用于诊断人乳头瘤病毒阳性和阴性头颈癌的唾液DNA甲基化检测板
Salivary DNA methylation panel to diagnose HPV-positive and HPV-negative head and neck cancers.
作者信息
Lim Yenkai, Wan Yunxia, Vagenas Dimitrios, Ovchinnikov Dmitry A, Perry Chris F L, Davis Melissa J, Punyadeera Chamindie
机构信息
The School of Biomedical Sciences, Institute of Health and Biomedical Innovation, Queensland University of Technology, GPO Box 2434, 60 Musk Avenue, Kelvin Grove, Brisbane, QLD, 4059, Australia.
Australian Institute for Bioengineering and Nanotechnology, University of Queensland, St Lucia, Brisbane, QLD, 4072, Australia.
出版信息
BMC Cancer. 2016 Sep 23;16(1):749. doi: 10.1186/s12885-016-2785-0.
BACKGROUND
Head and neck squamous cell carcinoma (HNSCC) is a heterogeneous group of tumours with a typical 5 year survival rate of <40 %. DNA methylation in tumour-suppressor genes often occurs at an early stage of tumorigenesis, hence DNA methylation can be used as an early tumour biomarker. Saliva is an ideal diagnostic medium to detect early HNSCC tumour activities due to its proximity to tumour site, non-invasiveness and ease of sampling. We test the hypothesis that the surveillance of DNA methylation in five tumour-suppressor genes (RASSF1α, p16 , TIMP3, PCQAP/MED15) will allow us to diagnose HNSCC patients from a normal healthy control group as well as to discriminate between Human Papillomavirus (HPV)-positive and HPV-negative patients.
METHODS
Methylation-specific PCR (MSP) was used to determine the methylation levels of RASSF1α, p16 , TIMP3 and PCQAP/MED15 in DNA isolated from saliva. Statistical analysis was carried out using non-parametric Mann-Whitney's U-test for individually methylated genes. A logistic regression analysis was carried out to determine the assay sensitivity when combing the five genes. Further, a five-fold cross-validation with a bootstrap procedure was carried out to determine how well the panel will perform in a real clinical scenario.
RESULTS
Salivary DNA methylation levels were not affected by age. Salivary DNA methylation levels for RASSF1α, p16 , TIMP3 and PCQAP/MED15 were higher in HPV-negative HNSCC patients (n = 88) compared with a normal healthy control group (n = 122) (sensitivity of 71 % and specificity of 80 %). Conversely, DNA methylation levels for these genes were lower in HPV-positive HNSCC patients (n = 45) compared with a normal healthy control group (sensitivity of 80 % and specificity of 74 %), consistent with the proposed aetiology of HPV-positive HNSCCs.
CONCLUSIONS
Salivary DNA tumour-suppressor methylation gene panel has the potential to detect early-stage tumours in HPV-negative HNSCC patients. HPV infection was found to deregulate the methylation levels in HPV-positive HNSCC patients. Large-scale double-blinded clinical trials are crucial before this panel can potentially be integrated into a clinical setting.
背景
头颈部鳞状细胞癌(HNSCC)是一组异质性肿瘤,其典型的5年生存率<40%。肿瘤抑制基因中的DNA甲基化通常发生在肿瘤发生的早期阶段,因此DNA甲基化可作为早期肿瘤生物标志物。唾液因其靠近肿瘤部位、无创且易于采集,是检测早期HNSCC肿瘤活动的理想诊断介质。我们检验了这样一个假设,即监测五个肿瘤抑制基因(RASSF1α、p16 、TIMP3、PCQAP/MED15)中的DNA甲基化将使我们能够从正常健康对照组中诊断出HNSCC患者,并区分人乳头瘤病毒(HPV)阳性和HPV阴性患者。
方法
采用甲基化特异性PCR(MSP)来确定从唾液中分离的DNA中RASSF1α、p16 、TIMP3和PCQAP/MED15的甲基化水平。对单个甲基化基因使用非参数曼-惠特尼U检验进行统计分析。进行逻辑回归分析以确定组合这五个基因时检测方法的敏感性。此外,采用带有自助法的五重交叉验证来确定该检测组合在实际临床场景中的表现。
结果
唾液DNA甲基化水平不受年龄影响。与正常健康对照组(n = 122)相比,HPV阴性的HNSCC患者(n = 88)中RASSF1α、p16 、TIMP3和PCQAP/MED15的唾液DNA甲基化水平更高(敏感性为71%,特异性为80%)。相反,与正常健康对照组相比,HPV阳性的HNSCC患者(n = 45)中这些基因的DNA甲基化水平更低(敏感性为80%,特异性为74%),这与HPV阳性HNSCC的病因学假设一致。
结论
唾液DNA肿瘤抑制甲基化基因检测组合有潜力检测HPV阴性HNSCC患者的早期肿瘤。发现HPV感染会使HPV阳性HNSCC患者的甲基化水平失调。在该检测组合有可能整合到临床应用之前,大规模双盲临床试验至关重要。
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