Moati Emilie, Blons Hélène, Taly Valerie, Garlan Fanny, Wang-Renault Shu-Fang, Pietrasz Daniel, Didelot Audrey, Garrigou Sonia, Saint Angélique, Pernot Simon, Taieb Julien, Laurent-Puig Pierre, Zaanan Aziz
Centre de Recherche des Cordeliers, INSERM, CNRS, Sorbonne Université, USPC, Université Paris Descartes, Université Paris Diderot, F-75006, Paris, France.
Department of Gastroenterology and Digestive Oncology, European Georges Pompidou Hospital, AP-HP, Paris Descartes University, Paris, France.
Int J Cancer. 2020 Aug 15;147(4):1185-1189. doi: 10.1002/ijc.32657. Epub 2019 Oct 12.
In metastatic colorectal cancer (mCRC), circulating tumor DNA (ctDNA) monitoring can be used to genotype tumors and track clonal evolution. We investigated the clearance of RAS mutated clones under chemotherapy pressure by ctDNA analysis in patients with a RAS mutated mCRC. Patients with a RAS mutated tumor included in the prospective PLACOL study were monitored for ctDNA. Analyses were based on optimized targeted next-generation sequencing and/or droplet-based digital polymerase chain reaction (ddPCR). For plasma samples without detectable mutations at progression disease, we tested the methylation status of WIF1 and NPY genes using methylation-ddPCR (met-ddPCR) to validate the presence of ctDNA. Among the 36 patients with positive plasma samples for RAS mutations at inclusion, 28 (77.8%) remained RAS positive at disease progression and 8 (22.2%) became negative. Subsequent met-ddPCR for methylated markers showed that only two out of the eight patients with RAS negative plasma had detectable ctDNA at progression. Therefore, only 2 samples among 36 were confirmed for clearance of RAS mutation in our series. In conclusion, this study suggests that the clearance of RAS mutations in patients treated by chemotherapy for a RAS mutated mCRC is a rare event. Monitoring tumor mutations in plasma samples should be combined with a strict control of the presence of ctDNA. The therapeutic impacts of RAS clearance need to be further explored.
在转移性结直肠癌(mCRC)中,循环肿瘤DNA(ctDNA)监测可用于肿瘤基因分型和追踪克隆进化。我们通过对RAS突变型mCRC患者进行ctDNA分析,研究了化疗压力下RAS突变克隆的清除情况。对前瞻性PLACOL研究中纳入的RAS突变肿瘤患者进行ctDNA监测。分析基于优化的靶向二代测序和/或基于液滴的数字聚合酶链反应(ddPCR)。对于疾病进展时未检测到突变的血浆样本,我们使用甲基化-ddPCR(met-ddPCR)检测WIF1和NPY基因的甲基化状态,以验证ctDNA的存在。在纳入时血浆样本RAS突变呈阳性的36例患者中,28例(77.8%)在疾病进展时仍为RAS阳性,8例(22.2%)转为阴性。随后对甲基化标志物进行的met-ddPCR显示,血浆RAS阴性的8例患者中只有2例在疾病进展时可检测到ctDNA。因此,在我们的系列研究中,36例样本中只有2例被证实RAS突变清除。总之,本研究表明,化疗治疗的RAS突变型mCRC患者中RAS突变的清除是罕见事件。监测血浆样本中的肿瘤突变应与严格控制ctDNA的存在相结合。RAS清除的治疗影响需要进一步探索。
