Monitoring of somatic mutations in circulating cell-free DNA by digital PCR and next-generation sequencing during afatinib treatment in patients with lung adenocarcinoma positive for EGFR activating mutations

阿法替尼 数字聚合酶链反应 医学 肺癌 液体活检 表皮生长因子受体 腺癌 冷PCR 内科学 肿瘤科 癌症研究 突变 癌症 聚合酶链反应 点突变 吉非替尼 生物 遗传学 基因
作者
Eiji Iwama,Kazuko Sakai,Koichi Azuma,Taishi Harada,Daijiro Harada,Kaname Nosaki,K. Hotta,F. Ohyanagi,Takeshi Kurata,Tatsuro Fukuhara,Hiroaki Akamatsu,Kōichi Goto,Takayuki Shimose,Junji Kishimoto,Yoichi Nakanishi,Kazuto Nishio,Isamu Okamoto
出处
期刊:Annals of Oncology [Elsevier BV]
卷期号:28 (1): 136-141 被引量:70
标识
DOI:10.1093/annonc/mdw531
摘要

BackgroundAnalysis of circulating cell-free DNA (cfDNA) is under intensive investigation for its potential to identify tumor somatic mutations. We have now explored the usefulness of such liquid biopsy testing with both the digital polymerase chain reaction (dPCR) and next-generation sequencing (NGS) during treatment of patients with the epidermal growth factor receptor (EGFR) inhibitor afatinib.Patients and methodsEligible patients had advanced lung adenocarcinoma with EGFR activating mutations and were treated with afatinib. Plasma samples were collected before and during (4 and 24 weeks) afatinib treatment as well as at disease progression. Tumor and plasma DNA were analyzed by dPCR and NGS.ResultsThirty-five patients were enrolled. The objective response rate and median progression-free survival (PFS) were 77.1% and 13.8 months, respectively. Tumor and plasma DNA were available for 32 patients. dPCR and NGS detected EGFR activating mutations in 81.3% and 71.9% of baseline cfDNA samples, respectively. In 19 patients treated with afatinib for ≥24 weeks, the number of EGFR mutant alleles detected in cfDNA by dPCR declined rapidly and markedly after treatment onset, becoming undetectable or detectable at only a low copy number (<10 copies per milliliter) at 4 weeks. Median PFS was slightly longer for patients with undetectable EGFR mutant alleles in cfDNA at 4 weeks than for those in whom such alleles were detectable (14.3 versus 10.0 months). A total of 45 somatic mutations was identified in baseline tumor DNA, and 30 (66.7%) of these mutations were identified in cfDNA by NGS. Allele frequency for somatic mutations in cfDNA determined by NGS changed concordantly during afatinib treatment with the number of EGFR mutant alleles determined by dPCR.ConclusionsMonitoring of cfDNA by dPCR is informative for prediction of afatinib efficacy, whereas that by NGS is reliable and has the potential to identify mechanisms of treatment resistance.

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