The methylation status of PCDH8 was detected using primers specif

The methylation status of PCDH8 was detected using primers specific for PCDH8 unmethylated and methylated sequences respectively, as our reported previously [18]. The following primers were used: unmethylated:

forward 5’- GGTGGTTATTGGTTATTTGGTTT-3’ and reverse 5’- CCAACAAACTCTAAAAACACACA-3’; methylated: forward 5’- CGGTTATTGGTTATTCGGTTCC-3’ Apoptosis inhibitor and reverse 5’- ACGAACTCTAAAAACGCGCG -3’. The PCR amplification of the modified DNA consisted of one cycle of 95°C for 5 min, 40 cycles of 95°C for 30 s, 60°C for 30 s, and 72°C for 30 s, and 1 cycle of 72°C for 5 min. Water blanks were included with each assay, in vitro methylated DNA and unmethylated DNA (New England Biolabs, Beverly, MA, USA) was used as methylation and unmethylation positive control. PCR products were separated

in 2% agarose gel, stained with ethidium bromide, and visualized under ultraviolet illumination for analysis. Samples were scored as methylation positive when methylated alleles were present in the methylated DNA lane and methylation negative when bands were present only in the unmethylated DNA lane [18]. Statistical analysis Statistical analysis was conducted using SAS version 8.0 (SAS Institute, Cary, N.C., USA). Fisher’s exact test was used to assess the difference of PCDH8 methylation status between NMIBC patients and controls. Chi-square test was used to assess the relationship between PCDH8 methylation and clinicopathologic features. Kaplan-Meier survival analysis and log-rank test were SIS3 purchase used to assess the differences of recurrence-free survival, progression-free survival and this website five-year overall survival between patients with PCDH8 methylated and unmethylated. Multivariate Cox proportional hazard model analysis was used to assess the independent prognostic effect of PCDH8 methylation. A

two-sided p value < 0.05 was considered statistically significant. Results The methylation status of PCDH8 in NMIBC and normal bladder epithelial tissues In the current study, the methylation status of PCDH8 in NMIBC and normal bladder epithelial tissues was examined by MSP. We found that PCDH8 methylation occurred in 128 (54.9%) patients with NMIBC (Figure 1). However, no methylation was detected in controls, and the difference between these two groups was statistically AMP deaminase significant. The result is shown in Table 1. Figure 1 Representative MSP results for PCDH8 methylation in tumor-derived DNA samples from patients with NMIBC. W: water; P: positive control; N: negative control; M: methylated; U: unmethylated. Cases 71, 73 and 74 exhibited PCDH8 methylation. Case 72 exhibited PCDH8 unmethylation. Table 1 The methylation status of PCDH8 in NMIBC and normal bladder epithelial (NBE) tissues Group M (%) U (%) P NMIBC 128 (54.9) 105 (45.1) <0.0001 NBE 0 (0.0) 43 (100.0) M: Methylation; U: Unmethylation.

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