Regulation of DEK expression by AP-2α and methylation level of DEK promoter in hepatocellular carcinoma.

Oncol Rep

College of Life Sciences and Bioengineering, School of Science, Beijing Jiaotong University, Beijing 100044, P.R. China.

Published: October 2016

AI Article Synopsis

  • - DEK is found to be overexpressed in various invasive tumors, but the ways it is regulated at the genetic level remain unclear.
  • - The study identifies the DEK core promoter region, showing that its methylation affects DEK expression, especially comparing levels in normal liver cells versus hepatocellular carcinoma (HCC) cells.
  • - AP-2α is highlighted as a crucial transcription factor for DEK expression, with its binding influenced by methylation, and experiments show that altering AP-2α levels significantly affects DEK activity.

Article Abstract

DEK is overexpressed in multiple invasive tumors. However, the transcriptional regulatory mechanism of DEK remains unclear. In the present study, progressive-type truncation assay indicated that CpG2-2 (-167 bp/+35 bp) was the DEK core promoter, whose methylation inhibited DEK expression. Bisulfite genomic sequencing analysis indicated that the methylation levels of the DEK promoter in normal hepatic cells and tissues were higher than those in hepatocellular carcinoma (HCC) cells. TFSEARCH result revealed transcription factor binding sites in CpG2-2. Among the sites, the AP-2α binding site showed the most significant methylation difference; hence, AP-2α is a key transcription factor that regulates DEK expression. Point or deletion mutation of the AP-2α binding site significantly reduced the promoter activity. Chromatin immunoprecipitation assay demonstrated the binding of AP-2α to the core promoter. Furthermore, knock down of endogenous AP-2α downregulated DEK expression, whereas overexpression of AP-2α upregulated DEK expression. Thus, AP-2α is an important transcription factor of DEK expression, which is correlated with the methylation level of the DEK core promoter in HCC.

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Source
http://dx.doi.org/10.3892/or.2016.4984DOI Listing

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