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Transcriptomic data of Clozapine-treated Ngn2-induced Human Excitatory Neurons

机译:氯氮平处理的NGN2诱导的人兴奋性神经元的转录组数据

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摘要

We generated human excitatory neurons using a protocol for rapid 21-day induction using neurogenin-2 overexpression (Zhang et al., 2013) in a publicly available control iPSC line. We validated the glutamatergic neuronal identity of the neurons by immunofluorescence and transcriptomics. We exposed 6 of the 12 replicate neuron cultures to therapeutic plasma levels of clozapine (300 ng/mL) for the last 3 days of culture, and the remaining 6 to replicates to the clozapine solvent alone (methanol) to be used as controls. We harvested the cultures and extracted total RNA, depleted ribosomal RNA and subjected them to RNA sequencing. Of the 6 control replicates 2 failed RNA quality control, and thus a total of 6 exposed and 4 control cultures were used for further analysis. Here, we provide that raw sequencing data as well as a list of all of the genes and their expression levels resulting from the RNA-sequencing. This dataset can be used as a reference data for future studies that access additional neuronal cell types, clozapine exposure conditions, and other antipsychotic medication.
机译:我们使用神经植入素-2过表达(Zhang等人,2013)在公开的控制IPSC线路中使用方案生成人兴奋性神经元。我们通过免疫荧光和转录组织验证了神经元的谷氨酸神经元形象。我们将12个重复的神经元培养物中的6个暴露于培养的最后3天的氯氮平(300ng / ml)的治疗性等离子体水平,并且其余6以单独用作氯氮平溶剂(甲醇)作为对照的重复。我们收获了培养物并提取了总RNA,耗尽的核糖体RNA,并使它们进行RNA测序。在6对照中重复2例,RNA质量控制失败,因此总共6个暴露和4个对照培养物用于进一步分析。这里,我们提供原始测序数据以及由RNA测序引起的所有基因的列表及其表达水平。该数据集可用作参考数据,以用于访问其他神经元细胞类型,氯氮平暴露条件和其他抗精神病药的研究。

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