Validation and benchmarking of targeted panel sequencing for cancer genomic profiling

标杆管理 重复性 再现性 微卫星不稳定性 DNA测序 计算生物学 预测值 肿瘤科 医学 生物 内科学 微卫星 遗传学 基因 色谱法 化学 等位基因 营销 业务
作者
Duo Wang,Sizhen Wang,Yuanfeng Zhang,Xiaolei Cheng,Xin Huang,Yanxi Han,Zhaohui Chen,Cong Liu,Jinming Li,Rui Zhang
出处
期刊:American Journal of Clinical Pathology [Oxford University Press]
卷期号:160 (5): 507-523
标识
DOI:10.1093/ajcp/aqad078
摘要

To validate a large next-generation sequencing (NGS) panel for comprehensive genomic profiling and improve patient access to more effective precision oncology treatment strategies.OncoPanScan was designed by targeting 825 cancer-related genes to detect a broad range of genomic alterations. A practical validation strategy was used to evaluate the assay's analytical performance, involving 97 tumor specimens with 25 paired blood specimens, 10 engineered cell lines, and 121 artificial reference DNA samples.Overall, 1107 libraries were prepared and the sequencing failure rate was 0.18%. Across alteration classes, sensitivity ranged from 0.938 to more than 0.999, specificity ranged from 0.889 to more than 0.999, positive predictive value ranged from 0.867 to more than 0.999, repeatability ranged from 0.908 to more than 0.999, and reproducibility ranged from 0.832 to more than 0.999. The limit of detection for variants was established based on variant frequency, while for tumor mutation burden and microsatellite instability, it was based on tumor content, resulting in a minimum requirement of 20% tumor content. Benchmarking variant calls against validated NGS assays revealed that variations in the dry-bench processes were the primary cause of discordances.This study presents a detailed validation framework and empirical recommendations for large panel validation and elucidates the sources of discordant alteration calls by comparing with "gold standard measures."
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