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通过单细胞基因表达谱定义神经外胚层细胞的发育多样化。

Defining developmental diversification of diencephalon neurons through single cell gene expression profiling.

机构信息

Department of Genetics and Genome Sciences, University of Connecticut School of Medicine, 263 Farmington Avenue, Farmington, CT 06030-6403, USA.

Department of Genetics and Genome Sciences, University of Connecticut School of Medicine, 263 Farmington Avenue, Farmington, CT 06030-6403, USA

出版信息

Development. 2019 Apr 1;146(12):dev174284. doi: 10.1242/dev.174284.

DOI:10.1242/dev.174284
PMID:30872278
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6602344/
Abstract

The embryonic diencephalon forms integration centers and relay stations in the forebrain. Anecdotal expression studies suggest that the diencephalon contains multiple developmental compartments and subdivisions. Here, we utilized single cell RNA sequencing to profile transcriptomes of dissociated cells from the diencephalon of E12.5 mouse embryos. We identified the divergence of different progenitors, intermediate progenitors, and emerging neurons. By mapping the identified cell groups to their spatial origins, we characterized the molecular features of cell types and cell states arising from various diencephalic domains. Furthermore, we reconstructed the developmental trajectory of distinct cell lineages, and thereby identified the genetic cascades and gene regulatory networks underlying the progression of the cell cycle, neurogenesis and cellular diversification. The analysis provides new insights into the molecular mechanisms underlying the amplification of intermediate progenitor cells in the thalamus. The single cell-resolved trajectories not only confirm a close relationship between the rostral thalamus and prethalamus, but also uncover an unexpected close relationship between the caudal thalamus, epithalamus and rostral pretectum. Our data provide a useful resource for systematic studies of cell heterogeneity and differentiation kinetics within the diencephalon.

摘要

胚胎神经前脑形成前脑的整合中心和中继站。轶事表达研究表明,神经前脑包含多个发育区室和细分。在这里,我们利用单细胞 RNA 测序对 E12.5 小鼠胚胎神经前脑分离细胞的转录组进行了分析。我们确定了不同祖细胞、中间祖细胞和新兴神经元的分化。通过将鉴定出的细胞群映射到它们的空间起源,我们描述了来自不同神经前脑区域的细胞类型和细胞状态的分子特征。此外,我们重建了不同细胞谱系的发育轨迹,从而确定了细胞周期、神经发生和细胞多样化进展的遗传级联和基因调控网络。该分析为丘脑中间祖细胞扩增的分子机制提供了新的见解。单细胞解析轨迹不仅证实了前脑和丘脑之间的密切关系,而且揭示了丘脑、上丘和前脑之间出人意料的密切关系。我们的数据为神经前脑内部细胞异质性和分化动力学的系统研究提供了有用的资源。