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使用空间转录组学和 mRNA 空间定位对交感神经系统进行细胞类型分析。

Cell-type profiling of the sympathetic nervous system using spatial transcriptomics and spatial mapping of mRNA.

机构信息

Stowers Institute for Medical Research, Kansas City, Missouri, USA.

Children's Mercy Hospital, Kansas City, Missouri, USA.

出版信息

Dev Dyn. 2023 Aug;252(8):1130-1142. doi: 10.1002/dvdy.577. Epub 2023 Mar 9.

Abstract

BACKGROUND

The molecular identification of neural progenitor cell populations that connect to establish the sympathetic nervous system (SNS) remains unclear. This is due to technical limitations in the acquisition and spatial mapping of molecular information to tissue architecture.

RESULTS

To address this, we applied Slide-seq spatial transcriptomics to intact fresh frozen chick trunk tissue transversely cryo-sectioned at the developmental stage prior to SNS formation. In parallel, we performed age- and location-matched single cell (sc) RNA-seq and 10× Genomics Visium to inform our analysis. Downstream bioinformatic analyses led to the unique molecular identification of neural progenitor cells within the peripheral sympathetic ganglia (SG) and spinal cord preganglionic neurons (PGNs). We then successfully applied the HiPlex RNAscope fluorescence in situ hybridization and multispectral confocal microscopy to visualize 12 gene targets in stage-, age- and location-matched chick trunk tissue sections.

CONCLUSIONS

Together, these data demonstrate a robust strategy to acquire and integrate single cell and spatial transcriptomic information, resulting in improved resolution of molecular heterogeneities in complex neural tissue architectures. Successful application of this strategy to the developing SNS provides a roadmap for functional studies of neural connectivity and platform to address complex questions in neural development and regeneration.

摘要

背景

连接建立交感神经系统(SNS)的神经祖细胞群体的分子鉴定仍不清楚。这是由于在获取和将分子信息空间映射到组织架构方面存在技术限制。

结果

为了解决这个问题,我们应用 Slide-seq 空间转录组学对在 SNS 形成之前的发育阶段的新鲜冷冻鸡躯干组织进行横向冷冻切片。平行地,我们进行了年龄和位置匹配的单细胞(sc)RNA-seq 和 10× Genomics Visium 以告知我们的分析。下游生物信息学分析导致在外周交感神经节(SG)和脊髓节前神经元(PGN)内独特的神经祖细胞的分子鉴定。然后,我们成功地将 HiPlex RNAscope 荧光原位杂交和多光谱共聚焦显微镜应用于在阶段、年龄和位置匹配的鸡躯干组织切片中可视化 12 个基因靶标。

结论

这些数据共同证明了一种获取和整合单细胞和空间转录组学信息的强大策略,从而提高了复杂神经组织架构中分子异质性的分辨率。该策略在发育中的 SNS 中的成功应用为神经连接的功能研究提供了路线图,并为解决神经发育和再生中的复杂问题提供了平台。

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