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使用 MethSCAn 分析单细胞 bisulfite 测序数据。

Analyzing single-cell bisulfite sequencing data with MethSCAn.

机构信息

BioQuant Centre, University of Heidelberg, Heidelberg, Germany.

Division of Molecular Neurobiology, German Cancer Research Center, Heidelberg, Germany.

出版信息

Nat Methods. 2024 Sep;21(9):1616-1623. doi: 10.1038/s41592-024-02347-x. Epub 2024 Jul 31.

Abstract

Single-cell bisulfite sequencing (scBS) is a technique that enables the assessment of DNA methylation at single-base pair and single-cell resolution. The analysis of large datasets obtained from scBS requires preprocessing to reduce the data size, improve the signal-to-noise ratio and provide interpretability. Typically, this is achieved by dividing the genome into large tiles and averaging the methylation signals within each tile. Here we demonstrate that this coarse-graining approach can lead to signal dilution. We propose improved strategies to identify more informative regions for methylation quantification and a more accurate quantitation method than simple averaging. Our approach enables better discrimination of cell types and other features of interest and reduces the need for large numbers of cells. We also present an approach to detect differentially methylated regions between groups of cells and demonstrate its ability to identify biologically meaningful regions that are associated with genes involved in the core functions of specific cell types. Finally, we present the software tool MethSCAn for scBS data analysis ( https://anders-biostat.github.io/MethSCAn ).

摘要

单细胞亚硫酸氢盐测序(scBS)是一种能够评估单碱基对和单细胞分辨率下 DNA 甲基化的技术。分析从 scBS 获得的大型数据集需要预处理来减小数据量、提高信噪比并提供可解释性。通常,这是通过将基因组划分为大片段并平均每个片段内的甲基化信号来实现的。在这里,我们证明了这种粗粒度方法可能导致信号稀释。我们提出了改进的策略来识别更具信息量的甲基化定量区域,并提出了比简单平均更准确的定量方法。我们的方法能够更好地区分细胞类型和其他感兴趣的特征,并减少对大量细胞的需求。我们还提出了一种用于检测细胞群之间差异甲基化区域的方法,并证明其能够识别与特定细胞类型核心功能相关的基因的生物学有意义的区域。最后,我们介绍了用于 scBS 数据分析的软件工具 MethSCAn(https://anders-biostat.github.io/MethSCAn)。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2a80/11399085/1c00183843da/41592_2024_2347_Fig1_HTML.jpg

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