However BC after the administration of FG020326. However, at the same time, paclitaxel and doxorubicin were almost completely Constantly degraded. This suggested that FG020326 k Nnte the concentration that would be reversed strong hold on MDR in vivo and long enough to the action of chemotherapeutic agents used in usual doses to Nacktm Nozzles achieve xenograft treat improvement. 3.4. FG020236 effect on BTZ043 the activity of t Human hepatic CYP 3A4 Many reports indicate that there are significant overlaps in tissue distribution and substrate Pr difference Between ABCB1 and CYP3A4. To determine whether MDR modulator FG020326 go Rt to the third generation, we have found. Their effects on human liver microsomal CYP3A4 in vitro Troleandomycin, a potent CYP3A4 inhibitor, inhibited the activity t of CYP3A4 in a concentration dependent-Dependent manner.
Only FG020326 produced a significant inhibition of CYP3A4 to 25 million, the h significantly from Than necessary to reverse MDR in vitro. 3.5. FG020326 effect on the pharmacokinetics of paclitaxel to M usen FG020236 The effect on the pharmacokinetic profile of paclitaxel Hesperadin is shown in Figure 2B. The administration of FG020236 not significantly change Plasma concentrations of paclitaxel compared with animals treated with vehicle. There was no significant difference in the pharmacokinetic parameters of paclitaxel usen between a vehicle and treated FG020236 M. These results suggest that FG020326 had no apparent effect on the pharmacokinetics of paclitaxel. 3.6.
FG020326 effect on intracellular Re accumulation of Dox fundamental experiments showed that the intracellular Re accumulation in cells of Dox only KBv200 was about a quarter of that of KB cells. Were exposed to KBv200 and KB cells to 0.625, 1.25, 2.5, 5 or 10 M FG020326, Dox enrichment significantly in cells KBv200 1.4, 2.1, 2.6 was improved, 3,0 and 3 0.7-fold for the. However, in the cells of the drug-sensitive KB FG020236 has not substantially ver Change the intracellular Re accumulation of Dox. Subsequently End we performed experiments to determine whether the increased Hte accumulation of Dox in the cells by KBv200 FG020326 caused by inhibition of the efflux is Dox. The temporal evolution of Dox efflux after 2 h of accumulation is shown in Figure 3B. KBv200 cells released a significantly h Heren percentage of accumulated intracellularly Ren Dox compared to KB cells.
For example, 30 minutes, 58 of the accumulated effluxed Dox KBv200 of cells, compared with only 28 of KB cells. FG020326 fa inhibited It significant efflux of Dox KBv200 cells, KB-cells are not. Incubation of cells with KBv200 1.25, 2.5 or 5 M 2 h FG020326 significantly increased Ht Rho 123 accumulation in a dose-dependent-Dependent manner. However, the accumulation of Rho 123 KB cells sensitive drugs is not significantly changed by the addition of FG020326 ver. 3.7. Photolabeling of ABCB1 with azidopine, dosage ATPase ABCB1, ABCB1 expression and localization of FG