Figure 6.
Figure 6. Analysis of the degradation mechanisms of WT and Nramp2G185R. LLC-PK1 cells transfected with WT or Nramp2G185R-HA were labeled metabolically by a one-hour pulse of 35S-Met/Cys. Samples of the labeled cells were taken immediately after the pulse (0 chase) or after a 2-hour chase in the absence of presence of either 10 μM of MG132 or 15 mM of NH4Cl, as indicated. The cells were next subjected to lysis, immunoprecipitation of Nramp2, gel electrophoresis, and autoradiography, as in Figure 4. (A) Typical radiograms of WT (top) and Nramp2G185R (bottom) transfected cells. Only the band corresponding to the core-glycosylated species is shown. (B) Quantification of the fraction of core-glycosylated Nramp2 remaining after a 2-hour chase, normalized to the amount of the respective protein immediately after the radioactive pulse. Data are means plus or minus SE of 3 experiments like that shown in panel A. ***P < .001, calculated using Student t test.

Analysis of the degradation mechanisms of WT and Nramp2G185R. LLC-PK1 cells transfected with WT or Nramp2G185R-HA were labeled metabolically by a one-hour pulse of 35S-Met/Cys. Samples of the labeled cells were taken immediately after the pulse (0 chase) or after a 2-hour chase in the absence of presence of either 10 μM of MG132 or 15 mM of NH4Cl, as indicated. The cells were next subjected to lysis, immunoprecipitation of Nramp2, gel electrophoresis, and autoradiography, as in Figure 4. (A) Typical radiograms of WT (top) and Nramp2G185R (bottom) transfected cells. Only the band corresponding to the core-glycosylated species is shown. (B) Quantification of the fraction of core-glycosylated Nramp2 remaining after a 2-hour chase, normalized to the amount of the respective protein immediately after the radioactive pulse. Data are means plus or minus SE of 3 experiments like that shown in panel A. ***P < .001, calculated using Student t test.

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