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胸腔积液中异常的 DNA 甲基化谱可用于恶性胸膜间皮瘤的鉴别诊断。

Aberrant DNA methylation profile in pleural fluid for differential diagnosis of malignant pleural mesothelioma.

机构信息

Department of Respiratory Medicine, Okayama Rosai Hospital, Okayama, Japan.

出版信息

Cancer Sci. 2012 Mar;103(3):510-4. doi: 10.1111/j.1349-7006.2011.02180.x. Epub 2012 Jan 13.

Abstract

Malignant pleural mesothelioma (MPM) usually develops pleural fluid. We investigated the value of DNA methylation in the pleural fluid for differentiating MPM from lung cancer (LC). Pleural fluid was collected from 39 patients with MPM, 46 with LC, 25 with benign asbestos pleurisy (BAP) and 30 with other causes. The methylation of O(6)-methylguanine-DNA methyltransferase (MGMT), p16(INK4a) , ras association domain family 1A (RASSF1A), death-associated protein kinase (DAPK), and retinoic acid receptor β (RARβ) was examined using quantitative real-time PCR. DNA methylation of RASSF1A, p16(INK4a), RARβ, MGMT and DAPK was detected in 12 (30.8%), 3 (7.7%), 11 (28.2%), 0 (0.0%) and five patients (12.8%) with MPM, and in 22 (47.8%), 14 (30.4%), 24 (52.2%), 1 (2.2%) and six patients (13.0%) with LC, respectively. The mean methylation ratios of RASSF1A, p16(INK4a) and RARβ were 0.37 (range 0.0-2.84), 0.11 (0.0-2.67) and 0.44 (0.0-3.32) in MPM, and 0.87 (0.0-3.14), 1.16 (0.0-5.35) and 1.69 (0.0-6.49) in LC, respectively. The methylation ratios for the three genes were significantly higher in LC than in MPM (RASSF1A, P = 0.039; p16(INK4a), P = 0.005; and RARβ, P = 0.002). Patients with methylation in at least one gene were 3.51 (95% confidence interval, 1.09-11.34) times more likely to have LC. Hypermethylation seemed no greater with MPM than with BAP. Extended exposure to asbestos (≧30 years) was correlated with an increased methylation frequency (P = 0.020). Hypermethylation of tumor suppressor genes in pleural fluid DNA has the potential to be a valuable marker for differentiating MPM from LC.

摘要

恶性胸膜间皮瘤(MPM)通常会产生胸腔积液。我们研究了胸腔积液中的 DNA 甲基化在区分 MPM 和肺癌(LC)中的价值。收集了 39 名 MPM 患者、46 名 LC 患者、25 名良性石棉性胸膜炎(BAP)患者和 30 名其他原因患者的胸腔积液。使用定量实时 PCR 检查 O(6)-甲基鸟嘌呤-DNA 甲基转移酶(MGMT)、p16(INK4a)、ras 相关结构域家族 1A(RASSF1A)、死亡相关蛋白激酶(DAPK)和维甲酸受体β(RARβ)的甲基化。在 12 名(30.8%)、3 名(7.7%)、11 名(28.2%)、0 名(0.0%)和 5 名(12.8%)MPM 患者中检测到 RASSF1A、p16(INK4a)、RARβ、MGMT 和 DAPK 的 DNA 甲基化,在 22 名(47.8%)、14 名(30.4%)、24 名(52.2%)、1 名(2.2%)和 6 名(13.0%)LC 患者中检测到 RASSF1A、p16(INK4a)和 RARβ的甲基化比例分别为 0.37(范围 0.0-2.84)、0.11(0.0-2.67)和 0.44(0.0-3.32),LC 患者为 0.87(0.0-3.14)、1.16(0.0-5.35)和 1.69(0.0-6.49)。与 MPM 相比,LC 中这三个基因的甲基化比例明显更高(RASSF1A,P = 0.039;p16(INK4a),P = 0.005;和 RARβ,P = 0.002)。至少有一个基因发生甲基化的患者发生 LC 的可能性是 MPM 的 3.51 倍(95%置信区间,1.09-11.34)。与 BAP 相比,MPM 中似乎没有更大的高甲基化。石棉暴露时间延长(≧30 年)与甲基化频率增加相关(P = 0.020)。胸腔积液 DNA 中肿瘤抑制基因的高甲基化有可能成为区分 MPM 和 LC 的有价值的标志物。

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