| Abstract: | In Aplysia intestine,stimulation of Na+ absorption withluminal alanine increases apical membraneK+ conductance(GK,a), whichpresumably regulates enterocyte volume during stimulatedNa+ absorption. However, themechanism responsible for the sustained increase in plasma membraneK+ conductance is not known forany nutrient-absorbing epithelium. In the present study, we have begunto test the hypothesis that the alanine-induced increase inGK,a inAplysia enterocytes results fromexocytic insertion of K+ channelsinto the apical membrane. We used the fluid-phase marker horseradishperoxidase to assess the effect of alanine on apical membraneexocytosis and conventional microelectrode techniques to assess theeffect of alanine on fractional capacitance of the apical membrane(fCa). Luminalalanine significantly increased apical membrane exocytosis from 1.04 ± 0.30 to 1.39 ± 0.38 ng · min 1 · cm2.To measure fCa,we modeled the Aplysia enterocyte as adouble resistance-capacitance (RC) electric circuit arranged in series. Several criteria were tested to confirm application of the model to theenterocytes, and all satisfied the model. When added to the luminalsurface, alanine significantly increasedfCa from 0.27 ± 0.02 to 0.33 ± 0.04 (n = 10)after 4 min. There are two possible explanations for our findings:1) the increase in exocytosis, whichadds membrane to the apical plasma membrane, prevents plasma membranefracture, and 2) the increase inexocytosis delivers K+ channels tothe apical membrane by exocytic insertion. After the alanine-induceddepolarization of apical membrane potential (Va), there isa strong correlation (r = 0.96)between repolarization ofVa, whichreflects the increase inGK,a, andincrease in fCa. This correlation supports the exocytic insertion hypothesis for activation ofGK,a. |
