0 (ABI) Figure 1A illustrates the structure of the SPARC gene an

0 (ABI). Figure 1A illustrates the structure of the SPARC gene and the topology of the BSP primer, indicating the Apoptosis inhibitor position of the CpG island containing 12 CpG sites and the BSP primers. Figure 1 Detection of SPARC gene TRR methylation. GSK690693 cell line (A) Illustration of the SPARC gene TRR and topology of the BSP primer. The black bar indicates the analyzed region. The bold “”G”" indicates the transcriptional start site. The bold italic “”CG”" indicates the location of 12 CpG island sites. The underlined sequence indicates the primers for BSP. Blue and red rectangles indicate the Sp1 and

AP1 binding consensus sequences, respectively. The red triangles indicate the region whose representative sequence analyses were

showed in Figure 1B. (B) Representative sequencing data of the SPARC gene TRR in four different groups of pancreatic tissues obtained using BSP PCR-based sequencing analysis. CpG dinucleotides see more “”C”" in the objective sequence are shown in red. The red, yellow, green, light blue, and deep blue dots under the analyzed sequence represent different methylation ratios, respectively. We next performed BSP PCR-based sequencing analysis to assess the methylation status of the SPARC gene TRR in four tissue groups: 40 pancreatic cancer samples and their corresponding adjacent normal pancreatic tissues, 6 chronic pancreatitis samples, and 6 real normal pancreatic tissue samples. Figure 1B shows representative BSP PCR-based sequencing analysis results for these four different groups of pancreatic tissues. The methylation pattern of the SPARC gene TRR in these four types of pancreatic tissues

is shown in Figure 2. According to the curve fitted to the mean percent methylation of pancreatic cancer tissue data by the MACD (moving average convergence/divergence) method, we found two hypermethylation wave peak regions in these CpG Demeclocycline islands. The first contained CpG site 1-7 (CpG Region 1) and the second contained CpG sites 8-12 (CpG Region 2). We searched the web site http://​www.​cbrc.​jp/​research/​db/​TFSEARCH.​html and found that CpG Region 1 contained two Sp1 sites while CpG Region 2 contained one Ap1 site (Figure 1A). Figure 3 shows the mean percentage of gene methylation and the 95% CI of these two hypermethylation wave peak regions in the four types of pancreatic tissues. Methylation of these two regions appeared to gradually increase from normal, chronic pancreatitis, and adjacent normal to pancreatic cancer tissues. Furthermore, CpG Region 2 was rarely methylated in real normal pancreatic tissues but CpG Region 1 was more frequently methylated in some of normal tissues. In addition, the methylation level of CpG Region 2 in the adjacent normal tissues was significantly increased compared with the normal tissues.

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