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首页> 外文期刊>Journal of Neuroscience Methods >A new method to isolate microglia from adult mice and culture them for an extended period of time.
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A new method to isolate microglia from adult mice and culture them for an extended period of time.

机译:从成年小鼠中分离小胶质细胞并进行长时间培养的新方法。

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摘要

As the major immuno-competent cells of the brain, microglia are highly implicated in neuro-protection as well as in neurodegeneration. Therefore, they are of key interest for research on numerous CNS diseases. Currently, to model inflammation in the brain, microglial cell lines or primary microglia prepared from embryonic or neo-natal rodents are widely used. However, these in vitro microglial models are not suitable for research in the field of neuro-degenerative diseases where aging is a crucial parameter. Only a few in vitro studies on aged microglia have been published so far, most of which use ex vivo microglia which cannot be kept in culture for prolonged periods of time. In the present study, we provide a new approach which allows the isolation and culture of an almost pure population of microglia from adult mouse brains. The isolation is based on a procedure which combines density separation and a subsequent culture selection process. After these steps, microglia form a non-adherent floating cell layer that can be easily and repeatedly harvested and replated. This method is simple and allows for a comparatively high yield and purity of adult microglial cells. The collected primary adult microglia proliferate and can be kept in culture for extended periods of time. We compared the primary adult microglia to primary microglia from neo-natal mice as well as to the C8-B4 microglial cell line. We found that adult microglia have similar, but not identical, immuno-phenotypic, functional and electrophysiological characteristics to the other in vitro models.
机译:小胶质细胞是大脑的主要免疫功能细胞,与神经保护和神经变性高度相关。因此,它们是研究多种中枢神经系统疾病的关键兴趣。当前,为了模拟大脑中的炎症,从胚胎或新生啮齿动物制备的小胶质细胞系或原发性小胶质细胞被广泛使用。但是,这些体外小胶质细胞模型不适用于以衰老为关键参数的神经退行性疾病领域的研究。迄今为止,仅发表了几篇关于老年小胶质细胞的体外研究,其中大多数使用离体小胶质细胞,无法长期培养。在本研究中,我们提供了一种新方法,该方法可以从成年小鼠脑中分离和培养几乎纯净的小胶质细胞。分离基于结合了密度分离和随后的培养物选择过程的程序。在这些步骤之后,小胶质细胞形成了一个非粘附性的漂浮细胞层,可以很容易地重复收获并重新铺贴。这种方法很简单,可以使成年的小胶质细胞获得较高的产量和纯度。收集的原发性成年小胶质细胞增生,可以长时间培养。我们比较了成年小胶质细胞与新生小鼠的小胶质细胞以及C8-B4小胶质细胞系。我们发现成人小胶质细胞具有与其他体外模型相似但不相同的免疫表型,功能和电生理特性。

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