通过激光捕获显微切割从冷冻人脑组织中分离出的神经元和星形胶质细胞的基因表达分析
Gene Expression Analysis of Neurons and Astrocytes Isolated by Laser Capture Microdissection from Frozen Human Brain Tissues.
作者信息
Tagliafierro Lidia, Bonawitz Kirsten, Glenn Omolara C, Chiba-Falek Ornit
机构信息
Department of Neurology, Duke University Medical CenterDurham, NC, USA; Center for Genomic and Computational Biology, Duke University Medical CenterDurham, NC, USA.
出版信息
Front Mol Neurosci. 2016 Aug 18;9:72. doi: 10.3389/fnmol.2016.00072. eCollection 2016.
Different cell types and multiple cellular connections characterize the human brain. Gene expression analysis using a specific population of cells is more accurate than conducting analysis of the whole tissue homogenate, particularly in the context of neurodegenerative diseases, where a specific subset of cells is affected by the different pathology. Due to the difficulty of obtaining homogenous cell populations, gene expression in specific cell-types (neurons, astrocytes, etc.) has been understudied. To leverage the use of archive resources of frozen human brains in studies of neurodegenerative diseases, we developed and calibrated a method to quantify cell-type specific-neuronal, astrocytes-expression profiles of genes implicated in neurodegenerative diseases, including Parkinson's and Alzheimer's diseases. Archive human frozen brain tissues were used to prepare slides for rapid immunostaining using cell-specific antibodies. The immunoreactive-cells were isolated by Laser Capture Microdissection (LCM). The enrichment for a particular cell-type of interest was validated in post-analysis stage by the expression of cell-specific markers. We optimized the technique to preserve the RNA integrity, so that the RNA was suitable for downstream expression analyses. Following RNA extraction, the expression levels were determined digitally using nCounter Single Cell Gene Expression assay (NanoString Technologies®). The results demonstrated that using our optimized technique we successfully isolated single neurons and astrocytes from human frozen brain tissues and obtained RNA of a good quality that was suitable for mRNA expression analysis. We present here new advancements compared to previous reported methods, which improve the method's feasibility and its applicability for a variety of downstream molecular analyses. Our new developed method can be implemented in genetic and functional genomic research of neurodegenerative diseases and has the potential to significantly advance the field.
不同的细胞类型和多种细胞连接是人类大脑的特征。使用特定细胞群体进行基因表达分析比分析整个组织匀浆更准确,特别是在神经退行性疾病的背景下,其中特定的细胞亚群受到不同病理的影响。由于难以获得同质的细胞群体,特定细胞类型(神经元、星形胶质细胞等)中的基因表达研究不足。为了在神经退行性疾病研究中利用冷冻人脑的存档资源,我们开发并校准了一种方法,用于量化与神经退行性疾病(包括帕金森病和阿尔茨海默病)相关的基因的细胞类型特异性神经元、星形胶质细胞表达谱。使用存档的人类冷冻脑组织制备玻片,以便使用细胞特异性抗体进行快速免疫染色。通过激光捕获显微切割(LCM)分离免疫反应性细胞。在分析后阶段,通过细胞特异性标志物的表达验证了感兴趣的特定细胞类型的富集情况。我们优化了该技术以保持RNA完整性,使RNA适合下游表达分析。RNA提取后,使用nCounter单细胞基因表达测定法(NanoString Technologies®)以数字方式确定表达水平。结果表明,使用我们优化的技术,我们成功地从人类冷冻脑组织中分离出单个神经元和星形胶质细胞,并获得了适合mRNA表达分析的高质量RNA。与先前报道的方法相比,我们在此展示了新的进展,这些进展提高了该方法的可行性及其对各种下游分子分析的适用性。我们新开发的方法可用于神经退行性疾病的遗传和功能基因组研究,并有可能显著推动该领域的发展。
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