| Literature DB >> 19816938 |
Masashi Kusakabe1, Tomoko Kutomi2, Kousuke Watanabe2, Noriko Emoto2, Naomi Aki2, Hidenori Kage3, Emi Hamano2, Hiroshi Kitagawa2, Takahide Nagase2, Atsushi Sano1, Yukihiro Yoshida1, Takeshi Fukami1, Tomohiro Murakawa1, Jun Nakajima1, Shinichi Takamoto1, Satoshi Ota4, Masashi Fukayama4, Yutaka Yatomi3, Nobuya Ohishi2, Daiya Takai3.
Abstract
Epigenetic changes can lead to abnormal expression of genes in cancer, and several genes have been reported to have aberrant promoter DNA methylation in non-small-cell lung cancer (NSCLC). We identified aberrantly methylated genes in NSCLC by combination of in silico and experimental approaches. We first applied bioinformatics, and from microarray datasets, we selected genes with low expression and having functions related to cancer. Next, combined bisulfite restriction analysis was carried out in 10 pooled resected lung cancer tissues to screen for genes that were aberrantly methylated, and the methylation ratio (the fraction of methylated DNA in extracted DNA from a cancer tissue sample) was quantified using quantitative analysis of methylated alleles. We identified 8 methylated genes (ARPC1B, DNAH9, FLRT2, G0S2, IRS2, PKP1, SPOCK1 and UCHL1) previously unreported in NSCLC. Analyses of methylation profiles of 101 resected lung cancer tissue samples revealed quantitatively low methylation in whole, methylation ratios were almost less than 30% even in the methylated samples, and no significant correlation to prognosis after 2 years of follow-up using hierarchical clustering. DNA methylation of G0S2 gene was significantly more frequent in squamous lung cancer (n = 18, mean of methylation ratios: 15%) compared with nonsquamous lung cancer (n = 83, mean of methylation ratios: 2.6%) (Mann-Whitney U test, p < 0.001). DNA methylation of G0S2 can be an important biomarker for squamous lung cancer.Entities:
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Year: 2010 PMID: 19816938 DOI: 10.1002/ijc.24947
Source DB: PubMed Journal: Int J Cancer ISSN: 0020-7136 Impact factor: 7.396