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Development and validation of a clinical cancer genomic profiling test based on massively parallel DNA sequencing

机译:基于大规模并行DNA测序的临床癌症基因组谱分析测试的开发和验证

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As more clinically relevant cancer genes are identified, comprehensive diagnostic approaches are needed to match patients to therapies, raising the challenge of optimization and analytical validation of assays that interrogate millions of bases of cancer genomes altered by multiple mechanisms. Here we describe a test based on massively parallel DNA sequencing to characterize base substitutions, short insertions and deletions (indels), copy number alterations and selected fusions across 287 cancer-related genes from routine formalin-fixed and paraffin-embedded (FFPE) clinical specimens. We implemented a practical validation strategy with reference samples of pooled cell lines that model key determinants of accuracy, including mutant allele frequency,indel length and amplitude of copy change. Test sensitivity achieved was 95-99% across alteration types, with high specificity (positive predictive value >99%). We confirmed accuracy using 249 FFPE cancer specimens characterized by established assays. Application of the test to 2,221 clinical cases revealed clinically actionable alterations in 76% of tumors, three times the number of actionable alterations detected by current diagnostic tests.
机译:随着更多临床相关癌症基因的鉴定,需要综合的诊断方法来使患者与治疗相匹配,从而提出了对优化和分析验证方法的挑战,这些方法可查询由多种机制改变的数百万个癌症基因组碱基。在这里,我们描述了一种基于大规模并行DNA测序的测试,用于表征常规福尔马林固定和石蜡包埋(FFPE)临床标本中287个与癌症相关的基因的碱基取代,短插入和缺失(indels),拷贝数变化和选择的融合。我们对合并细胞系的参考样品实施了实用的验证策略,该模型对准确性的关键决定因素建模,包括突变体等位基因频率,插入缺失长度和拷贝变化幅度。各种变异类型的测试灵敏度为95-99%,具有高特异性(阳性预测值> 99%)。我们使用已建立的检测方法表征的249个FFPE癌症样本确认了准确性。该测试在2,221例临床病例中的应用表明,在76%的肿瘤中,临床上可行的变化是当前诊断测试中检测到的可行变化的三倍。

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