Mansuet-Lupo Audrey, Zouiti Fouzia, Alifano Marco, Tallet Anne, Charpentier Marie-Christine, Ducruit Véronique, Devez Fabrice, Lemaitre Fanny, Laurent-Puig Pierre, Damotte Diane, Blons Hélène
Université Paris Descartes, Sorbonne, Paris cité, France.
J Transl Med. 2014 May 16;12:131. doi: 10.1186/1479-5876-12-131.
Activating epidermal growth factor receptor (EGFR) mutations characterize a subgroup of non-small-cell lung cancer that benefit from first line EGFR tyrosine kinase inhibitors (EGFR-TKI). However, the existence of polyclonal cell populations may hinder personalized-medicine strategies as patients' screening often depends upon a single tumor-biopsy sample. The purpose of this study is to clarify and to validate in clinical testing conditions the accuracy of EGFR genotyping using different tumor sites and various types of samples (transthoracic, surgical or endoscopic biopsies and cytology specimens).
We conducted a retrospective review of 357 consecutive patients addressed for EGFR mutation screening in accordance with the directive of the European Medicines Agency (stage IV NSCLC). Fifty-seven samples were EGFR mutated and 40 had adequate tumor specimens for analysis on multiple spatially separated sites. Ten wild type samples were also analyzed. A total of 153 and 39 tumor fragments, from mutated and non-mutated cases respectively, were generated to analyze tumor heterogeneity or primary-metastatic discordances. After histological review of all fragments, EGFR genotyping was assessed using the routine diagnostic tools: fragment analysis for insertions and deletions and allele specific TaqMan probes for point mutations. EGFR copy number (CN) was evaluated by qPCR using TaqMan probes.
The identification of EGFR mutations was independent of localization within primary tumor, of specimen type and consistent between primary and metastases. At the opposite, for half of the samples, tumor loci showed different EGFR copy number that may affect mutation detection cut-off.
This is the largest series reporting multiple EGFR testing in Caucasians. It validates the accuracy of EGFR mutation screening from single tumor-biopsy samples before first line EGFR-TKI. The unpredictable variability in EGFR CN and therefore in EGFR wild type/mutant allelic ratio justifies the implementation of sensitive methods to identify patients with EGFR mutated tumors.
激活型表皮生长因子受体(EGFR)突变是一类非小细胞肺癌的特征,这类患者可从一线EGFR酪氨酸激酶抑制剂(EGFR-TKI)治疗中获益。然而,多克隆细胞群体的存在可能会阻碍个性化医疗策略,因为患者的筛查通常依赖于单个肿瘤活检样本。本研究的目的是在临床检测条件下阐明并验证使用不同肿瘤部位和各种类型样本(经胸、手术或内镜活检及细胞学标本)进行EGFR基因分型的准确性。
我们对357例按照欧洲药品管理局指南进行EGFR突变筛查的连续患者(IV期非小细胞肺癌)进行了回顾性研究。57个样本存在EGFR突变,40个有足够的肿瘤标本用于多个空间分离部位的分析。还分析了10个野生型样本。分别从突变和未突变病例中获取了共153个和39个肿瘤片段,以分析肿瘤异质性或原发灶与转移灶的不一致性。在对所有片段进行组织学检查后,使用常规诊断工具评估EGFR基因分型:用于插入和缺失的片段分析以及用于点突变的等位基因特异性TaqMan探针。使用TaqMan探针通过qPCR评估EGFR拷贝数(CN)。
EGFR突变的鉴定与原发肿瘤内的定位、标本类型无关,且原发灶和转移灶之间一致。相反,对于一半的样本,肿瘤位点显示出不同的EGFR拷贝数,这可能会影响突变检测阈值。
这是报道高加索人群中多次EGFR检测的最大系列研究。它验证了在一线EGFR-TKI治疗前从单个肿瘤活检样本进行EGFR突变筛查的准确性。EGFR CN的不可预测变异性以及因此导致的EGFR野生型/突变等位基因比例的变异性证明了采用敏感方法来识别EGFR突变肿瘤患者的合理性。
Zotero 插件