Yang Xue, Zhuo Minglei, Ye Xin, Bai Hua, Wang Zhijie, Sun Yun, Zhao Jun, An Tongtong, Duan Jianchun, Wu Meina, Wang Jie
Department of Thoracic Medical Oncology, Key Laboratory of Carcinogenesis and Translational Research (Ministry of Education), Peking University Cancer Hospital and Institute, Beijing, China.
Asia and Emerging Markets Innovative Medicine of AstraZeneca R & D, Shanghai, China.
Oncotarget. 2016 Apr 12;7(15):20810-24. doi: 10.18632/oncotarget.8021.
We aimed to investigate the feasibility of droplet digital PCR (ddPCR) for the quantitative and dynamic detection of EGFR mutations and next generation sequencing (NGS) for screening EGFR-tyrosine kinase inhibitors (EGFR-TKIs) resistance-relevant mutations in circulating tumor DNA (ctDNA) from advanced lung adenocarcinoma (ADC) patients.
Detection limit of EGFR mutation in ctDNA by ddPCR was 0.04%. Taking the EGFR mutation in tumor tissue as the golden standard, the concordance of EGFR mutations detected in ctDNA was 74% (54/73). Patients with EGFR mutation in ctDNA (n = 54) superior progression-free survival (PFS, median, 12.6 vs. 6.7 months, P < 0.001) and overall survival (OS, median, 35.6 vs. 23.8 months, P = 0.028) compared to those with EGFR wild type in ctDNA (n = 19). Patients with high EGFR-mutated abundance in ctDNA (> 5.15%) showed better PFS compared to those with low EGFR mutated abundance (≤ 5.15%) (PFS, median, 15.4 vs. 11.1 months, P = 0.021). NGS results showed that 66.6% (8/12) total mutational copy number were elevated and 76.5% (26/34) mutual mutation frequency increased after disease progression.
Seventy-three advanced ADC patients with tumor tissues carrying EGFR mutations and their matched pre- and post-EGFR-TKIs plasma samples were enrolled in this study. Absolute quantities of plasma EGFR mutant and wild-type alleles were measured by ddPCR. Multi-genes testing was performed using NGS in 12 patients.
Dynamic and quantitative analysis of EGFR mutation in ctDNA could guide personalized therapy for advanced ADC. NGS shows good performance in multiple genes testing especially novel and uncommon genes.
我们旨在研究液滴数字PCR(ddPCR)用于定量和动态检测表皮生长因子受体(EGFR)突变的可行性,以及二代测序(NGS)用于筛查晚期肺腺癌(ADC)患者循环肿瘤DNA(ctDNA)中与EGFR酪氨酸激酶抑制剂(EGFR-TKIs)耐药相关突变的可行性。
ddPCR检测ctDNA中EGFR突变的检测限为0.04%。以肿瘤组织中的EGFR突变作为金标准,ctDNA中检测到的EGFR突变的一致性为74%(54/73)。与ctDNA中EGFR野生型患者(n = 19)相比,ctDNA中存在EGFR突变的患者(n = 54)的无进展生存期(PFS,中位数,12.6对6.7个月,P < 0.001)和总生存期(OS,中位数,35.6对23.8个月,P = 0.028)更长。ctDNA中EGFR突变丰度高(> 5.15%)的患者与EGFR突变丰度低(≤ 5.15%)的患者相比,PFS更好(PFS,中位数,15.4对11.1个月,P = 0.021)。NGS结果显示,疾病进展后,总突变拷贝数的66.6%(8/12)升高,相互突变频率的76.5%(26/34)增加。
本研究纳入了73例肿瘤组织携带EGFR突变的晚期ADC患者及其匹配的EGFR-TKIs治疗前后的血浆样本。通过ddPCR测量血浆EGFR突变和野生型等位基因的绝对量。对12例患者使用NGS进行多基因检测。
对ctDNA中EGFR突变进行动态和定量分析可为晚期ADC的个体化治疗提供指导。NGS在多基因检测尤其是新的和不常见基因检测方面表现良好。
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