Intracellular sodium activity and sodium transport inNecturus gallbladder epithelium |
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Authors: | J. Graf G. Giebisch |
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Affiliation: | (1) Yale University School of Medicine, 333 Cedar Street, 06510 New Haven, Connecticut;(2) Present address: Department of General and Experimental Pathology, University of Vienna, Wahringerstraße 13, A-1090 Vienna, Austria |
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Abstract: | Summary Ion-sensitive glass microelectrodes, conventional microelectrodes and isotope flux measurements were employed inNecturus gallbladder epithelium to study intracellular sodium activity, [Na]i, electrical parameters of epithelial cells, and properties of active sodium transport. Mean control values were: [Na]i: 9.2 to 12.1mm; transepithelial potential difference,ms: –1.5 mV (lumen negative); basolateral cell membrane potential,es: –62 mV (cell interior negative); sodium conductance of the luminal cell membrane,gNa: 12 mho cm–2; active transcellular sodium flux, 88 to 101 pmol cm–2 sec–1 (estimated as instantaneous short-circuit current). Replacement of luminal Na by K led to a decrease of the intracellular sodium activity at a rate commensurate to the rate of active sodium extrusion across the basolateral cell membrane. Mucosal application of amphotericin B resulted in an increase of the luminal membrane conductance, a rise of intracellular sodium activity, and an increase of short-circuit current and unidirectional mucosa to serosa sodium flux. Conclusions: (i) sodium transport across the basolateral membrane can proceed against a steeper chemical potential difference at a higher rate than encountered under control conditions; (ii) the luminal Na-conductance is too low to accommodate sodium influx at the rate of active basolateral sodium extrusion, suggesting involvement of an electrically silent luminal transport mechanism; (iii) sodium entry across the luminal membrane is the rate-limiting step of transcellular sodium transport and active sodium extrusion across the basolateral cell membrane is not saturated under control conditions. |
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