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首页> 外文期刊>Journal of neural transmission >Enrichment of single neurons and defined brain regions from human brain tissue samples for subsequent proteome analysis
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Enrichment of single neurons and defined brain regions from human brain tissue samples for subsequent proteome analysis

机译:从人脑组织样品中富集单个神经元和定义的大脑区域,以进行后续蛋白质组分析

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摘要

Brain function in normal aging and neurological diseases has long been a subject of interest. With current technology, it is possible to go beyond descriptive analyses to characterize brain cell populations at the molecular level. However, the brain comprises over 100 billion highly specialized cells, and it is a challenge to discriminate different cell groups for analyses. Isolating intact neurons is not feasible with traditional methods, such as tissue homogenization techniques. The advent of laser microdissection techniques promises to overcome previous limitations in the isolation of specific cells. Here, we provide a detailed protocol for isolating and analyzing neurons from postmortem human brain tissue samples. We describe a workflow for successfully freezing, sectioning and staining tissue for laser microdissection. This protocol was validated by mass spectrometric analysis. Isolated neurons can also be employed for western blotting or PCR. This protocol will enable further examinations of brain cell-specific molecular pathways and aid in elucidating distinct brain functions.
机译:长期以来,正常衰老和神经系统疾病中的脑功能一直是人们关注的主题。使用当前的技术,有可能超越描述性分析来在分子水平上表征脑细胞种群。但是,大脑包含超过1000亿个高度专门化的细胞,因此区分不同的细胞组进行分析是一项挑战。使用传统方法(例如组织均质化技术)来隔离完整的神经元是不可行的。激光显微解剖技术的出现有望克服以前在分离特定细胞方面的局限性。在这里,我们提供了用于从死后人脑组织样本中分离和分析神经元的详细协议。我们描述了成功冷冻,切片和染色组织以进行激光显微切割的工作流程。该方案已通过质谱分析验证。分离的神经元也可以用于蛋白质印迹或PCR。该协议将使大脑细胞特异性分子途径的进一步检查成为可能,并有助于阐明不同的大脑功能。

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