Genome-wide profiling of promoter methylation in human

被引:0
|
作者
I Hatada
M Fukasawa
M Kimura
S Morita
K Yamada
T Yoshikawa
S Yamanaka
C Endo
A Sakurada
M Sato
T Kondo
A Horii
T Ushijima
H Sasaki
机构
[1] Laboratory of Genome Science,Department of Molecular and Cellular Biology
[2] Biosignal Genome Resource Center,Department of Thoracic Surgery
[3] Gunma University,Department of Molecular Pathology
[4] PRESTO,Carcinogenesis Division
[5] Japan Science and Technology Corporation (JST),Division of Human Genetics, Department of Integrated Genetics
[6] Laboratory for Molecular Psychiatry,Department of Genetics
[7] RIKEN Brain Science Institute,undefined
[8] Institute of Development,undefined
[9] Aging and Cancer,undefined
[10] Tohoku University,undefined
[11] Tohoku University School of Medicine,undefined
[12] National Cancer Center Research Institute,undefined
[13] National Institute of Genetics,undefined
[14] Research Organization of Information and Systems,undefined
[15] School of Life Science,undefined
[16] Graduate University for Advanced Studies,undefined
来源
Oncogene | 2006年 / 25卷
关键词
DNA methylation; genome-wide profiling; epigenetics; microarray;
D O I
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中图分类号
学科分类号
摘要
DNA methylation in the promoter region of a gene is associated with a loss of that gene's expression and plays an important role in gene silencing. The inactivation of tumor-suppressor genes by aberrant methylation in the promoter region is well recognized in carcinogenesis. However, there has been little study in this area when it comes to genome-wide profiling of the promoter methylation. Here, we developed a genome-wide profiling method called Microarray-based Integrated Analysis of Methylation by Isoschizomers to analyse the DNA methylation of promoter regions of 8091 human genes. With this method, resistance to both the methylation-sensitive restriction enzyme HpaII and the methylation-insensitive isoschizomer MspI was compared between samples by using a microarray with promoter regions of the 8091 genes. The reliability of the difference in HpaII resistance was judged using the difference in MspI resistance. We demonstrated the utility of this method by finding epigenetic mutations in cancer. Aberrant hypermethylation is known to inactivate tumour suppressor genes. Using this method, we found that frequency of the aberrant promoter hypermethylation in cancer is higher than previously hypothesized. Aberrant hypomethylation is known to induce activation of oncogenes in cancer. Genome-wide analysis of hypomethylated promoter sequences in cancer demonstrated low CG/GC ratio of these sequences, suggesting that CpG-poor genes are sensitive to demethylation activity in cancer.
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页码:3059 / 3064
页数:5
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