Abstract
A common single-nucleotide polymorphism in the telomerase reverse transcriptase (TERT) promoter, rs2853669 influences patient survival rates and the risk of developing cancer. Recently, several lines of evidence suggest that the rs2853669 suppresses TERT promoter mutation-mediated TERT expression levels and cancer mortality as well as recurrence rates. However, no reports are available on the impact of rs2853669 on TERT expression in hepatocellular carcinoma (HCC) and its association with patient survival. Here, we found that HCC-related overall and recurrence-free survival rates were not associated with TERT promoter mutation individually, but rs2853669 and the TERT promoter mutation in combination were associated with poor survival rates. TERT mRNA expression and telomere fluorescence levels were greater in patients with HCC who had both the combination. The combination caused TERT promoter methylation through regulating the binding of DNA methyltransferase 1 and histone deacetylase 1 to the TERT promoter in HCC cell lines. The TERT expression level was significantly higher in HCC tumor with a methylated promoter than in that with an unmethylated promoter. In conclusion, we demonstrate a substantial role for the rs2853669 in HCC with TERT promoter mutation, which suggests that the combination of the rs2853669 and the mutation indicate poor prognoses in liver cancer.
Highlights
For measurement of telomere fluorescence levels, 93 surgically resected paraffin-embedded HCC tumor tissue samples and corresponding non-tumorous liver tissue samples were analyzed
The TERT promoter methylation levels were determined by methylation specific quantitative PCR (MSqPCR) as previously described [10,11,12] with certain modifications
Methylation levels of the TERT promoter were calculated as the fraction of methylated molecules in the total methylated and unmethylated DNA, which was described in a previous report [10, 11]
Summary
For measurement of telomere fluorescence levels, 93 surgically resected paraffin-embedded HCC tumor tissue samples and corresponding non-tumorous liver tissue samples were analyzed. The TERT promoter containing rs2853669 (-245T) [4], -124C [5], and -146C [5] (chr5: 1,295,349; chr5: 1,295,228; chr5: 1,295,250, respectively; hg19 assembly) was amplified using hTaq polymerase (Solgent, Daejeon, Korea) with 10 ng of genomic DNA containing each primer (forward primer: GGCCGATTCGACCTCTCT; reverse primer: AGCACCTCGCGGTAGTGG) [6]. After purification of a 489 bp PCR-amplified product with the NucleoSpin DNA Clean-up Kit (Macherey-Nagel, Düren, Germany; 740609.250), the TERT promoter region was analyzed by Sanger sequencing (Macrogen, Seoul, Korea).
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