Journal of Clinical Medicine (Sep 2019)

Subtyping Lung Cancer Using DNA Methylation in Liquid Biopsies

  • Sandra P. Nunes,
  • Francisca Diniz,
  • Catarina Moreira-Barbosa,
  • Vera Constâncio,
  • Ana Victor Silva,
  • Júlio Oliveira,
  • Marta Soares,
  • Sofia Paulino,
  • Ana Luísa Cunha,
  • Jéssica Rodrigues,
  • Luís Antunes,
  • Rui Henrique,
  • Carmen Jerónimo

DOI
https://doi.org/10.3390/jcm8091500
Journal volume & issue
Vol. 8, no. 9
p. 1500

Abstract

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Background: Lung cancer (LCa) is the most frequently diagnosed and lethal cancer worldwide. Histopathological subtyping, which has important therapeutic and prognostic implications, requires material collection through invasive procedures, which might be insufficient to enable definitive diagnosis. Aberrant DNA methylation is an early event in carcinogenesis, detectable in circulating cell-free DNA (ccfDNA). Herein, we aimed to assess methylation of selected genes in ccfDNA from LCa patients and determine its accuracy for tumor subtyping. Methods: Methylation levels of APC, HOXA9, RARβ2, and RASSF1A were assessed in three independent study groups (study group #1: 152 tissue samples; study group #2: 129 plasma samples; study group #3: 28 benign lesions of lung) using quantitative methylation-specific PCR. Associations between gene promoter methylation levels and LCa subtypes were evaluated using non-parametric tests. Receiver operating characteristic (ROC) curve analysis was performed. Results: In study group #2, HOXA9 and RASSF1A displayed higher methylation levels in small-cell lung cancer (SCLC) than in non-small-cell lung cancer (NSCLC). HOXA9 displayed high sensitivity (63.8%), whereas RASSF1A disclosed high specificity (96.2%) for SCLC detection in ccfDNA. Furthermore, HOXA9 methylation levels showed to be higher in squamous cell carcinoma in comparison with adenocarcinoma in study group #1. Conclusions: Methylation level assessments in ccfDNA may provide a minimally invasive procedure for LCa subtyping, complementing standard diagnostic procedures.

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