d eluted. Eluted DNA can be used for e-book downstream applications ChIP PCR. Fold enrichment was calculated by using a ratio of amplifi cation efficiency of the ChIP sample over that of non immune IgG. Amplification efficiency of Polymerase RNA II was used as a positive control. FE% 2 100%. Cell proliferation assay A cell proliferation assay was performed using the Cell Counting Kit 8 according to the manufacturers instructions. Before the addition of CCK 8, the cells were washed with warm culture media by spinning the plate at 500 rpm for 3 m and then dis carding the supernatant. Cell apoptosis Inhibitors,Modulators,Libraries assay The cancer cells were harvested and resuspended in 500 ul of a binding buffer. The cell suspension was incubated with 5 ul anne in V and propidium iodide at room temperature for 20 minutes.
Inhibitors,Modulators,Libraries The stained cells were analyzed with fluorescent activated cell sorting using BD LSR II flow cytometry. Cell cycle analysis For the flow cytometry analysis, cells were trypsinized and fi ed in 70% ethanol overnight. The cells were then incubated in 0. 5 ml of propidium iodide solution con taining 25 ug ml?1 RNase for 15 minutes at 37 C and measured. Mouse e periments The NCI N87 cells were injected into the right flanks of athymic nu nu mice. One week after the injec tions, mice with comparably sized tumors were treated for 4 weeks with anti miR 425. The anti miR 425 were Inhibitors,Modulators,Libraries injected directly into the tumors twice weekly for 4 weeks. Statistical Inhibitors,Modulators,Libraries analysis The results are presented as means SEM, and the data were analyzed with Students t test. A value of p 0. 05 was considered statistically significant.
Results IL 1B treatment induces miR 425 e pression To characterize the miRNAs responsible for IL 1B in duction, we profiled miRNA e pression in PBS treated AGS cells and IL 1B induced AGS cells using the E iqon miRCURY Cilengitide LNA Array System. The miRNA levels differed greatly between the PBS treated group and the IL 1B induced group, as illustrated in the heat map shown in Figure 1A. Among the 1,891 capture probes, 46 miRNAs were differentially e pressed in IL 1B induced AGS cells compared with paired PBS treated AGS cells. of these miRNAs, 29 were increased and 17 were decreased in the IL 1B induced AGS cells, indicating that a specific miRNA pattern is associated with IL 1B induction. Among these miRNAs, miR 425 was the most highly upregulated upon IL 1B induction.
Using real time PCR analysis, we analyzed miR 425 e pression in 36 paired samples. We found a significantly higher level of miR 425 e pression in the tumor samples relative to the levels in the adjacent normal tissues. We e amined the e pression 17-AAG supplier level of miR 425 in a set of gastric cancer cell lines and si normal gas tric mucosa cells. As shown in Figure 1C, we picked up the AGS cells with down regulated miR 425 and the NCI N87 cells with up regulated miR 425 for further study. Although the activation of miR 425 has been reported to have a fundamental impact on cancer initi ation and progression of cancer cells by red