Figure 1
Figure 1. Cdk1 and cdk6 phosphorylate RUNX1 on S48 and S424 in vitro. (A) Diagram of RUNX1 showing its 3 cdk consensus phosphorylation sites. (B) In vitro kinase assay in which cdk1/cyclin B1 (left panel) or cdk6/cyclin D3 (right panel) were incubated with γ-ATP and GST-RUNX1 fusion proteins containing the RUNX1 amino acid segments 28-290, 290-480, and 290-480 with the S424A mutation, or the 86-217 Runt domain, GST alone, or GST-Rb protein (2 μg), followed by polyacrylamide gel electrophoresis, drying, and autoradiography. (C) In vitro kinase assays (top panels) using the indicated cdk/cyclin complexes and GST-RUNX1 fusion proteins 320-480, 320-480/S424A, 410-480, 410-480/S424A, 27-86, 27-86/T41A, 27-86/S48A, 27-86/T41A/S48A, or GST-Rb. Results are representative of 2 independent assessments for GST-RUNX1(410-480) and its S424A variant and 4 assessments for GST-RUNX1(28-86) and its 3 variants, with the data shown for the right 3 panels from the same experiment run on the same gel (Rb lanes are juxtaposed). Asterisks (*) indicate locations of relevant phosphorylated fragments. Equal volumes of bacterial lysates used for this experiment were also subjected to Western blotting using GST antibody (bottom panels).

Cdk1 and cdk6 phosphorylate RUNX1 on S48 and S424 in vitro. (A) Diagram of RUNX1 showing its 3 cdk consensus phosphorylation sites. (B) In vitro kinase assay in which cdk1/cyclin B1 (left panel) or cdk6/cyclin D3 (right panel) were incubated with γ-ATP and GST-RUNX1 fusion proteins containing the RUNX1 amino acid segments 28-290, 290-480, and 290-480 with the S424A mutation, or the 86-217 Runt domain, GST alone, or GST-Rb protein (2 μg), followed by polyacrylamide gel electrophoresis, drying, and autoradiography. (C) In vitro kinase assays (top panels) using the indicated cdk/cyclin complexes and GST-RUNX1 fusion proteins 320-480, 320-480/S424A, 410-480, 410-480/S424A, 27-86, 27-86/T41A, 27-86/S48A, 27-86/T41A/S48A, or GST-Rb. Results are representative of 2 independent assessments for GST-RUNX1(410-480) and its S424A variant and 4 assessments for GST-RUNX1(28-86) and its 3 variants, with the data shown for the right 3 panels from the same experiment run on the same gel (Rb lanes are juxtaposed). Asterisks (*) indicate locations of relevant phosphorylated fragments. Equal volumes of bacterial lysates used for this experiment were also subjected to Western blotting using GST antibody (bottom panels).

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