Genomic DNAs from 64 H. pylori strains isolated from

22 gastric cancer patients and 42 superficial gastritis patients were used for screening cancer-specific genes. PCR primers corresponding to cancer-specific or superficial gastritis-specific genes (see Tables 1 and 2) were designed using primerpremier 5.0. PCR was performed in a volume of 20 μL containing 10 pM of primer, 0.5 μg genomic DNA, 2.5 mM dNTPs (Takara Company) and 2.5 U of Taq DNA polymerase selleck chemicals llc (Takara Company). PCR were performed at 25 cycles in T gradient PCR thermal cycler (Biometra Co., Germany). The amplified PCR products were resolved in 2% agarose gels containing 0.5 × TBE, stained with ethidium bromide and visualized under a short-wavelength UV light. All analyses were performed using spss for Windows version 12.0. The frequency distribution of GC-specific genes in GC and NGC patients was analyzed using χ2 test. P<0.05 was considered statistically

this website significant. In this study, we used a well-established SSH method (Diatchenko et al., 1996; Akopyants et al., 1998) in an attempt to assess the differences in gene content between gastric cancer-associated H. pylori strain and superficial gastritis-associated strain. To detect genes specific to gastric cancer, L301 H. pylori strain, which was isolated from a gastric cancer patient, was used as the tester and B975 strain, which was isolated from a superficial gastritis patient, was used as the driver. DNA fragments recovered after subtractive hybridization were PCR amplified and cloned into pMD19-T plasmid. About 300 colonies grew on ampicillin plates. Among these, 152 colonies were randomly selected and used as a high-copy library for the gastric cancer strain (H library). Conversely, to Sclareol detect genes that were less abundant or absent in gastric cancer strain, B975 strain was used as the tester and L301 strain was used as the driver. One hundred and sixty colonies were randomly selected

and used as a low-copy library for the gastric cancer strain (L library). Inserts from either H or L libraries were amplified using the primers NP1 and NP2. Electrophoresis analysis of the PCR products revealed that the size of the subtractive fragments ranged from 200 to 1000 bp, suggesting that both high-copy and low-copy of gastric cancer-associated H. pylori DNA libraries were successfully generated, respectively. To detect H. pylori genes specific to gastric cancer, PCR products of the H library inserts were arrayed on nylon membranes and hybridized with either DIG-labeled L301 or B975 digested DNAs (data not shown). Twelve positive clones of gastric cancer-specific DNAs present in all three replicates were selected and sequenced. Homology analysis reveals that the cancer-specific genes belong to several functional groups (Table 1).