小细胞肺癌血浆游离 DNA 的基因组改变及其临床意义。

Genomic alterations of plasma cell-free DNAs in small cell lung cancer and their clinical relevance.

机构信息

Department of Pathology and Cancer Center, Medical College of Wisconsin, Milwaukee, WI, USA.

Division of Hematology/Oncology, Department of Medicine, Medical College of Wisconsin, Milwaukee, WI, USA.

出版信息

Lung Cancer. 2018 Jun;120:113-121. doi: 10.1016/j.lungcan.2018.04.008. Epub 2018 Apr 12.

DOI:10.1016/j.lungcan.2018.04.008

PMID:29748005

Abstract

OBJECTIVES

To identify genomic variations in cell-free DNA (cfDNA) and evaluate their clinical utility in small cell lung cancer (SCLC).

MATERIALS AND METHODS

We performed whole genome sequencing using plasma cfDNAs derived from 24 SCLC patients for copy number variation (CNV) analysis, and targeted sequencing using 17 pairs of plasma cfDNA and their matched gDNA for mutation analysis. We defined somatic mutations by comparing cfDNA to its matched gDNA with 5% variant alleles as the cutoff for mutation calls. We applied Kaplan-Meier to correlate the genomic alterations with overall survival (OS) and progression-free survival (PFS).

RESULTS

We observed widespread somatic copy-number alterations and mutations, including amplification of MYC at 8q24, FGF10 at 5p13, SOX2 at 3q26 and FGFR1 at 8p12, as well as deletion of TP53 at 17p13, RASSF1 at 3p21.3, RB1 at 13q14.2, FHIT at 3p14, and PTEN at 10q23. The most frequent mutations were genes involved in chromatin regulation (KMT2D, ARID1A, SETBP1 and PBRM1), PI3K/MTOR pathway(MTOR,PIK13G), Notch1 signalling pathway (NOTCH1), and DNA repair related gene ATRX. Kaplan-Meier analysis revealed poor OS and PFS in patients with somatic mutations in gene SETBP1 (P = 0.0061/0.0264, HR = 4.785/3.841, 95% CI = 2.014-28.25/1.286-16.58) and PBRM1 (P = 0.0276/0.0286, HR = 3.532/3.506, 95% CI = 1.275 to 25.34/1.26-24.87). Poor OS was also associated with somatic mutations in ATRX (P = 0.0099, HR = 4.024, 95% CI = 1.926-42.95), EP300 (P = 0.025/0.0622, HR = 3.382/2.891, 95% CI = 1.448-27.76/1.013-17.29), while poor PFS was associated with ATM mutation (P = 0.0038, HR = 4.604, 95% CI = 2.211-40.93). The mutation index produced by summing up the number of mutations in the five genes was significantly associated with the poor OS/PFS (P = 0.0185/0.0294) after adjusting the effect of the stage.

CONCLUSIONS

Our result supports blood plasma as a promising sample source for the genomic analysis in SCLC patients whose tumor tissues are scarcely available and demonstrates potential clinical utilities of cfDNA-based liquid biopsy for clinical management of this deadly disease.

摘要

目的

鉴定游离 DNA(cfDNA)中的基因组变异，并评估其在小细胞肺癌(SCLC)中的临床应用。

材料和方法

我们对 24 名 SCLC 患者的血浆 cfDNA 进行全基因组测序，进行拷贝数变异(CNV)分析，并对 17 对血浆 cfDNA 及其匹配的 gDNA 进行靶向测序，进行突变分析。我们通过将 cfDNA 与匹配的 gDNA 进行比较，将等位基因变异百分比为 5%的定义为突变。我们应用 Kaplan-Meier 法将基因组改变与总生存期(OS)和无进展生存期(PFS)相关联。

结果

我们观察到广泛的体细胞拷贝数改变和突变，包括 8q24 处 MYC 的扩增、5p13 处 FGF10、3q26 处 SOX2 和 8p12 处 FGFR1，以及 17p13 处 TP53、3p21.3 处 RASSF1、13q14.2 处 RB1、3p14 处 FHIT 和 10q23 处 PTEN 的缺失。最常见的突变涉及染色质调节基因(KMT2D、ARID1A、SETBP1 和 PBRM1)、PI3K/MTOR 通路(MTOR、PIK13G)、Notch1 信号通路(NOTCH1)和 DNA 修复相关基因 ATRX。Kaplan-Meier 分析显示，SETBP1 基因体细胞突变患者的 OS 和 PFS 较差(P=0.0061/0.0264，HR=4.785/3.841，95%CI=2.014-28.25/1.286-16.58)，PBRM1 基因体细胞突变患者的 OS 和 PFS 也较差(P=0.0276/0.0286，HR=3.532/3.506，95%CI=1.275-25.34/1.26-24.87)。ATRX 基因体细胞突变与 OS 较差也相关(P=0.0099，HR=4.024，95%CI=1.926-42.95)，EP300 基因体细胞突变与 OS 和 PFS 较差相关(P=0.025/0.0622，HR=3.382/2.891，95%CI=1.448-27.76/1.013-17.29)，而 ATM 突变与 PFS 较差相关(P=0.0038，HR=4.604，95%CI=2.211-40.93)。调整阶段的影响后，五个基因的突变数之和产生的突变指数与 OS/PFS 较差显著相关(P=0.0185/0.0294)。