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Effects of hyper-osmotic stress on K+ fluxes, H+ extrusion, transmembrane electric potential difference and comparison with the effects of fusicoccin
Authors:Luisa Zingarelli  Maria Teresa Marrè  Ferdinando Massardi  & Piera Lado
Institution:Centro di Studio del CNR per la Biologia Cellulare e Molecolare delle Piante, Dipartimento di Biologia Universitàdegli Studi di Milano, Via Celoria, 26, I-20133 Milano, Italy
Abstract:The stimulation of H+ extrusion by hyper-osmotic stress (0.2–0.3 M mannitol) in cultured cells of Arabidopsis thaliana (L.) Heynh. was shown to be associated with an inhibition of Cl? efflux, whereas hypo-osmotic stress, inhibiting H+ extrusion, early and strongly stimulated Cl? efflux. In this paper, we investigate the contribution of other factors K+ transport and transmembrane electric potential difference (Em)] to the hyper-osmotic-induced activation of the plasma membrane (PM) H+-ATPase. The effects of mannitol (MA) on K+ transport and on Em were compared with those of fusicoccin (FC) since the modes of action of osmotica and of the toxin in stimulating H+-ATPase activity seem to differ at least in some steps. The changes in H+ extrusion induced by hyper- or hypo-osmotic stress were opposite and could be reversed by the application of the respective opposite stress. The effect of MA on H+ extrusion was dependent on the presence of K+ (or Rb+) similarly to that of FC, while Na+ and Li+, which also stimulated the FC effect, were ineffective on that of MA. The MA effect was independent of the anions (Cl?, SO42?, NO3?) accompanying K+. K+ net uptake and K+ influx were stimulated by both MA and FC. Tetraethylammonium (TEA+) and Cs+ inhibited both MA- and FC-induced H+ extrusion, suggesting the involvement of K+ channels. MA (0.2 M) induced a strong hyperpolarization of Em both in the absence and in the presence of K+. The hyperpolarizing effect of MA was also found when the cells were already hyperpolarized by FC, and was rapidly reversed by removing the osmoticum from the medium. In the presence of the lipophilic cation tributylbenzylammonium (TBBA+), MA was no longer able to stimulate H+ extrusion, while FC still stimulated it. In cells pretreated with TBBA+, which strongly depolarized Em, the subsequent addition of FC repolarized it, while the hyperpolarizing effect of MA was lacking. On the contrary, in cells pretreated with Erythrosine B (EB), Em was strongly depolarized and the following addition of FC did not hyperpolarize it, while the hyperpolarizing effect of MA was still observed. These results suggest that the mechanism of MA in activating H+ extrusion and K+ uptake is different from that of FC. The rise in net K+ uptake seems to be driven by the activation of some hyperpolarizing system that does not seem to depend on a direct activation of PM H+-ATPase, but rather on the inhibition of Cl? efflux induced by hyper-osmotic stress.
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