Figure 3.
Figure 3. Induction of γ-catenin by X-RARα (A) Sca1+/lin- stem cells transduced with PML/RARα, PLZF/RARα, or γ-catenin were transplanted into sublethally irradiated recipient mice. At day 10 after transplantation MNCs from the BM and the spleen were analyzed by Western blotting for the expression of X-RARα and γ-catenin. Another PML/RARα-positive animal that showed disease symptoms at day 12 after transplantation (PML/RARα-2) was included. The blots were first incubated with an anti-RARα antibody and after stripping with an anti-γ-catenin antibody. Equal protein loading was confirmed after further stripping of the membrane and staining with an anti-β-tubulin antibody. The corresponding bands are indicated. (B) Transactivation of the γ-catenin promoter by X-RARα and AML-1/ETO. The γ-catenin promoter construct was transfected by electroporation into U937 cells expressing the respective transgenes under the control of an Zn2+-inducible methallothionein 1 (MT-1) promoter. The pGL3basic was used as control. Twelve hours after transfection the transgene expression was induced by the exposure to 100 μM Zn2SO4, and luciferase expression was measured 24 hours later and normalized with Renilla activity. The average of triplicates of one representative of 3 independent experiments is given. (C) Effect of t-RA on the transactivation of the γ-catenin promoter by X-RARα and AML-1/ETO. Twelve hours after transfection the transgene expression was induced by the exposure to 100 μM Zn2SO4 for 4 hours prior to adding t-RA at a concentration of 10-6 M, and luciferase expression was measured 24 hours later. The average of triplicates of one representative of 3 independent experiments is given.

Induction of γ-catenin by X-RARα (A) Sca1+/lin- stem cells transduced with PML/RARα, PLZF/RARα, or γ-catenin were transplanted into sublethally irradiated recipient mice. At day 10 after transplantation MNCs from the BM and the spleen were analyzed by Western blotting for the expression of X-RARα and γ-catenin. Another PML/RARα-positive animal that showed disease symptoms at day 12 after transplantation (PML/RARα-2) was included. The blots were first incubated with an anti-RARα antibody and after stripping with an anti-γ-catenin antibody. Equal protein loading was confirmed after further stripping of the membrane and staining with an anti-β-tubulin antibody. The corresponding bands are indicated. (B) Transactivation of the γ-catenin promoter by X-RARα and AML-1/ETO. The γ-catenin promoter construct was transfected by electroporation into U937 cells expressing the respective transgenes under the control of an Zn2+-inducible methallothionein 1 (MT-1) promoter. The pGL3basic was used as control. Twelve hours after transfection the transgene expression was induced by the exposure to 100 μM Zn2SO4, and luciferase expression was measured 24 hours later and normalized with Renilla activity. The average of triplicates of one representative of 3 independent experiments is given. (C) Effect of t-RA on the transactivation of the γ-catenin promoter by X-RARα and AML-1/ETO. Twelve hours after transfection the transgene expression was induced by the exposure to 100 μM Zn2SO4 for 4 hours prior to adding t-RA at a concentration of 10-6 M, and luciferase expression was measured 24 hours later. The average of triplicates of one representative of 3 independent experiments is given.

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