Figure 3.
Figure 3. Tyrosine dephosphorylation of p27Kip1 alters the binding to cdks. (A) NB4 cells were stimulated with G-CSF and harvested at different time points. Immunoprecipitations with cdk2 and cdk4 were performed and probed by Western blotting with antibodies as indicated. A total of 50 or 100 μg NB4 lysate from untreated cells was also loaded as a control. (B) p27Kip1 immunoprecipitate from NB4 lysate was incubated with LAR-PTP. The Western blot was probed with antibodies to cdk4 and p27Kip1. Binding of cdk4 to p27Kip1 (treated with LAR-PTP or untreated) was detected. (C) GST-p27Kip1 fusion proteins (p27Kip1 wt and tyrosine to phenylalanine mutations Y74F, Y88F, Y89F, Y88/89F, Y74/88/89F) were expressed in E coli strains DH5α (pTyr -: not tyrosine-phosphorylated) and TKX1 (pTyr +: tyrosine-phosphorylated). After incubation of the fusion proteins in NB4 lysate together with GSH agarose for 15 minutes at 4°C, the protein complexes were separated by PAGE and blotted and binding of the p27Kip1 wt or point mutations with cdk2 and cdk4 was evaluated by detection with the appropriate antibodies. (D) Plasmids containing p27Kip1 wt sequence as well as point mutations (with or without Abl-PP sequence) were transiently expressed in NIH/3T3 cells. p27Kip1 immunoprecipitations were performed and probed with antibodies as indicated. As control for Abl-PP expression, a total of 100 μg lysate was also detected. (E) Lysate from transfected NIH/3T3 cells was immunoprecipitated and probed as indicated.

Tyrosine dephosphorylation of p27Kip1 alters the binding to cdks. (A) NB4 cells were stimulated with G-CSF and harvested at different time points. Immunoprecipitations with cdk2 and cdk4 were performed and probed by Western blotting with antibodies as indicated. A total of 50 or 100 μg NB4 lysate from untreated cells was also loaded as a control. (B) p27Kip1 immunoprecipitate from NB4 lysate was incubated with LAR-PTP. The Western blot was probed with antibodies to cdk4 and p27Kip1. Binding of cdk4 to p27Kip1 (treated with LAR-PTP or untreated) was detected. (C) GST-p27Kip1 fusion proteins (p27Kip1 wt and tyrosine to phenylalanine mutations Y74F, Y88F, Y89F, Y88/89F, Y74/88/89F) were expressed in E coli strains DH5α (pTyr -: not tyrosine-phosphorylated) and TKX1 (pTyr +: tyrosine-phosphorylated). After incubation of the fusion proteins in NB4 lysate together with GSH agarose for 15 minutes at 4°C, the protein complexes were separated by PAGE and blotted and binding of the p27Kip1 wt or point mutations with cdk2 and cdk4 was evaluated by detection with the appropriate antibodies. (D) Plasmids containing p27Kip1 wt sequence as well as point mutations (with or without Abl-PP sequence) were transiently expressed in NIH/3T3 cells. p27Kip1 immunoprecipitations were performed and probed with antibodies as indicated. As control for Abl-PP expression, a total of 100 μg lysate was also detected. (E) Lysate from transfected NIH/3T3 cells was immunoprecipitated and probed as indicated.

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