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通过cfDNA分析对晚期非小细胞肺癌患者进行分子特征分析:来自常规实验室实践的经验

Molecular characterization of advanced non-small cell lung cancer patients by cfDNA analysis: experience from routine laboratory practice.

作者信息

González de Aledo-Castillo José Manuel, Arcocha Ainara, Victoria Iván, Martinez-Puchol Ana Isabel, Sánchez Cristina, Jares Pedro, Rodríguez Gabriel Felipe, Viñolas Núria, Reyes Roxana, Reguart Noemí, Puig-Butillé Joan Antón

机构信息

Biochemistry and Molecular Genetics Department, Hospital Clínic, Barcelona, Spain.

Thoracic Oncology Unit, Hospital Clínic, Barcelona, Spain.

出版信息

J Thorac Dis. 2021 Mar;13(3):1658-1670. doi: 10.21037/jtd-20-3142.

Abstract

BACKGROUND

Analysis of circulating free DNA (cfDNA) by the real-time PCR cobas EGFR Mutation Test v2 (cobas EGFR Test) is a diagnostic approach used in clinical practice for the characterization of advanced non-small cell lung cancer (NSCLC) patients. The test additionally outputs a semiquantitative index (SQI) which reflects the proportion of mutated versus wild-type copies of the gene in cfDNA with potential use as a biomarker. CfDNA concentration and cfDNA fragmentation pattern have also shown potential utility as biomarkers for cancer patients. We evaluated the implementation of testing and cfDNA related parameters in NSCLC patients in routine clinical setting as biomarkers for disease stage and diagnosis.

METHODS

A prospective cohort of 173 locally advanced or metastatic NSCLC TKI-naïve patients analyzed by the cobas EGFR Test were included in the study. Reproducibility of the test was assessed in 56 patients. The concentration of cfDNA and fragment size pattern was measured using fluorometry and microchip electrophoresis respectively.

RESULTS

The test showed high diagnostic accuracy when compared to the gold standard of biopsy tumor tissue testing. The SQI value showed a moderate reproducibility (r=0.70) and did not correlate with cfDNA concentration (r=0.17, P=0.28) or disease stage (stage III patients SQI =9.1±3.1 and stage IV patients SQI =11.5±4.8, P=0.41). We found differences in SQI values according to the type of mutation (Ex19Del mutations, SQI =13.6; p.L858R, SQI =8.88; P=0.001). Stage IV patients had higher concentrations of cfDNA (P<0.0001) and higher fractions of cfDNA 100-250 base pairs (bp) fragments (P=0.01) compared to stage III patients. From the ROC curve analysis, cfDNA concentration showed higher AUC compared to cfDNA 100-250 bp fragments (0.86 . 0.71). We obtained a cut-off value for cfDNA concentration of 20.3 ng/mL with 72.3% sensitivity and 95% specificity for predicting disease stage in TKI-naïve advanced NSCLC patients.

CONCLUSIONS

The study indicates that cfDNA analysis in plasma for testing by RT-PCR is an accurate and fast method to initially stratify NSCLC patients in a real-world clinical setting. However, the SQI has limited clinical value. The cfDNA concentration and fragmentation pattern have clear potential clinical utility for tumor staging in NSCLC patients.

摘要

背景

采用实时荧光定量PCR cobas EGFR突变检测v2(cobas EGFR检测)分析循环游离DNA(cfDNA)是临床实践中用于晚期非小细胞肺癌(NSCLC)患者特征分析的一种诊断方法。该检测还会输出一个半定量指标(SQI),它反映了cfDNA中该基因的突变型与野生型拷贝的比例,有可能用作生物标志物。cfDNA浓度和cfDNA片段化模式也已显示出作为癌症患者生物标志物的潜在效用。我们评估了在常规临床环境中对NSCLC患者进行该检测及cfDNA相关参数作为疾病分期和诊断生物标志物的实施情况。

方法

本研究纳入了173例未经TKI治疗的局部晚期或转移性NSCLC患者的前瞻性队列,通过cobas EGFR检测进行分析。对56例患者评估了该检测的重复性。分别使用荧光测定法和微芯片电泳测量cfDNA的浓度和片段大小模式。

结果

与活检肿瘤组织检测的金标准相比,该检测显示出较高的诊断准确性。SQI值显示出中等重复性(r = 0.70),且与cfDNA浓度(r = 0.17,P = 0.28)或疾病分期无关(III期患者SQI = 9.1±3.1,IV期患者SQI = 11.5±4.8,P = 0.41)。我们发现根据突变类型,SQI值存在差异(Ex19Del突变,SQI = 13.6;p.L858R,SQI = 8.88;P = 0.001)。与III期患者相比,IV期患者的cfDNA浓度更高(P < 0.0001),且cfDNA 100 - 250碱基对(bp)片段的比例更高(P = 0.01)。通过ROC曲线分析,cfDNA浓度的AUC高于cfDNA 100 - 250 bp片段(0.86对0.71)。我们得出cfDNA浓度的截断值为20.3 ng/mL,在预测未经TKI治疗的晚期NSCLC患者疾病分期时,灵敏度为72.3%,特异性为95%。

结论

该研究表明,在现实临床环境中,通过RT-PCR对血浆中的cfDNA进行分析以进行检测是一种准确且快速的方法,可用于对NSCLC患者进行初步分层。然而,SQI的临床价值有限。cfDNA浓度和片段化模式在NSCLC患者肿瘤分期方面具有明确的潜在临床效用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/091f/8024825/d05025b3b8b1/jtd-13-03-1658-f1.jpg

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