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一种经误差校正的超灵敏ctDNA下一代测序检测方法的分析验证

Analytical validation of an error-corrected ultra-sensitive ctDNA next-generation sequencing assay.

作者信息

Fettke Heidi, Steen Jason A, Kwan Edmond M, Bukczynska Patricia, Keerthikumar Shivakumar, Goode David, Docanto Maria, Ng Nicole, Martelotto Luciano, Hauser Christine, Southey Melissa C, Azad Arun A, Nguyen-Dumont Tu

机构信息

Department of Medicine, School of Clinical Sciences, Monash University, Melbourne, Australia.

Precision Medicine, School of Clinical Sciences at Monash Health, Melbourne, Australia.

出版信息

Biotechniques. 2020 Aug;69(2):133-140. doi: 10.2144/btn-2020-0045. Epub 2020 Jul 13.

Abstract

Plasma circulating tumor DNA (ctDNA) analysis has emerged as a minimally invasive means to perform molecular tumor typing. Here we developed a custom ultra-sensitive ctDNA next-generation sequencing assay using molecular barcoding technology and off-the-shelf reagents combined with bioinformatics tools for enhanced ctDNA analysis. Assay performance was assessed via a spike-in experiment and the technique was applied to analyze 41 plasma samples from men with advanced prostate cancer. Orthogonal validation was performed using a commercial assay. Sensitivity and specificity of 93 and 99.5% were recorded for ultra-rare somatic variants (<1%), with high concordance observed between the in-house and commercial assays. The optimized protocol dramatically improved the efficiency of the assay and enabled the detection of low-frequency somatic variants from plasma cell-free DNA (cfDNA).

摘要

血浆循环肿瘤DNA(ctDNA)分析已成为一种用于进行分子肿瘤分型的微创手段。在此,我们开发了一种定制的超灵敏ctDNA下一代测序检测方法,该方法使用分子条形码技术和现成试剂,并结合生物信息学工具以增强ctDNA分析。通过加标实验评估检测性能,并将该技术应用于分析41例晚期前列腺癌男性患者的血浆样本。使用商业检测方法进行正交验证。对于超罕见体细胞变异(<1%),记录的灵敏度和特异性分别为93%和99.5%,内部检测方法与商业检测方法之间观察到高度一致性。优化后的方案显著提高了检测效率,并能够从血浆游离DNA(cfDNA)中检测低频体细胞变异。

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