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从新生大鼠脑和视神经中获取的少突胶质细胞系细胞的分离、扩增及成熟

Isolation, Expansion, and Maturation of Oligodendrocyte Lineage Cells Obtained from Rat Neonatal Brain and Optic Nerve.

作者信息

Sánchez-Gómez Maria Victoria, Serrano Mari Paz, Alberdi Elena, Pérez-Cerdá Fernando, Matute Carlos

机构信息

Departamento de Neurociencias, Achucarro Basque Center for Neuroscience, CIBERNED, Universidad del País Vasco (UPV/EHU), Leioa, Spain.

出版信息

Methods Mol Biol. 2018;1791:95-113. doi: 10.1007/978-1-4939-7862-5_8.

DOI:10.1007/978-1-4939-7862-5_8
PMID:30006704
Abstract

Oligodendrocytes are the myelin-forming cells in the central nervous system (CNS) and their loss or dysfunction is a hallmark of CNS demyelinating diseases, such as multiple sclerosis (MS), hypoxic-ischemic demyelination, or spinal cord injury. In the rodent CNS, oligodendrocyte progenitor cells (OPCs) arise in multiple ventral and dorsal locations of the forebrain during late embryogenesis and early postnatal periods. OPCs migrate out from these germinal zones and disperse throughout the CNS, to populate the developing white and gray matter. There, OPCs can begin to mature through a series of intermediate states characterized by the expression of stage-specific proteins until completely differentiated into postmitotic myelinating oligodendrocytes. Elucidating the cellular and molecular mechanisms that control oligodendrocyte maturation requires isolating OPCs and premyelinating oligodendrocytes by rapid and reliable methods that provide high yield, pure and viable culture, being a powerful tool to characterize their differentiation and potential capacity for myelin repair after injury. This chapter describes in detail two simple and efficient protocols for the preparation of highly enriched rat OPC populations and immature oligodendrocytes derived from mixed glial cultures and optic nerves, respectively. Functional oligodendrocytes obtained with these protocols can be cocultured with primary neurons to study myelination.

摘要

少突胶质细胞是中枢神经系统(CNS)中形成髓鞘的细胞,其丢失或功能障碍是中枢神经系统脱髓鞘疾病的标志,如多发性硬化症(MS)、缺氧缺血性脱髓鞘或脊髓损伤。在啮齿动物的中枢神经系统中,少突胶质前体细胞(OPC)在胚胎后期和出生后早期在前脑的多个腹侧和背侧位置产生。OPC从这些生发区迁移出来并散布于整个中枢神经系统,以填充发育中的白质和灰质。在那里,OPC可以通过一系列以阶段特异性蛋白表达为特征的中间状态开始成熟,直到完全分化为有丝分裂后形成髓鞘的少突胶质细胞。阐明控制少突胶质细胞成熟的细胞和分子机制需要通过快速可靠的方法分离OPC和前髓鞘形成少突胶质细胞,这些方法要能提供高产量、纯净且有活力的培养物,这是表征它们分化以及损伤后髓鞘修复潜在能力的有力工具。本章详细描述了两种简单有效的方案,分别用于制备源自混合胶质细胞培养物和视神经的高度富集的大鼠OPC群体和未成熟少突胶质细胞。用这些方案获得的功能性少突胶质细胞可以与原代神经元共培养以研究髓鞘形成。

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