Finally, procaspase 3, an executioner caspase, and PARP, a hallmark of caspase activation, were cleaved profoundly in CEM/VLB100 cells compared with CEM cells. Meanwhile, we investigated whether the modulation of www.selleckchem.com/products/ganetespib-sta-9090.html Bcl 2 family proteins is involved in TRAIL induced apoptosis of MDR cells. Down regulation Inhibitors,Modulators,Libraries of Bcl 2 and up regulation of Bax apparently occurred after treatment with TRAIL in CEM/VLB100 cells but not in CEM cells and these results were followed by TRAIL induced trun cation of Bid in CEM/VLB100 cells but not in CEM cells, consistent with activation status of procaspase 9 in CEM/VLB100 cells and CEM cells after treatment with TRAIL. Therefore, these data indicated that TRAIL induces apoptosis occurred in the MDR cells through caspase dependent mitochondrial pathway as well as receptor mediated apoptotic pathway.
The increased expression of DNA PKcs is associated with up regulation of P gp and c Myc expression via Akt/GSK 3b pathway in MDR cells It has been reported DNA PKcs regulates c Myc stabi lity via phosphorylation of Akt on Ser473, which in turn inactivates GSK 3b by the phosphorylation of GSK 3b on Ser9, resulting in stabilization of c Myc. The c Myc is known to be involved in regulating Inhibitors,Modulators,Libraries expression of P gp, the product of MDR1 gene and renders cells sensitive to TRAIL induced apoptosis. Since the increased activity of DNA PK participates in the development of MDR phenotype, we determined the relationships among P gp, c Myc and DNA PKcs/ Akt/GSK 3b molecules in MDR variants.
We found that the gradually increased level of P gp in CEM/VLB10 2, CEM/VLB55 8 and CEM/VLB100 Inhibitors,Modulators,Libraries cells was well correlated with the level of c Myc in the each MDR variant. Therefore, we examined whether the basal levels of DNA PKcs, phosphorylated Akt and phos phorylated GSK 3b in MDR variants were compared with those in parental CEM cells. The basal level of DNA PKcs was gradually higher in CEM/VLB10 2, CEM/VLB55 8 and CEM/VLB100 cells than in CEM cells, which was followed by gradual increase in pAkt and pGSK 3b levels without change Inhibitors,Modulators,Libraries in total Akt and GSK 3a/b levels. We also observed that the basal level of DR5 but not DR4 in MDR variants was signifi cantly increased as compared with those in CEM cells. These results suggested that the increased expression of DNA PKcs in MDR cells might lead to up regulation of P gp Inhibitors,Modulators,Libraries and c Myc expression via phosphorylation of Akt and GSK 3b proteins.
TRAIL induced down regulation of DNA PKcs/Akt/GSK 3b pathway and c FLIP and up regulation of DR4/DR5 cell surface expression are associated with the susceptibility to TRAIL of MDR cells Since our data showed that the level of DR5 was selleckchem well correlated with the activity of the DNA PKcs/Akt/GSK 3b pathway in MDR cells, we determined whether the levels of DNA PKcs, Akt as a downstream target of DNA PKcs, and GSK 3b, a downstream target of the Akt pathway, are modulated after treatment of CEM and CEM/VLB100 cells with TRAIL.