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DC3 is a method for deconvolution and coupled clustering from bulk and single-cell genomics data

机译:DC3是从散装和单细胞基因组学数据进行解卷积和耦合聚类的方法

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Characterizing and interpreting heterogeneous mixtures at the cellular level is a critical problem in genomics. Single-cell assays offer an opportunity to resolve cellular level heterogeneity, e.g., scRNA-seq enables single-cell expression profiling, and scATAC-seq identifies active regulatory elements. Furthermore, while scHi-C can measure the chromatin contacts (i.e., loops) between active regulatory elements to target genes in single cells, bulk HiChIP can measure such contacts in a higher resolution. In this work, we introduce DC3 (De-Convolution and Coupled-Clustering) as a method for the joint analysis of various bulk and single-cell data such as HiChIP, RNA-seq and ATAC-seq from the same heterogeneous cell population. DC3 can simultaneously identify distinct subpopulations, assign single cells to the subpopulations (i.e., clustering) and de-convolve the bulk data into subpopulation-specific data. The subpopulation-specific profiles of gene expression, chromatin accessibility and enhancer-promoter contact obtained by DC3 provide a comprehensive characterization of the gene regulatory system in each subpopulation.
机译:在细胞水平下表征和解释异质混合物是基因组学中的关键问题。单细胞测定提供了解决细胞水平异质性的机会,例如,ScrNA-SEQ能够进行单细胞表达分析,并且Scatac-SEQ识别有源调节元件。此外,而Schi-C可以测量在单细胞中的活性调节元件至靶基因之间的染色蛋白触点(即,环)之间,散装HICHIP可以以更高的分辨率测量这种接触。在这项工作中,我们将DC3(去卷积和耦合聚类)介绍作为与同一异质细胞群相同的异质细胞群的各种散装和单细胞数据的联合分析各种散装和单细胞数据的方法。 DC3可以同时识别不同的子步骤,将单个小区分配给子步骤(即,群集)并将批量数据De-Truplve归档为特定于群数据。通过DC3获得的基因表达,染色质表达和增强剂 - 启动子接触的特异性特异性谱提供了每个亚群中基因调节系统的综合表征。

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