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Fig. 3. Deglycosylated Na+/K+-ATPase ß-subunits can still interact with the catalytic {alpha}-subunits. (A) Hep G2 cells treated with tunicamycin (TM) or untreated were subjected to immunoprecipitation (IP) experiments using either anti-{alpha}-subunit antibody (anti-{alpha}) or anti-ß-subunit antibody (anti-ß). The resulting immunoprecipitates were analyzed by western blotting. The positions of the {alpha}-subunit and the fully glycosylated (***ß), intermediately glycosylated (**ß), and the core (*ß) proteins of the ß-subunit are indicated. (B) The interactions between the exogenous FLAG-tagged ß-subunit (the wild-type and three deglycosylated mutant constructs) and the endogenous {alpha} protein were tested by IP-western analyses; co-transfected EYFP-{alpha}-tubulin were used as a control. (C) The localization of {alpha}- and ß-subunits before and after tunicamycin treatment was visualized by IF using antibodies specific to either {alpha}- or ß-subunit (green), together with F-actin staining (red). Note the basolateral only (arrowheads) and the apical presence (double arrowheads) of both subunits in the control (CTL) and tunicamycin-treated (TM) cells, respectively. (D) Hep G2 cells transfected with EGFP-labelled ß-subunit (wild-type or N124Q mutant, green), were stained for endogenous {alpha}-subunit (blue) and F-actin (red). Note both wild-type ß-subunit and {alpha}-subunit were found only along the basolateral membrane (arrowheads) in the wild-type transfectants, whereas a portion of the N124Q ß-subunit and the endogenous {alpha}-subunit was aberrantly translocated to the apical domain (double arrowheads) in Hep G2 cell transfected with N124Q ß-subunit. Bars, 10 µm.





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