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流式细胞术分选中枢神经系统组织中的神经元和神经胶质细胞核。

Flow cytometric sorting of neuronal and glial nuclei from central nervous system tissue.

机构信息

Superstar Program Stem Cell Unit, Graduate School of Medical Sciences, Kyushu University, Higashi-ku, Fukuoka, Japan.

出版信息

J Cell Physiol. 2011 Feb;226(2):552-8. doi: 10.1002/jcp.22365.

DOI:10.1002/jcp.22365
PMID:20717962
Abstract

Due to the complex cellular heterogeneity of the central nervous system (CNS), it is relatively difficult to reliably obtain molecular descriptions with cell-type specificity. In particular, comparative analysis of epigenetic regulation or molecular profiles is hampered by the lack of adequate methodology for selective purification of defined cell populations from CNS tissue. Here, we developed a direct purification strategy of neural nuclei from CNS tissue based on fluorescence-activated cell sorting (FACS). We successfully fractionated nuclei from complex tissues such as brain, spinal cord, liver, kidney, and skeletal muscle extruded mechanically or chemically, and fractionated nuclei were structurally maintained and contained nucleoproteins and nuclear DNA/RNA. We collected sufficient numbers of nuclei from neurons and oligodendrocytes using FACS with immunolabeling for nucleoproteins or from genetically labeled transgenic mice. In addition, the use of Fab fragments isolated from papain antibody digests, which effectively enriched the specialized cell populations, significantly enhanced the immunolabeling efficacy. This methodology can be applied to a wide variety of heterogeneous tissues and is crucial for understanding the cell-specific information about chromatin dynamics, nucleoproteins, protein-DNA/RNA interactions, and transcriptomes retained in the nucleus, such as non-coding RNAs.

摘要

由于中枢神经系统 (CNS) 的细胞异质性复杂,因此很难可靠地获得具有细胞类型特异性的分子描述。特别是,由于缺乏从 CNS 组织中选择性纯化特定细胞群体的适当方法,因此对表观遗传调控或分子谱的比较分析受到阻碍。在这里,我们基于荧光激活细胞分选 (FACS) 开发了一种从 CNS 组织中直接纯化神经核的策略。我们成功地从机械或化学挤压的脑、脊髓、肝、肾和骨骼肌等复杂组织中分离出核,分离出的核结构保持完整,并含有核蛋白和核 DNA/RNA。我们使用针对核蛋白的免疫标记或从遗传标记的转基因小鼠通过 FACS 收集了足够数量的神经元和少突胶质细胞核。此外,使用木瓜蛋白酶抗体消化物分离的 Fab 片段的使用有效地富集了特化细胞群体,显著提高了免疫标记效率。该方法适用于各种异质组织,对于了解保留在核中的染色质动力学、核蛋白、蛋白质-DNA/RNA 相互作用和转录组(如非编码 RNA)的特定于细胞的信息至关重要。

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