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量化突变检测对肿瘤亚克隆重建的影响。

Quantifying the influence of mutation detection on tumour subclonal reconstruction.

机构信息

Department of Medical Biophysics, University of Toronto, Toronto, ON, M5G 1L7, Canada.

Princess Margaret Cancer Centre, University Health Network, Toronto, ON, M5G 2C1, Canada.

出版信息

Nat Commun. 2020 Dec 7;11(1):6247. doi: 10.1038/s41467-020-20055-w.

Abstract

Whole-genome sequencing can be used to estimate subclonal populations in tumours and this intra-tumoural heterogeneity is linked to clinical outcomes. Many algorithms have been developed for subclonal reconstruction, but their variabilities and consistencies are largely unknown. We evaluate sixteen pipelines for reconstructing the evolutionary histories of 293 localized prostate cancers from single samples, and eighteen pipelines for the reconstruction of 10 tumours with multi-region sampling. We show that predictions of subclonal architecture and timing of somatic mutations vary extensively across pipelines. Pipelines show consistent types of biases, with those incorporating SomaticSniper and Battenberg preferentially predicting homogenous cancer cell populations and those using MuTect tending to predict multiple populations of cancer cells. Subclonal reconstructions using multi-region sampling confirm that single-sample reconstructions systematically underestimate intra-tumoural heterogeneity, predicting on average fewer than half of the cancer cell populations identified by multi-region sequencing. Overall, these biases suggest caution in interpreting specific architectures and subclonal variants.

摘要

全基因组测序可用于估计肿瘤中的亚克隆群体,肿瘤内异质性与临床结局相关。已经开发了许多用于亚克隆重建的算法,但它们的可变性和一致性在很大程度上尚不清楚。我们评估了 16 种用于从单个样本重建 293 例局部前列腺癌进化史的管道,以及 18 种用于重建 10 例多区域采样肿瘤的管道。我们表明,亚克隆结构和体细胞突变时间的预测在管道之间存在广泛差异。管道显示出一致的偏差类型,那些包含 SomaticSniper 和 Battenberg 的管道优先预测同质的癌细胞群体,而那些使用 MuTect 的管道倾向于预测多个癌细胞群体。使用多区域采样的亚克隆重建证实,单样本重建系统地低估了肿瘤内异质性,平均预测的癌细胞群体数量不到多区域测序确定的一半。总的来说,这些偏差表明在解释特定的结构和亚克隆变体时需要谨慎。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8a3f/7721877/3052d6f2a663/41467_2020_20055_Fig1_HTML.jpg

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