖的两种基本方案。第一种方案针对培养物中的细胞增殖,从分离自小鼠脑室下区(SVZ)的原代细胞培养物开始,其中源自SVZ的NSC作为神经球保存在培养物中。通过使用这种培养系统,我们能够研究成体神经发生的不同阶段,如增殖、分化、迁移和存活。因此,在第一个基本方案中,我们描述了基于EdU掺入评估细胞增殖的两种不同技术:(a)免疫细胞化学和(b)流式细胞术。EdU是一种新的胸苷类似物,通过基于点击化学的可重复且灵敏的方法进行检测,不像BrdU那样需要DNA变性。因此,EdU可以与细胞外或细胞内靶点的其他特异性抗体以及其他DNA染料进行共标记。在第二个基本方案中,我们描述了一种体内试验,通过检测BrdU和EdU来评估成年小鼠海马齿状回中NSC的增殖。通过这种方法,通过将胸苷类似物与其他特异性标记物(如双皮质素(DCX)或神经元核蛋白(NeuN))进行共标记,也有可能研究成体神经发生的不同阶段。

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