4.7 Article

Promoter methylation of P16, RARβ, E-cadherin, cyclin A1 and cytoglobin in oral cancer:: quantitative evaluation using pyrosequencing

Journal

BRITISH JOURNAL OF CANCER
Volume 94, Issue 4, Pages 561-568

Publisher

NATURE PUBLISHING GROUP
DOI: 10.1038/sj.bjc.6602972

Keywords

methylation; oral squamous cell carcinoma; pyrosequencing

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Methylation profiling of cancer tissues has identified this mechanism as an important component of carcinogenesis. Epigenetic silencing of tumour suppressor genes through promoter methylation has been investigated by a variety of means, the most recent of which is pyrosequencing. We have investigated quantitative methylation status in oral squamous cell carcinoma patients. Fresh tumour tissue and normal control tissue from resection margin was obtained from 79 consecutive patients undergoing resection of oral squamous cell carcinoma. DNA was extracted and bisulphite treated. PCR primers were designed to amplify 75-200 bp regions of the CpG rich gene promoters of p16, RARb, E-cadherin, cytoglobin and cyclinAI. Methylation status of 4-5 CpG sites per gene was determined by pyrosequencing. Significant CpG methylation of gene promoters within tumour specimens was found in 28% for p16, 73% for RARb, 42% for E-cadherin, 65% for cytoglobin and 53% for cyclinAI. Promoter methylation was significantly elevated in tumours compared to normal tissue for p16 (P = 0.048), cytoglobin (P = 0.002) and cyclin AI (P = 0.001) but not in RARb (P = 0.088) or E-cadherin (P = 0.347). Concordant methylation was demonstrated in this tumour series (P = 0.03). Significant differences in degree of methylation of individual CpG sites were noted for all genes except RARb and these differences were in a characteristic pattern that was reproduced between tumour samples. Cyclin AI promoter methylation showed an inverse trend with histological grade. Promoter methylation analysis using pyrosequencing reveals valuable quantitative data from several CpG sites. In contrast to qualitative data generated from methylation specific PCR, our data demonstrated p16 promoter methylation in a highly tumour specific pattern. Significant tumour specific methylation of cyclin AI promoter was also seen. Cytoglobin is a novel candidate tumour suppressor gene highly methylated in upper aero-digestive tract squamous cancer.

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