Abstract
BackgroundAlu methylation is correlated with the overall level of DNA methylation and recombination activity of the genome. However, the maintenance and methylation status of each CpG site within Alu elements (Alu) and its methylation status have not well characterized. This information is useful for understanding natural status of Alu in the genome and helpful for developing an optimal assay to quantify Alu hypomethylation.MethodsBisulfite clone sequencing was carried out in 14 human gastric samples initially. A Cac8I COBRA-DHPLC assay was developed to detect methylated-Alu proportion in cell lines and 48 paired gastric carcinomas and 55 gastritis samples. DHPLC data were statistically interpreted using SPSS version 16.0.ResultsFrom the results of 427 Alu bisulfite clone sequences, we found that only 27.2% of CpG sites within Alu elements were preserved (4.6 of 17 analyzed CpGs, A ~ Q) and that 86.6% of remaining-CpGs were methylated. Deamination was the main reason for low preservation of methylation targets. A high correlation coefficient of methylation was observed between Alu clones and CpG site J (0.963), A (0.950), H (0.946), D (0.945). Comethylation of the sites H and J were used as an indicator of the proportion of methylated-Alu in a Cac8I COBRA-DHPLC assay. Validation studies showed that hypermethylation or hypomethylation of Alu elements in human cell lines could be detected sensitively by the assay after treatment with 5-aza-dC and M.SssI, respectively. The proportion of methylated-Alu copies in gastric carcinomas (3.01%) was significantly lower than that in the corresponding normal samples (3.19%) and gastritis biopsies (3.23%).ConclusionsMost Alu CpG sites are deaminated in the genome. 27% of Alu CpG sites represented in our amplification products. 87% of the remaining CpG sites are methylated. Alu hypomethylation in primary gastric carcinomas could be detected with the Cac8I COBRA-DHPLC assay quantitatively.
Highlights
Alu methylation is correlated with the overall level of DNA methylation and recombination activity of the genome
Total methylation content of Alu elements and LINE-1 sequences is highly correlated with global DNA methylation content [12]
A significant difference of CpG retention rate was observed at the site L between gastric carcinoma (GC)-Nor and normal control samples (P = 0.022)
Summary
Alu methylation is correlated with the overall level of DNA methylation and recombination activity of the genome. The maintenance and methylation status of each CpG site within Alu elements (Alu) and its methylation status have not well characterized. The Alu element is a member of the SINE family of repetitive elements It is an example of a non-automatic retrotransposon. Alu elements are mainly distributed in gene-rich regions. A consensus Alu element usually contains 24 CpG sites (Figure 1) [3]. Demethylation of Alu elements is an indicator of lower genome stability, which is necessary for gene recombination and chromosome translocation [10]. Total methylation content of Alu elements and LINE-1 sequences is highly correlated with global DNA methylation content [12]. Estimation of total methylation content of Alu elements is useful for evaluation of the global genomic methylation status and level of homologous and non-homologous chromatin recombination in gene-rich regions
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