RiPA correctly predicts suitability of E3 ligases for WDR5 PROTACs
(A) Immunoblot of WDR5, VHL, and CRBN. HEK293 cells were transfected with WDR5-Luc-FKBP12 and VHL-FRB or CRBN-FRB or FRB in a 1:10 ratio, expressed for 24 hr, and treated with 10 nM rapamycin for 6 hr.
(B) WDR5 levels based on luciferase measurement. Luminescence was measured in HEK293 cells as described in (A) after 10 nM rapamycin treatment at specified time points. Data represent mean ± s.d. of n=3 replicates.
(C) Immunoblot of AURKA, VHL and CRBN. HEK293 cells were transfected with AURKA-Luc-FKBP12 and VHL-FRB or CRBN-FRB or FRB in a 1:10 ratio and treated with 10 nM rapamycin for 6 hr.
(D) AURKA levels based on luciferase measurement. Luminescence was measured in HEK293 cells as described in (C) after 10 nM rapamycin treatment at indicated time points. Data represent mean ± s.d. of n=3 replicates.
(E) Structure of FKBP12 and luciferase. Molecular surface representation of FKBP12 (top) and luciferase (bottom) showing lysine residues on their surface. The lysine residues are labelled and two sides for each protein are shown.
(F) WDR5 levels based on luciferase measurement. HEK293 cells were co-transfected with either WDR5-Luc-FKBP12 (WT) or WDR5-Luc-FKBP12 construct where all lysine residues on Luc and FKBP12 were mutated to arginine (K-less) and FRB, expressed for ∼24 hr and luminescence measured. Bars represent mean ± s.d. of n=3 replicates.
(G) WDR5 levels based on luciferase measurement. Luminescence was measured in HEK293 cells expressing WDR5-Luc-FKBP12 (K-less) and VHL-FRB or CRBN-FRB or FRB after 10 nM rapamycin treatment at specified time points. Data represent mean ± s.d. of n=3 replicates.
(H) KRASG12D levels based on luciferase measurements. HEK293 cells were co-transfected with KRASG12D-Luc-FKBP12 (K-less) and VHL-FRB or FRB constructs, expressed for ∼24 hr, and treated with 10 nM rapamycin (Rapa.) in the presence or absence of 10 µM MG132 and 5 µM MLN4924 for 8 hr. Bars represent mean ± s.d. of n=2 replicates.