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Quantitative Identification of Mutant Alleles Derived from Lung Cancer in Plasma Cell-Free DNA via Anomaly Detection Using Deep Sequencing Data

机译:使用深度测序数据通过异常检测定量鉴定血浆中无细胞DNA中肺癌衍生的突变等位基因

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摘要

The detection of rare mutants using next generation sequencing has considerable potential for diagnostic applications. Detecting circulating tumor DNA is the foremost application of this approach. The major obstacle to its use is the high read error rate of next-generation sequencers. Rather than increasing the accuracy of final sequences, we detected rare mutations using a semiconductor sequencer and a set of anomaly detection criteria based on a statistical model of the read error rate at each error position. Statistical models were deduced from sequence data from normal samples. We detected epidermal growth factor receptor (EGFR) mutations in the plasma DNA of lung cancer patients. Single-pass deep sequencing (>100,000 reads) was able to detect one activating mutant allele in 10,000 normal alleles. We confirmed the method using 22 prospective and 155 retrospective samples, mostly consisting of DNA purified from plasma. A temporal analysis suggested potential applications for disease management and for therapeutic decision making to select epidermal growth factor receptor tyrosine kinase inhibitors (EGFR-TKI).
机译:使用下一代测序技术检测稀有突变体具有很大的诊断应用潜力。检测循环肿瘤DNA是该方法的最主要应用。使用它的主要障碍是下一代定序器的高读取错误率。我们没有提高最终序列的准确性,而是使用半导体定序器和一组基于每个错误位置处读取错误率的统计模型的异常检测标准来检测罕见突变。从正常样品的序列数据推导统计模型。我们检测到肺癌患者血浆DNA中的表皮生长因子受体(EGFR)突变。单遍深度测序(> 100,000个读数)能够在10,000个正常等位基因中检测到一个激活的突变等位基因。我们使用22个前瞻性样本和155个回顾性样本确认了该方法,这些样本主要由从血浆中纯化的DNA组成。暂时性分析提示了疾病控制和选择表皮生长因子受体酪氨酸激酶抑制剂(EGFR-TKI)的治疗决策的潜在应用。

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