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RNA 基础设施分析揭示了拥挤空间中的转录组结构。

RNA infrastructure profiling illuminates transcriptome structure in crowded spaces.

作者信息

Xiao Lu, Fang Linglan, Zhong Wenrui, Kool Eric T

机构信息

Department of Chemistry, Stanford University, Stanford, CA 94305, USA.

Department of Chemistry, Stanford University, Stanford, CA 94305, USA; Sarafan ChEM-H Institute, Stanford University, Stanford, CA 94305, USA.

出版信息

Cell Chem Biol. 2024 Dec 19;31(12):2156-2167.e5. doi: 10.1016/j.chembiol.2024.09.009. Epub 2024 Oct 23.

Abstract

RNAs fold into compact structures and undergo protein interactions in cells. These occluded environments can block reagents that probe the underlying RNAs. Probes that can analyze structure in crowded settings can shed light on RNA biology. Here, we employ 2'-OH-reactive probes that are small enough to access folded RNA structure underlying close molecular contacts within cells, providing considerably broader coverage for intracellular RNA structural analysis. The data are analyzed first with well-characterized human ribosomal RNAs and then applied transcriptome-wide to polyadenylated transcripts. The smallest probe acetylimidazole (AcIm) yields 80% greater structural coverage than larger conventional reagent NAIN3, providing enhanced structural information in hundreds of transcripts. The acetyl probe also provides superior signals for identifying mA modification sites in transcripts, particularly in sites that are inaccessible to a standard probe. Our strategy enables profiling RNA infrastructure, enhancing analysis of transcriptome structure, modification, and intracellular interactions, especially in spatially crowded settings.

摘要

RNA在细胞中折叠成紧密结构并与蛋白质相互作用。这些封闭的环境会阻碍探测潜在RNA的试剂。能够在拥挤环境中分析结构的探针可以揭示RNA生物学。在这里,我们使用2'-OH反应性探针,其足够小以进入细胞内紧密分子接触下的折叠RNA结构,为细胞内RNA结构分析提供了更广泛的覆盖范围。首先用特征明确的人类核糖体RNA分析数据,然后将其全转录组应用于多聚腺苷酸化转录本。最小的探针乙酰咪唑(AcIm)比更大的传统试剂NAIN3产生的结构覆盖率高80%,在数百个转录本中提供了增强的结构信息。乙酰探针还为识别转录本中的mA修饰位点提供了优越的信号,特别是在标准探针无法进入的位点。我们的策略能够对RNA基础设施进行分析,加强对转录组结构、修饰和细胞内相互作用的分析,特别是在空间拥挤的环境中。

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