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异常启动子甲基化作为肺癌分子细胞学诊断的生物标志物

[Aberrant promoter methylation as biomarker for molecular cytological diagnosis of lung cancer].

作者信息

Grote H J

机构信息

Institut für Cytopathologie, Universität, Düsseldorf.

出版信息

Verh Dtsch Ges Pathol. 2006;90:216-26.

PMID:17867600
Abstract

Aberrant promoter methylation represents a main mechanism of tumor suppressor gene inactivation and may serve as a new source for biomarker discovery. This study investigated its applicability as a molecular tool for lung cancer diagnostics on bronchial aspirates. A methylation assay was developed applying a quantitative methylation specific real-time PCR (QMSP). A total of 552 patients with the differential diagnosis of lung cancer were investigated. The QMSP findings on bronchial aspirates were compared with the methylation status of respective genes investigated in microdissected tumor tissues (QMSP, cloning and sequencing of promoter regions after bisulfite conversion). Among the genes tested a marker panel consisting of APC, p16(INK4a) and RASSF1A proved to be the best suited for lung cancer diagnostics. This panel allowed for a correct diagnosis of lung cancer in cases with an ambiguous or false negative conventional cytology. In a cohort study on 247 patients, the combination of histology (sensitivity 59 %), cytology (sensitivity 44 %) and QMSP-assay (sensitivity 53 %) raised the sensitivity of a single bronchoscopy for the diagnosis of lung cancer up to 81%. The methylation assay yielded its major diagnostic surplus with respect to peripheral tumors representing 59 % of all primaries detected. In patients without antecedent lung cancer its specificity considering malignancy was >99 %. Therefore, the QMSP-assay is a promising technique which could enhance the sensitivity and diagnostic impact of conventional cytology. The assay is applicable to residual material of regular diagnostic cytology even in retrospect.

摘要

异常的启动子甲基化是肿瘤抑制基因失活的主要机制,可能成为生物标志物发现的新来源。本研究探讨了其作为支气管吸出物肺癌诊断分子工具的适用性。采用定量甲基化特异性实时PCR(QMSP)开发了一种甲基化检测方法。共对552例肺癌鉴别诊断患者进行了研究。将支气管吸出物的QMSP检测结果与显微切割肿瘤组织中相应基因的甲基化状态进行比较(QMSP、亚硫酸氢盐转化后启动子区域的克隆和测序)。在所检测的基因中,由APC、p16(INK4a)和RASSF1A组成的标志物组合被证明最适合肺癌诊断。该组合能够在传统细胞学诊断不明确或假阴性的病例中正确诊断肺癌。在一项对247例患者的队列研究中,组织学(敏感性59%)、细胞学(敏感性44%)和QMSP检测(敏感性53%)的联合应用将单次支气管镜检查诊断肺癌的敏感性提高到了81%。甲基化检测在周围型肿瘤诊断方面具有显著优势,周围型肿瘤占所有原发性肿瘤的59%。在无既往肺癌病史的患者中,考虑恶性肿瘤时其特异性>99%。因此,QMSP检测是一种有前景的技术,可提高传统细胞学的敏感性和诊断价值。该检测方法甚至可追溯应用于常规诊断细胞学的剩余样本。

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引用本文的文献

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Effect of DNA methylation inhibitor on RASSF1A genes expression in non-small cell lung cancer cell line A549 and A549DDP.DNA 甲基化抑制剂对非小细胞肺癌细胞系 A549 和 A549DDP 中 RASSF1A 基因表达的影响。
Cancer Cell Int. 2013 Sep 8;13(1):91. doi: 10.1186/1475-2867-13-91.
2
DNA methylation biomarkers offer improved diagnostic efficiency in lung cancer.DNA 甲基化生物标志物可提高肺癌的诊断效率。
Cancer Res. 2012 Nov 15;72(22):5692-701. doi: 10.1158/0008-5472.CAN-12-2309. Epub 2012 Sep 7.