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膜片钳记录和钙成像技术,随后进行单细胞PCR,揭示了诱导多能干细胞衍生的人类神经元中13个基因的发育情况。

Patch-clamp recordings and calcium imaging followed by single-cell PCR reveal the developmental profile of 13 genes in iPSC-derived human neurons.

作者信息

Belinsky Glenn S, Rich Matthew T, Sirois Carissa L, Short Shaina M, Pedrosa Erika, Lachman Herbert M, Antic Srdjan D

机构信息

Department of Neuroscience, University of Connecticut Health Center, Farmington, CT, USA.

Department of Psychiatry and Behavioral Sciences, Albert Einstein College of Medicine, Bronx, New York, USA.

出版信息

Stem Cell Res. 2014 Jan;12(1):101-18. doi: 10.1016/j.scr.2013.09.014. Epub 2013 Oct 3.

Abstract

Molecular genetic studies are typically performed on homogenized biological samples, resulting in contamination from non-neuronal cells. To improve expression profiling of neurons we combined patch recordings with single-cell PCR. Two iPSC lines (healthy subject and 22q11.2 deletion) were differentiated into neurons. Patch electrode recordings were performed on 229 human cells from Day-13 to Day-88, followed by capture and single-cell PCR for 13 genes: ACTB, HPRT, vGLUT1, βTUBIII, COMT, DISC1, GAD1, PAX6, DTNBP1, ERBB4, FOXP1, FOXP2, and GIRK2. Neurons derived from both iPSC lines expressed βTUBIII, fired action potentials, and experienced spontaneous depolarizations (UP states) ~2 weeks before vGLUT1, GAD1 and GIRK2 appeared. Multisite calcium imaging revealed that these UP states were not synchronized among hESC-H9-derived neurons. The expression of FOXP1, FOXP2 and vGLUT1 was lost after 50 days in culture, in contrast to other continuously expressed genes. When gene expression was combined with electrophysiology, two subsets of genes were apparent; those irrelevant to spontaneous depolarizations (including vGLUT1, GIRK2, FOXP2 and DISC1) and those associated with spontaneous depolarizations (GAD1 and ERBB4). The results demonstrate that in the earliest stages of neuron development, it is useful to combine genetic analysis with physiological characterizations, on a cell-to-cell basis.

摘要

分子遗传学研究通常在匀浆的生物样本上进行,这会导致非神经元细胞的污染。为了改善神经元的表达谱分析,我们将膜片钳记录与单细胞PCR相结合。将两个诱导多能干细胞系(健康受试者和22q11.2缺失)分化为神经元。在第13天至第88天对229个人类细胞进行膜片电极记录,随后捕获并对13个基因进行单细胞PCR:ACTB、HPRT、vGLUT1、βTUBIII、COMT、DISC1、GAD1、PAX6、DTNBP1、ERBB4、FOXP1、FOXP2和GIRK2。来自两个诱导多能干细胞系的神经元均表达βTUBIII,产生动作电位,并在vGLUT1、GAD1和GIRK2出现前约2周经历自发去极化(UP状态)。多部位钙成像显示,这些UP状态在人胚胎干细胞H9来源的神经元中不同步。与其他持续表达的基因相比,培养50天后FOXP1、FOXP2和vGLUT1的表达消失。当基因表达与电生理学相结合时,明显有两个基因子集;那些与自发去极化无关的基因(包括vGLUT1、GIRK2、FOXP2和DISC1)以及那些与自发去极化相关的基因(GAD1和ERBB4)。结果表明,在神经元发育的最早阶段,在单细胞基础上结合遗传分析与生理特征分析是有用的。

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