Utility of incorporating next-generation sequencing (NGS) in an Asian non-small cell lung cancer (NSCLC) population: Incremental yield of actionable alterations and cost-effectiveness analysis

医学 克拉斯 ROS1型 肿瘤科 肺癌 腺癌 靶向治疗 DNA测序 生物标志物 内科学 阶段(地层学) 癌症 病理 生物信息学 基因 生物 遗传学 结直肠癌 古生物学
作者
Aaron C. Tan,Gillianne Lai,Gek San Tan,Shou Yu Poon,Brett Doble,Tse Hui Lim,Zaw Win Aung,Angela Takano,Wan Ling Tan,Mei‐Kim Ang,Bien Soo Tan,Devanand Anantham,Chow Wei Too,Apoorva Gogna,Boon‐Hean Ong,Tina Koh,Ravindran Kanesvaran,Quan Sing Ng,Amit Jain,Tanujaa Rajasekaran
出处
期刊:Lung Cancer [Elsevier BV]
卷期号:139: 207-215 被引量:114
标识
DOI:10.1016/j.lungcan.2019.11.022
摘要

Abstract

Objectives

There is an expanding list of therapeutically relevant biomarkers for non-small cell lung cancer (NSCLC), and molecular profiling at diagnosis is paramount. Tissue attrition in scaling traditional single biomarker assays from small biopsies is an increasingly encountered problem. We sought to compare the performance of targeted next-generation sequencing (NGS) panels with traditional assays and correlate the mutational landscape with PD-L1 status in Singaporean patients.

Materials and methods

We identified consecutive patients diagnosed between Jan 2016 to Sep 2017 with residual tissue after standard molecular testing. Tissue samples were tested using a targeted NGS panel for DNA alterations (29 selected genes including BRAF, EGFR, ERBB2 and TP53) and an RNA fusion panel (ALK, ROS1 and RET). PD-L1 immunohistochemistry was also performed. A cost-effectiveness analysis of NGS compared to standard molecular testing was conducted.

Results

A total of 174 samples were evaluated: PD-L1 (n = 169), NGS DNA panel (n = 173) and RNA fusion (n = 119) testing. Median age was 68 years, 53 % were male, 58 % were never smokers, 85 % were Chinese, 66 % had stage IV disease and 95 % had adenocarcinoma histology. In patients profiled with NGS on DNA, EGFR (56 %), KRAS (14 %), BRAF (2 %) and ERBB2 (1 %) mutations were found. RNA fusion testing revealed fusions in ALK (6 %), RET (3 %) and ROS1 (1 %). Cost-effectiveness analysis demonstrated that compared to sequential testing in EGFR negative patients, upfront NGS testing would result in an additional 1 % of patients with actionable alterations for targeted therapy being identified without significant increases in testing cost or turnaround time.

Conclusions

This study demonstrates that even in an EGFR mutant predominant population, upfront NGS represents a feasible, cost-effective method of diagnostic molecular profiling compared with sequential testing strategies. Our results support the implementation of diagnostic NGS in non-squamous NSCLC in Asia to allow patients access to the most appropriate personalized therapy.
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