Figure 6
Figure 6. CALR mutants modify TpoR stability, maturation, and trafficking. (A) The expression of CALR in calr−/− MEFs transduced with retroviral constructs expressing TpoR and CALR wild-type or mutants was assessed by immunofluorescence (top panel) and by western blotting after cycloheximide (30 μg/mL) treatment (bottom panel). (B) Maturation state of TpoR in Ba/F3-TpoR cells in the presence of CALR wild-type or mutants was assessed by western blotting upon endoglycosidase H treatment or not. (B) Subcellular fractionation of CALR wild-type and mutant del52 proteins in calr−/− MEF TpoR cells. The distribution patterns of CALR and GRP78 were shown in the diagram and the blots. (C) Confocal immunofluorescence microscopy was performed in previously described calr−/− MEF cell lines and stained with anti-CALN (Calnexin), anti-CALR, and 4,6 diamidino-2-phenylindole. (D) Maturation state of TpoR in Ba/F3-TpoR cells in the presence of wild-type or mutant CALR was assessed by western blotting upon endoglycosidase H treatment or not. (E) Western blot analysis of immunoprecipitated N-terminal HA-tagged TpoR present on cell surface, in Ba/F3-TpoR cells expressing wild-type or mutant CALR. All data are normalized, C being the amount per volume of subfraction, and Ci the corresponding value in the pooled subfractions.

CALR mutants modify TpoR stability, maturation, and trafficking. (A) The expression of CALR in calr−/− MEFs transduced with retroviral constructs expressing TpoR and CALR wild-type or mutants was assessed by immunofluorescence (top panel) and by western blotting after cycloheximide (30 μg/mL) treatment (bottom panel). (B) Maturation state of TpoR in Ba/F3-TpoR cells in the presence of CALR wild-type or mutants was assessed by western blotting upon endoglycosidase H treatment or not. (B) Subcellular fractionation of CALR wild-type and mutant del52 proteins in calr−/− MEF TpoR cells. The distribution patterns of CALR and GRP78 were shown in the diagram and the blots. (C) Confocal immunofluorescence microscopy was performed in previously described calr−/− MEF cell lines and stained with anti-CALN (Calnexin), anti-CALR, and 4,6 diamidino-2-phenylindole. (D) Maturation state of TpoR in Ba/F3-TpoR cells in the presence of wild-type or mutant CALR was assessed by western blotting upon endoglycosidase H treatment or not. (E) Western blot analysis of immunoprecipitated N-terminal HA-tagged TpoR present on cell surface, in Ba/F3-TpoR cells expressing wild-type or mutant CALR. All data are normalized, C being the amount per volume of subfraction, and Ci the corresponding value in the pooled subfractions.

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