Clinical utility of plasma-based digital next-generation sequencing in oncogene-driven non-small-cell lung cancer patients with tyrosine kinase inhibitor resistance

被引:22
|
作者
Zugazagoitia, Jon [1 ,2 ,3 ,4 ]
Gomez-Rueda, Ana [5 ]
Jantus-Lewintre, Eloisa [3 ,6 ]
Isla, Dolores [7 ]
Camps, Carlos [3 ,8 ]
Ramos, Inmaculada [9 ]
Manuel Trigo, Jose [9 ]
Bernabe, Reyes [10 ]
Juan-Vidal, Oscar [11 ]
Miguel Sanchez-Torres, Jose [12 ]
Garcia-Campelo, Rosario [13 ]
Provencio, Mariano [14 ]
Felip, Enriqueta [15 ]
de Castro, Javier [16 ]
Faull, Iris [17 ]
Lanman, Richard B. [18 ]
Ponce-Aix, Santiago [1 ,2 ]
Paz-Ares, Luis [1 ,2 ,3 ,19 ]
Garrido, Pilar [3 ,5 ]
机构
[1] Hosp Univ 12 Octubre & i 12 Res Inst, Med Oncol Dept, Madrid, Spain
[2] Spanish Natl Canc Res Ctr CNIO, Clin Res Program, Lung Canc Grp, Madrid, Spain
[3] CIBERONC, Madrid, Spain
[4] Yale Sch Med, Dept Pathol, New Haven, CT USA
[5] Univ Alcala, IRYCIS Hosp Univ Ramon y Cajal, Med Oncol Dept, Madrid, Spain
[6] Univ Politecn Valencia, Fdn Invest Hosp Gen Univ Valencia, Mol Oncol Lab, Valencia, Spain
[7] Hosp Univ Lozano Blesa, Med Oncol Dept, Zaragoza, Spain
[8] Univ Valencia, Med Dept, Hosp Gen Univ Valencia, Med Oncol Dept, Valencia, Spain
[9] Hosp Univ Virgen Victoria, Med Oncol Dept, Malaga, Spain
[10] Hosp Univ Virgen Rocio, Med Oncol Dept, Seville, Spain
[11] Hosp Univ & Politecn La Fe, Med Oncol Dept, Valencia, Spain
[12] Hosp Univ La Princesa, Med Oncol Dept, Madrid, Spain
[13] Hosp Univ Coruna, Med Oncol Dept, La Coruna, Spain
[14] Hosp Univ Puerta Hierro, Med Oncol Dept, Madrid, Spain
[15] Hosp Univ Vall dHebron, Med Oncol Dept, Barcelona, Spain
[16] Hosp Univ La Paz, Med Oncol Dept, Madrid, Spain
[17] Guardant Hlth, Med Affairs, Barcelona, Spain
[18] Guardant Hlth, Med Affairs, Redwood City, CA USA
[19] Univ Complutense Madrid, Madrid, Spain
关键词
Oncogene-driven NSCLC; TKI resistance; Osimertinib; ctDNA; Digital next-generation sequencing; EGFR; CHEMOTHERAPY; CRIZOTINIB; MECHANISMS; MUTATIONS; IMPACT;
D O I
10.1016/j.lungcan.2019.05.032
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Objectives: Resistance to tyrosine-kinase inhibitors (TKIs) is a clinical challenge in patients with oncogene-driven non-small-cell lung cancers (NSCLC). We have analyzed the utility of next-generation sequencing (NGS) of cell-free circulating tumor DNA (ctDNA) to impact the clinical care of patients with TKI resistance. Materials and methods: We conducted a multi-institutional prospective study including consecutive EGFR, ALK, or ROS1-altered NSCLC patients with TKI resistance from 12 Spanish institutions. Post-progression ctDNA NGS was performed by Guardant Health (Guardant360 assay). Results: We included 53 patients separated in 3 cohorts: 31 EGFR-mutant NSCLCs with first/second-generation TKI resistance (cohort 1), 15 EGFR T790M + NSCLCs with osimertinib resistance (cohort 2), and 7 ALK/ROS1-rearranged NSCLCs with crizotinib and/or next-generation TKI resistance (cohort 3). Besides Guardant360, 22 patients from cohort 1 (71%) underwent post-progression tumor biopsies and/or alternative plasma-based genotyping. In the entire study population, 34 patients (64%) had reliable evidence of tumor-DNA shed for resistance assessment, and 24 patients (45%) had actionable alterations. Target-independent pathogenic alterations were frequently detected, particularly at osimertinib resistance. Eleven patients (20%) received subsequent molecular-guided therapies indicated by plasma NGS alone (n = 9, 17%), or plasma NGS and tissue sequencing (n = 2, 4%), deriving the expected clinical benefit. Of these, 9 had EGFR T790 M mutation and received osimertinib, 1 had ALK G1202R mutation and received lorlatinib, and 1 had ROS1 G2032R mutation and received cabozantinib. Two additional cases from cohort 1 (6%) had undetectable EGFR T790 M by Guardant360 but were T790M + by tissue and BEAMing digital PCR respectively, and also received osimertinib. Conclusion: NGS of ctDNA detects actionable alterations in a large proportion of oncogene-driven NSCLC patients with TKI resistance, and can be used to guide subsequent treatments as a complement or alternative to tissue or PCR-based plasma genotyping in the real-world clinical setting.
引用
收藏
页码:72 / 78
页数:7
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