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听觉系统单个细胞中单个mRNA的检测。

Detection of single mRNAs in individual cells of the auditory system.

作者信息

Salehi Pezhman, Nelson Charlie N, Chen Yingying, Lei Debin, Crish Samuel D, Nelson Jovitha, Zuo Hongyan, Bao Jianxin

机构信息

Department of Anatomy and Neurobiology, Translational Research Center, Northeast Ohio Medical University, Rootstown, OH, 44272, USA.

Department of Pharmaceutical Sciences, Northeast Ohio Medical University, Rootstown, OH, 44272, USA.

出版信息

Hear Res. 2018 Sep;367:88-96. doi: 10.1016/j.heares.2018.07.008. Epub 2018 Jul 29.

Abstract

Gene expression analysis is essential for understanding the rich repertoire of cellular functions. With the development of sensitive molecular tools such as single-cell RNA sequencing, extensive gene expression data can be obtained and analyzed from various tissues. Single-molecule fluorescence in situ hybridization (smFISH) has emerged as a powerful complementary tool for single-cell genomics studies because of its ability to map and quantify the spatial distributions of single mRNAs at the subcellular level in their native tissue. Here, we present a detailed method to study the copy numbers and spatial localizations of single mRNAs in the cochlea and inferior colliculus. First, we demonstrate that smFISH can be performed successfully in adult cochlear tissue after decalcification. Second, we show that the smFISH signals can be detected with high specificity. Third, we adapt an automated transcript analysis pipeline to quantify and identify single mRNAs in a cell-specific manner. Lastly, we show that our method can be used to study possible correlations between transcriptional and translational activities of single genes. Thus, we have developed a detailed smFISH protocol that can be used to study the expression of single mRNAs in specific cell types of the peripheral and central auditory systems.

摘要

基因表达分析对于理解丰富多样的细胞功能至关重要。随着诸如单细胞RNA测序等灵敏分子工具的发展,可以从各种组织中获取并分析大量的基因表达数据。单分子荧光原位杂交(smFISH)已成为单细胞基因组学研究的一种强大的补充工具,因为它能够在原生组织的亚细胞水平上绘制和量化单个mRNA的空间分布。在此,我们展示一种详细的方法来研究耳蜗和下丘中单个mRNA的拷贝数和空间定位。首先,我们证明脱钙后的成年耳蜗组织中可以成功进行smFISH。其次,我们表明smFISH信号能够以高特异性被检测到。第三,我们采用一种自动化转录本分析流程以细胞特异性方式对单个mRNA进行量化和鉴定。最后,我们表明我们的方法可用于研究单个基因转录和翻译活性之间的可能相关性。因此,我们开发了一种详细的smFISH方案,可用于研究外周和中枢听觉系统特定细胞类型中单个mRNA的表达。

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