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Novel cell separation method for molecular analysis of neuron-astrocyte co-cultures

机译:用于神经元-星形细胞共培养的分子分析的新型细胞分离方法

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摘要

Over the last decade, the importance of astrocyte-neuron communication in neuronal development and synaptic plasticity has become increasingly clear. Since neuron-astrocyte interactions represent highly dynamic and reciprocal processes, we hypothesized that many astrocyte genes may be regulated as a consequence of their interactions with maturing neurons. In order to identify such neuron-responsive astrocyte genes in vitro, we sought to establish an expedited technique for separation of neurons from co-cultured astrocytes. Our newly established method makes use of cold jet, which exploits different adhesion characteristics of subpopulations of cells (), and is rapid, performed under ice-cold conditions and avoids protease-mediated isolation of astrocytes or time-consuming centrifugation, yielding intact astrocyte mRNA with approximately 90% of neuronal RNA removed. Using this purification method, we executed genome-wide profiling in which RNA derived from astrocyte-only cultures was compared with astrocyte RNA derived from differentiating neuron-astrocyte co-cultures. Data analysis determined that many astrocytic mRNAs and biological processes are regulated by neuronal interaction. Our results validate the cold jet as an efficient method to separate astrocytes from neurons in co-culture, and reveals that neurons induce robust gene-expression changes in co-cultured astrocytes.
机译:在过去的十年中,星形胶质细胞-神经元通讯在神经元发育和突触可塑性中的重要性已变得越来越明显。由于神经元-星形胶质细胞相互作用代表高度动态和相互的过程,我们假设许多星形胶质细胞基因可能由于其与成熟神经元的相互作用而受到调节。为了在体外鉴定这种神经元反应性星形胶质细胞基因,我们试图建立一种从共培养的星形胶质细胞中分离神经元的快速技术。我们新建立的方法利用了冷喷射技术,该技术利用了细胞亚群()的不同粘附特性,并且快速,可在冰冷条件下进行,并且避免了蛋白酶介导的星形胶质细胞分离或费时的离心分离,从而产生了完整的星形胶质细胞mRNA去除了大约90%的神经元RNA。使用这种纯化方法,我们执行了全基因组分析,其中将仅星形胶质细胞培养物的RNA与分化神经元-星形胶质细胞共培养物的星形胶质细胞RNA进行了比较。数据分析确定许多星形细胞的mRNA和生物学过程受神经元相互作用的调节。我们的结果验证了冷喷射是在共培养的星形胶质细胞与神经元分离的有效方法,并揭示了神经元在共培养的星形胶质细胞中诱导强大的基因表达变化。

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