Saw Stephanie P L, Tan Gek San, Tan Wei Chong, Tan Aaron C, Lai Gillianne G Y, Lim Darren W T, Kanesvaran Ravindran, Tan Wan Ling, Tan Sze Huey, Lim Kiat Hon, Skanderup Anders J, Tan Daniel S W
Division of Medical Oncology, National Cancer Centre Singapore, Singapore.
Duke-NUS Medical School, National University of Singapore, Singapore.
JTO Clin Res Rep. 2023 Nov 2;4(12):100599. doi: 10.1016/j.jtocrr.2023.100599. eCollection 2023 Dec.
To compare the performance of droplet digital polymerase chain reaction (ddPCR) and plasma next-generation sequencing (NGS) in detecting clearance of plasma EGFR (pEGFR) mutations.
Patients with treatment-naive advanced EGFR-mutated lung cancer treated with first-line tyrosine kinase inhibitors (TKIs) were included. pEGFR were measured at baseline and first response assessment using ddPCR and NGS. Clearance of pEGFR was defined as undetectable levels after a positive baseline result. Results were correlated with time-to-treatment failure (TTF). In exploratory analysis, corresponding change in carcinoembryonic antigen (CEA) levels was evaluated.
Between January 1, 2020, and December 31, 2021, 27 patients were recruited. Ex19del comprised 74% (20 of 27) and L858R 26% (seven of 27). Osimertinib was used in 59% (16 of 27), dacomitinib 4% (one of 27), and gefitinib/erlotinib 37% (10 of 27). Sensitivity of ddPCR and NGS in detecting pEGFR mutation at baseline was 70% (19 of 27) and 78% (21 of 27), respectively ( = 0.16). All patients with detectable pEGFR by ddPCR were detected by NGS.At a median of 8 (range 3-24) weeks post-TKI initiation, clearance of pEGFR was achieved in 68% (13 of 19) and 71% (15 of 21) using ddPCR and NGS, respectively. Concordance between ddPCR and NGS was 79% (kappa = 0.513, = 0.013). Clearance of pEGFR was associated with longer median TTF (not reached versus 6 months, = 0.03) and median decrease in CEA levels by 70% from baseline.In another cohort of 124 patients, decrease in CEA levels by greater than 70% within 90 days of TKI initiation was associated with doubling of both TTF and overall survival.
Plasma NGS trended toward higher sensitivity than ddPCR in detecting pEGFR, although both had similar concordance in detecting pEGFR clearance. Our results support using NGS at diagnosis and interchangeability of NGS and ddPCR for monitoring, whereas CEA could be explored as a surrogate for pEGFR clearance.
比较液滴数字聚合酶链反应(ddPCR)和血浆下一代测序(NGS)检测血浆表皮生长因子受体(pEGFR)突变清除情况的性能。
纳入初治的晚期EGFR突变型肺癌患者,一线使用酪氨酸激酶抑制剂(TKIs)治疗。在基线和首次疗效评估时使用ddPCR和NGS检测pEGFR。pEGFR清除定义为基线结果为阳性后检测不到。结果与治疗失败时间(TTF)相关。在探索性分析中,评估癌胚抗原(CEA)水平的相应变化。
2020年1月1日至2021年12月31日期间,招募了27例患者。外显子19缺失占74%(27例中的20例),L858R占26%(27例中的7例)。59%(27例中的16例)使用奥希替尼,4%(27例中的1例)使用达可替尼,37%(27例中的10例)使用吉非替尼/厄洛替尼。ddPCR和NGS在基线时检测pEGFR突变的敏感性分别为70%(27例中的19例)和78%(27例中的21例)(P = 0.16)。所有通过ddPCR检测到可检测pEGFR的患者均通过NGS检测到。在开始使用TKIs后的中位8周(范围3 - 24周),使用ddPCR和NGS分别有68%(19例中的13例)和71%(21例中的15例)实现了pEGFR清除。ddPCR和NGS之间的一致性为79%(kappa = 0.513,P = 0.013)。pEGFR清除与更长的中位TTF相关(未达到与6个月相比,P = 0.03),且CEA水平从基线下降中位数为70%。在另一组124例患者中,在开始使用TKIs后90天内CEA水平下降大于70%与TTF和总生存期加倍相关。
血浆NGS在检测pEGFR方面的敏感性有高于ddPCR的趋势,尽管两者在检测pEGFR清除方面具有相似的一致性。我们的结果支持在诊断时使用NGS以及NGS和ddPCR在监测方面的互换性,而CEA可作为pEGFR清除的替代指标进行探索。
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