Figure 1
Figure 1. Inhibition of Bcr-abl activity in CML cells augments cellular responses to IFNα. (A) Viability of KT1 cells that received indicated shRNA and were treated with IM (0.5μM for 8 hours), IFNα (250 IU/mL for 8 hours), or a combination (4 hours + 4 hours) of the 2 as indicated. (B) Viability of KU812 cells that received indicated shRNA and were treated as described in panel A. (C) KT1 cells were pretreated with IM (0.5μM) for 8 hours and then treated with IFNα (250 IU/mL) for 30 minutes. Activation and total levels of STAT1 was analyzed in whole cell lysates by immunoblotting using the indicated antibodies. (D) KT1 cells were pretreated with IM (0.5μM) for 8 hours and then treated with IFNα (250 IU/mL) or IFNγ (50 IU/mL) for 30 minutes. Activation and total levels of STAT1 was analyzed in whole cell lysates by immunoblotting using the indicated antibodies.

Inhibition of Bcr-abl activity in CML cells augments cellular responses to IFNα. (A) Viability of KT1 cells that received indicated shRNA and were treated with IM (0.5μM for 8 hours), IFNα (250 IU/mL for 8 hours), or a combination (4 hours + 4 hours) of the 2 as indicated. (B) Viability of KU812 cells that received indicated shRNA and were treated as described in panel A. (C) KT1 cells were pretreated with IM (0.5μM) for 8 hours and then treated with IFNα (250 IU/mL) for 30 minutes. Activation and total levels of STAT1 was analyzed in whole cell lysates by immunoblotting using the indicated antibodies. (D) KT1 cells were pretreated with IM (0.5μM) for 8 hours and then treated with IFNα (250 IU/mL) or IFNγ (50 IU/mL) for 30 minutes. Activation and total levels of STAT1 was analyzed in whole cell lysates by immunoblotting using the indicated antibodies.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal