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Methylation analysis of hMLH1 gene promoter by a bisulfite-sensitive single-strand conformation polymorphism–capillary electrophoresis method

✍ Scribed by Xianzhe Shi; Jianhua Li; Chunxia Zhao; Shen Lv; Guowang Xu


Publisher
John Wiley and Sons
Year
2006
Tongue
English
Weight
104 KB
Volume
20
Category
Article
ISSN
0269-3879

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✦ Synopsis


DNA methylation is an important epigenetic modification that alters transcription in those genes containing CpG islands. In this report, a novel DNA methylation analysis method was developed employing bisulfite-single strand conformation polymorphism combined with capillary electrophoresis (bisulfite-SSCP-CE). During the bisulfite treatment of genomic DNA, a high concentration of sodium bisulfite (4.8 mol/L) was preferred in order to shorten reaction time and minimize template degradation. The methylated and unmethylated ssDNA of hMLH1 promoter were simultaneously separated under the optimized CE conditions, including 6% SLPA with 10% glycerol as sieving medium, 25 degrees C as separation temperature and 12 kV as running voltage. The heterogeneous methylation of hMLH1 promoter was identified in 13 of 64 colorectal cancer patients. Moreover, hMLH1 promoter methylation had a significant relationship with protein expression loss and increased with the age of patients. Our results indicated that DNA methylation analysis for a large number of clinical samples would be facilitated by use of the bisulfite-SSCP-CE method.


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