Figure 4.
sTFR1 is a carrier protein for mutant CALR. (A) Allele burden and mutation profile of patients included in this study the analysis. (B) Identification of partners of plasmatic mutant CALR. Plasma from 5 patients with mutated CALR and 5 healthy controls was isolated by IP with biotinylated antimutant CALR antibody. Immunoblot shows the presence of mutant CALR in the IP product detected with a different antimutant CALR antibody. The IP product was analyzed by nontargeted MS to identify interacting partners. (C) Truncated violin plot of relative sTFR1 amount found coimmunoprecipitating with plasma CALR-del52. Negative control corresponds to the IP product after anti–mutant CALR IP to control for nonspecific binding to anti–mutant CALR antibody. (D) Stability study of rhCALR-del52 in medium with 10% fetal bovine serum (FBS), with or without addition of 2 or 4 μg/mL of rhTFRC. rhCALR-del52 mutant in different media was maintained at 37°C for various lengths of time and measured by ELISA before analysis using a 1-phase decay model (Prism6) to determine the averaged half-life. Values represent mean of triplicate ± SD. (E) Representative confocal microscopy pictures of HEK293T cotransfected with either CALR WT or CALR-del52 fused to green fluorescent protein at the C-terminus and TFR1 fused to mCherry at its C-terminus. Scale bars represent 10 μm. Microscopy analysis shows colocalization between CALR-del52 and TFR1 in subcellular compartments with high correlation between the 2 constructs. (F) IP and glycosylation profile analysis of endogenous TFR1 from UT-7/Tpo or UT-7/Tpo CRISPR CALR-del52. Western blot shows the TFR1 forms analyzed by MS. Data represent the percentage of peptide-spectrum match of immature N-glycans (high mannose) present on residue Asn251 in the cleaved or full form of TFR1.

sTFR1 is a carrier protein for mutant CALR. (A) Allele burden and mutation profile of patients included in this study the analysis. (B) Identification of partners of plasmatic mutant CALR. Plasma from 5 patients with mutated CALR and 5 healthy controls was isolated by IP with biotinylated antimutant CALR antibody. Immunoblot shows the presence of mutant CALR in the IP product detected with a different antimutant CALR antibody. The IP product was analyzed by nontargeted MS to identify interacting partners. (C) Truncated violin plot of relative sTFR1 amount found coimmunoprecipitating with plasma CALR-del52. Negative control corresponds to the IP product after anti–mutant CALR IP to control for nonspecific binding to anti–mutant CALR antibody. (D) Stability study of rhCALR-del52 in medium with 10% fetal bovine serum (FBS), with or without addition of 2 or 4 μg/mL of rhTFRC. rhCALR-del52 mutant in different media was maintained at 37°C for various lengths of time and measured by ELISA before analysis using a 1-phase decay model (Prism6) to determine the averaged half-life. Values represent mean of triplicate ± SD. (E) Representative confocal microscopy pictures of HEK293T cotransfected with either CALR WT or CALR-del52 fused to green fluorescent protein at the C-terminus and TFR1 fused to mCherry at its C-terminus. Scale bars represent 10 μm. Microscopy analysis shows colocalization between CALR-del52 and TFR1 in subcellular compartments with high correlation between the 2 constructs. (F) IP and glycosylation profile analysis of endogenous TFR1 from UT-7/Tpo or UT-7/Tpo CRISPR CALR-del52. Western blot shows the TFR1 forms analyzed by MS. Data represent the percentage of peptide-spectrum match of immature N-glycans (high mannose) present on residue Asn251 in the cleaved or full form of TFR1.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal