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Complete deconvolution of cellular mixtures based on linearity of transcriptional signatures

机译:基于转录信号线性的细胞混合物完全去卷积

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摘要

Changes in bulk transcriptional profiles of heterogeneous samples often reflect changes in proportions of individual cell types. Several robust techniques have been developed to dissect the composition of such mixed samples given transcriptional signatures of the pure components or their proportions. These approaches are insufficient, however, in situations when no information about individual mixture components is available. This problem is known as the  complete deconvolution problem, where the composition is revealed without any a priori knowledge about cell types and their proportions. Here, we identify a previously unrecognized property of tissue-specific genes – their mutual linearity – and use it to reveal the structure of the topological space of mixed transcriptional profiles and provide a noise-robust approach to the complete deconvolution problem. Furthermore, our analysis reveals systematic bias of all deconvolution techniques due to differences in cell size or RNA-content, and we demonstrate how to address this bias at the experimental design level.
机译:异质样品的整体转录谱的变化通常反映单个细胞类型比例的变化。已经开发了几种鲁棒的技术,以给出纯组分或其比例的转录特征来剖析这种混合样品的组成。但是,在没有有关单个混合物成分的信息的情况下,这些方法是不够的。这个问题被称为完全解卷积问题,其中在没有任何关于细胞类型及其比例的先验知识的情况下揭示了成分。在这里,我们确定了组织特异性基因以前无法识别的特性-它们的相互线性-并使用它揭示了混合转录谱的拓扑空间结构,并为完整的解卷积问题提供了一种鲁棒的方法。此外,我们的分析揭示了由于细胞大小或RNA含量差异而导致的所有反卷积技术的系统性偏差,并且我们展示了如何在实验设计水平上解决这种偏差。

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