Figure 1.
Expression of DMT1 and iron uptake study. (A) Western blot analysis of peripheral blood cell lysates (90 μg) and Caco-2 cells lysate (30 μg) with primary goat anti-Nramp2 antibody (1/1000, 16 hours, 4°C) and peroxidase-conjugated secondary antibody (Pierce; 1/1000, 90 minutes, room temperature). The 64-kDa band represents the DMT1 protein; lane 1, Caco-2; lane 2, patient's father; lane 3, patient's mother; lane 4, patient. (B-C) Western blot analysis of total cell lysates (30 μg) and crude membrane extracts (50 μg) from CHO cells expressing the empty vector (CHO), WT, E399D, and DEL forms of HA-tagged DMT1 with mouse anti-HA antibody (1/1000, 1 hour, room temperature) and peroxidase-conjugated secondary antibody (1/1000, 90 minutes, room temperature). Mature complex-glycosylated DMT1 form (90 to 100 kDa; ▹) and the core-glycosylated form of DMT1 (66 kDa; ◂) are indicated. Equal loading of proteins was assessed by probing with an antibody against β-actin or α-tubulin (1/1000, 1 hour, room temperature). Representative immunoblots of 3 separate experiments are illustrated. (D) Iron transport activities of WT, E399D, and DEL DMT1 incubated in pH 6.0 incubation buffer with 59Fe(II)-ascorbate (10 μM 59Fe). Iron uptake is expressed as intracellular 59Fe (cpm per 106 cells). “CHO empty” represents iron uptake by cells transfected with empty vector. Data shown are the means ± SD of duplicate determinations from a typical experiment that was performed 3 times.