H+ transport by reconstituted gastric (H+ + K+)-ATPase

Gastric (H+ + K+)-ATPase was reconstituted into artificial phosphatidylcholine/cholesterol liposomes by means of a freeze-thaw-sonication technique. Upon addition of MgATP, active H+ transport was observed, with a maximal rate of 2.1 mumol X mg-1 X min-1, requiring the presence of 100 mM K+ at the intravesicular site. However, in the absence of ATP an H+-K+ exchange with a maximal rate of 0.12 mumol X mg-1 X min-1 was measured, which could be inhibited by the well-known ATPase inhibitors vanadate and omeprazole, giving the first evidence of a passive K+-H+ exchange function of gastric (H+ + K+)-ATPase. An Na+-H+ exchange activity was also measured, which was fully inhibited by 1 mM amiloride. Simultaneous reconstitution of Na+/H+ antiport and (H+ + K+)-ATPase could explain why reconstituted ATPase appeared less cation-specific than the native enzyme (Rabon, E.C., Gunther, R.B., Soumarmon, A., Bassilian, B., Lewin, M.J.M. and Sachs, G. (1985) J. Biol. Chem. 260, 10200-10212).     

Effect of cisplatin on H+ transport by H+ -ATPase and Na+/H+ exchanger in rat renal brush-border membrane

The effect of the potent anticancer drug cisplatin, cis-diamminedichloroplatinum (II) (CDDP), on H+ -ATPase and Na+/H+ exchanger in rat renal brush-border membrane was examined. To measure H+ transport by vacuolar H+ -ATPase in renal brush-border membrane vesicles, we employed a detergent-dilution procedure, which can reorientate the catalytic domain of H+ -ATPase from an inward-facing configuration to outward-facing one. ATP-driven H+ pump activity decreased markedly in brush-border membrane prepared from rats two days after CDDP administration (5 mg/kg, i.p.). In addition, N-ethylmaleimide and bafilomycin A1 (inhibitors of vacuolar H+ -ATPase)-sensitive ATPase activity also decreased in these rats. The decrease in ATP-driven H+ pump activity was observed even at day 7 after the administration of CDDP. Suppression of ATP-driven H+ pump activity was also observed when brush-border membrane vesicles prepared from normal rats were pretreated with CDDP in vitro. In contrast with H+ -ATPase, the activity of Na+/H+ exchanger, which was determined by measuring acridine orange fluorescence quenching, was not affected by the administration of CDDP. These results provide new insights into CDDP-induced renal tubular dysfunctions, especially such as proximal tubular acidosis and proteinuria.     

Cation transport by gastric H+:K+ ATPase.

A vesicular microsomal fraction isolated from hog fundic mucosa demonstrates the capacity to take up equal amounts of RB+ and Cl-. The amount of the Rb+ uptake is sensitive to the extravesicular osmolarity, and rate of uptake is sensitive to temperature. 86Rb+ efflux is dependent upon the cation composition of the diluting solution. ATP, but not beta-gamma methylene ATP, induces a reversible efflux of 86Rb+ from loaded vesicles, and this is dependent upon a functional K+-ATPase. The ATP induced efflux is not affected by CCCP (carbonyl cyanide m-chlorophenylhydrazone) or TCS (tetrachlorosalicylanilide) nor by lipid soluble ions or valinomycin. Nigericin inhibits the efflux by 40%. Uptake of the lipid soluble ion 14C-SCN- has been demonstrated and is enhanced by ATP only in the presence of valinomycin. The results are consistent with a neutral or isopotential exchange of H+ for Rb+ mediated by K+-ATPase.     

The lysosomal H+ pump: 8-azido-ATP inhibition and the role of chloride in H+ transport

Lysosomes (tritosomes) were purified from the livers of rats injected with Triton WR 1339. The lysosomes developed an Mg2+-ATP-dependent pH gradient as measured by Acridine orange accumulation. H+ transport was supported by chloride, but not sulfate, and was independent of the cation used. H+ transport and Mg2+-stimulated ATPase was inhibited by diethylstilbesterol (K0.5 = 2 microM). N-Ethylmaleimide inhibited H+ transport (K0.5 = 30 microM). At low concentrations of N-ethylmaleimide, ATP partially protected H+ transport from inhibition with N-ethylmaleimide. Photolysis with 8-azido-ATP inhibited H+ transport and Mg2+-stimulated ATPase activity. Under these same conditions, 8-azido-[alpha-32P]ATP reacted with a number of polypeptides of the intact lysosome and lysosomal membranes. Pump-dependent potentials were measured using the fluorescent potential-sensitive dye, DiSC3(5) (3,3'-dipropylthiocarbocyanine) and ATP-dependent potential generation was inhibited by diethylstilbesterol. Chloride, but not sulfate reduced the magnitude of the ATP-dependent membrane potential, as measured using merocyanine 540. The chloride conductance, independent of ATP, was of sufficient magnitude to generate a H+ gradient driven by external chloride in the presence of tetrachlorosalicylanilide. In Cl- free media, ATP-dependent H+ transport was restored to control levels by outwardly directed K+ gradients in the presence of valinomycin. The role of cell Cl- is to provide the necessary conductance for supporting lysosomal acidification by the electrogenic proton pump.     

H+-coupled pantothenate transport in the intracellular malaria parasite

Pantothenate, the precursor of coenzyme A, is an essential nutrient for the intraerythrocytic stage of the malaria parasite Plasmodium falciparum. Pantothenate enters the malaria-infected erythrocyte via new permeation pathways induced by the parasite in the host cell membrane (Saliba, K. J., Horner, H. A., and Kirk, K. (1998) J. Biol. Chem. 273, 10190-10195). We show here that pantothenate is taken up by the intracellular parasite via a novel H(+)-coupled transporter, quite different from the Na(+)-coupled transporters that mediate pantothenate uptake into mammalian cells. The plasmodial H(+):pantothenate transporter has a low affinity for pantothenate (K(m) approximately 23 mm) and a stoichiometry of 1 H(+):1 pantothenate. It is inhibited by low concentrations of the bioflavonoid phloretin and the thiol-modifying agent p-chloromercuribenzene sulfonate. On entering the parasite, pantothenate is phosphorylated (and thereby trapped) by an unusually high affinity pantothenate kinase (K(m) approximately 300 nm). The combination of H(+)-coupled transporter and kinase provides the parasite with an efficient, high affinity pantothenate uptake system, which is distinct from that of the host and is therefore an attractive target for antimalarial chemotherapy.     

Plant sucrose-H+ symporters mediate the transport of vitamin H

A cDNA coding for a vitamin H (biotin) transport protein from Arabidopsis was identified by genetic complementation of a biotin uptake-deficient yeast mutant. Vitamin H transport by this protein was sensitive to the SH-group inhibitor p-chloromercuribenzene sulfonic acid (PCMBS) and to the uncoupler carbonyl cyanide-m-chlorophenylhydrazone (CCCP), suggesting an energy-dependent biotin-H+ symport mechanism. The transport activity could contribute to the so-far uncharacterized plant sucrose-H+ symporter AtSUC5 which mediates the energy-dependent transport of biotin and sucrose, and restores growth of the biotin transport-deficient yeast mutant on medium with low biotin concentrations. Functional comparison of the AtSUC5 transporter with previously characterized plant sucrose or monosaccharide transporters revealed that biotin transport may be a general and specific property of all plant sucrose transporters (sucrose/biotin-H+ symporters). This first report on a transporter with dual substrate specificity for two structurally unrelated molecules has a major impact on general thinking concerning the specificity of membrane transporters. The physiological relevance of this finding is discussed.     

Coupling between H+ transport and anaerobic glycolysis in turtle urinary bladder: Effects of inhibitors of H+ ATPase

Summary The coupling between H⁺ transport (J _H) and anaerobic glycolysis was examinedin vitro in an anaerobic preparation of turtle urinary bladder.J _H was measured as the short-circuit current after Na⁺ transport was abolished with ouabain and by pH stat titration. The media were gassed with N₂ and 1% CO₂ (PO₂<0.5 mm Hg) and contained 10mm glucose. Under these conditions,J _H was not inhibited by 3mm serosal (S) cyanide or by 0.1mm mucosal (M) dinitrophenol. Control anerobic lactate production (J _lac) of 47 bladders was plotted as a function of simultaneously measuredJ _H. The slope ofJ _lac onJ _H was 0.58±0.12 with an intercept forJ _lac atJ _H=0 of 0.55 mol/hr. Values for J _lac/J _H were determined in groups of individual bladders whenJ _H was inhibited by an opposing pH gradient (0.55±0.16), by acetazolamide (0.58±0.19) and by dicyclohexylcarbodiimide, DCCD (0.58±0.14). The constancy of J _lac/J _H indicates a high degree of coupling betweenJ _H andJ _lac. Since the anaerobic metabolism of glucose produces one ATP for each lactate formed, the J _lac/J _H values can be used to estimate the stoichiometry of H⁺ translocation. The movement of slightly less than 2 H⁺ ions is coupled to the hydrolysis of one ATP. During anaerobiosis (absence of mitochondrial ATPase function) the acidification pump was not inhibited byM addition of oligomycin but was inhibited byM addition of DCCD and Dio-9, inhibitors of H⁺ flow in the proteolipid portion of H⁺-translocating ATPases. DCCD inhibited anaerobicJ _H without change in J _lac/J _H or basalJ _lac and, therefore, acted primarily on the H⁺ pump.S addition of vanadate also inhibitedJ _H, but the inhibition was associated with an increase inJ _lac. The site of this apparent uncoupling remains to be defined. The acidification pump of the luminal cell membrane of the turtle bladder has H⁺-ATPase characteristics that differ from mitochondrial ATPase in that H⁺ transport is oligomycin-resistant and vanadate-sensitive. As judged from the flows of H⁺ and lactate, the H⁺/ATP stoichiometry of the pump is about 2.     

Ischemic preconditioning inhibits mitochondrial respiration,increases H2O2 release,and enhances K+ transport

Ischemic preconditioning, or the protective effect of short ischemic episodes on a longer, potentially injurious, ischemic period, is prevented by antagonists of mitochondrial ATP-sensitive K+ channels (mitoKATP) and involves changes in mitochondrial energy metabolism and reactive oxygen release after ischemia. However, the effects of ischemic preconditioning itself on mitochondria are still poorly understood. We determined the effects of ischemic preconditioning on isolated heart mitochondria and found that two brief (5 min) ischemic episodes are sufficient to induce a small but significant decrease ( approximately 25%) in mitochondrial NADH-supported respiration. Preconditioning also increased mitochondrial H2O2 release, an effect related to respiratory inhibition, because it is not observed in the presence of succinate plus rotenone and can be mimicked by chemically inhibiting complex I in the presence of NADH-linked substrates. In addition, preconditioned mitochondria presented more substantial ATP-sensitive K+ transport, indicative of higher mitoKATP activity. Thus we directly demonstrate that preconditioning leads to mitochondrial respiratory inhibition in the presence of NADH-linked substrates, increased reactive oxygen release, and activation of mitoKATP.     

Ammonium transport by the colonic H+-K+-ATPase expressed in Xenopus oocytes

Functional expression of the rat colonicH⁺-K⁺-ATPasewas obtained by coexpressing its catalytic -subunit and the₁-subunit of theNa⁺-K⁺-ATPasein Xenopus laevis oocytes. We observedthat, in oocytes expressing the rat colonicH⁺-K⁺-ATPasebut not in control oocytes (expressing₁ alone),NH₄Cl induced a decrease in⁸⁶Rb uptake and the initial rateof intracellular acidification induced by extracellularNH₄Cl was enhanced, consistentwith NH⁺₄ influx via the colonicH⁺-K⁺-ATPase.In the absence of extracellularK⁺, only oocytes expressing thecolonicH⁺-K⁺-ATPasewere able to acidify an extracellular medium supplemented withNH₄Cl. In the absence ofextracellular K⁺ and in thepresence of extracellular NH⁺₄, intracellular Na⁺ activity in oocytes expressingthe colonicH⁺-K⁺-ATPasewas lower than that in control oocytes. A kinetic analysis of⁸⁶Rb uptake suggests thatNH⁺₄ acts as a competitive inhibitor of thepump. Taken together, these results are consistent withNH⁺₄ competition forK⁺ on the external site of thecolonicH⁺-K⁺-ATPaseand with NH⁺₄ transport mediated by this pump.

     

Specificity of ligand binding to transport sites: Ca2+ binding to the Ca2+ transport ATPase and its dependence on H+ and Mg2+

Ligand binding to transport sites constitutes the initial step in the catalytic cycle of transport ATPases. Here, we consider the well characterized Ca²⁺ ATPase of sarcoplasmic reticulum (SERCA) and describe a series of Ca²⁺ binding isotherms obtained by equilibrium measurements in the presence of various H⁺ and Mg²⁺ concentrations. We subject the isotherms to statistical mechanics analysis, using a model based on a minimal number of mechanistic steps. The analysis allows satisfactory fits and yields information on occupancy of the specific Ca²⁺ sites under various conditions. It also provides a fundamental method for analysis of binding specificity to transport sites under equilibrium conditions that lead to tightly coupled catalytic activation.     

Mechanism of action of gastric secretory inhibitors: effects of SCN- OCN-, NO-2, and NH+4 on (H+ + K+)-ATPase-mediated transport of H+ inside gastric microsomal vesicles

The mechanisms of action of the known inhibitors of gastric acid secretion such as SCN^?, OCN^?, NO₂^?, and NH₄⁺ (M. E. LeFevre, E. J. Gohmann, Jr. and W. S. Rehm, 1964, Amer. J. Physiol.207, 613–618) were investigated using isolated pig gastric microsomal vesicles as a model system. The gastric microsomal vesicles enriched in (H⁺ + K⁺)-ATPase have previously been demonstrated to accumulate H⁺ in exchange for K⁺. The vesicular accumulation of acridine orange, which is a measure of H⁺ uptake, shows sigmoidal kinetics in the presence of increasing K⁺ with a Hill coefficient of 2.27 and a S₅₀ of 19.05 mm. None of those agents affects the microsomal (H⁺ + K⁺)-ATPase activity, although they inhibit vesicular H⁺ transport in a dose-dependent manner; the order of efficacy being NH₄⁺ > SCN^? > OCN^? > NO₂^?. The inhibitory effects of NH₄⁺ on vesicular H⁺ transport appear to be due to neutralization of the transported H⁺ by freely permeable NH₃ generated from the dissociation of NH₄⁺ in the bulk medium. SCN^?, OCN^?, and NO₂^? appear to work by a different mechanism. These agents do not act as protonophores. Our data demonstrate that the presence of SCN^?, OCN^?, and NO₂^? within the vesicle interior are essential for exerting their inhibitory effects. Furthermore, the inhibitory effects of SCN^? and OCN^? on vesicular H⁺ transport could be reversed by an elevation of intravesicular K⁺. Our data strongly suggest that the effects of SCN^?, OCN^?, and NO₂^? are exerted by interfering with a low-affinity K⁺ site (S₅₀ = 19.05 mm) within the domain of the gastric ATPase complex. This low-affinity K⁺ site is accessible only from the vesicle interior and appears to be essential for the vectorial transport of H⁺ by the gastric microsomal (H⁺ + K⁺)-ATPase system.     

Characteristics of light-induced H+ transport in spinach chloroplast at lower temperatures I. Relationship between H+ transport and physical changes of the microenvironment in chloroplast membranes

Light-induced H⁺ transport of spinach chloroplasts was investigatedin the temperature range from 5° to 30°C with a glasselectrode. The rate of H⁺ transport was reduced by lowering the temperature.Addition of 1 µM phenazine methosulfate (PMS) considerablystimulated the H⁺ uptake in chloroplasts. PMS was also effectivein stimulating the H⁺ efflux when the illumination was turnedoff. The latter effect became more marked at lower temperatures.These results indicate that electron transfer reactions in thechloroplast not only drive the forward process of H⁺ gradientformation, but also participate in the backward H⁺ efflux. The Arrhenius plot applied to the first-order rate constantof the H⁺ efflux showed a discontinuity at about 20°C. Nohysteresis was detected with the temperature dependence andits discontinuity in the H⁺ transport. On the other hand, theaddition of PMS abolished the discontinuity and a linear relationshipwas observed in the Arrhenius plot. Probably, temperature-dependentphysical changes in the microenvironment of the chloroplastlamellae are responsible for determining the characteristicsof the H⁺transport. (Received September 11, 1975; )     

Serosal Na/Ca exchange and H+ and Na+ transport by the turtle and toad bladders

Summary A Na/Ca exchange system has been described in the plasma membrane of several tissues and seems to regulate the concentration of calcium in cytosol. Replacement of extracellular Na by sucrose increases calcium uptake into and decreases calcium efflux from the cell, leading to an increase in cytosolic calcium. The effect of an increase in cytosolic calcium mediated by the Na/Ca exchange system on H⁺ and Na transport in the turtle and toad bladder was investigated by replacing serosal Na isosmotically by sucrose or choline. Replacement of serosal by sucrose was associated with a significant inhibition of H⁺ secretion or Na transport which was reversible by addition of NaCl. Replacement of mucosal Na by sucrose failed to alter H⁺ secretion. Removal of serosal Na was associated with a significant increase in⁴⁵Ca uptake which could be blocked by pretreatment with lanthanum chloride. Pretreatment with lanthanum chloride blunted the inhibitory effect of replacement of serosal Na by sucrose on H⁺ and Na transport, thus suggesting that the increase in calcium uptake and the inhibition of transport are causally related. Under anaerobic conditions the rate of H⁺ or Na transport are linked to the rate of lactate production. The inhibition of Na or H⁺ transport by removal of serosal Na was accompanied by a proportional decrease in lactate production, thus suggesting that an increase in cytosolic calcium does not inhibit transport by uncoupling glycolysis from transport. Replacement of serosal Na by sucrose did not alter the force of the H⁺ or Na pump but led to an increase in resistance of the active pathway of H⁺ and Na transport. The inhibition of Na transport by replacement of serosal Na with sucrose could be reversed by addition of amphotericin B, an agent which increases luminal permeability to Na, thus suggesting that decreased Na entry across the apical membrane is the mechanism responsible for the inhibition of Na transport. The results of the present studies strongly suggest that an increase in cytosolic calcium through the serosal Na/Ca exchange system inhibits H⁺ and Na transport in the turtle and toad bladder probably by increasing the resistance of the luminal membrane.     

Metabolic pathways coupled to H+ transport in turtle urinary bladder

Summary Active H⁺ transport in the turtle urinary bladder is mediated by an ATPase. Although the source of ATP is usually mitochondrial oxidative phosphorylation, it is possible because of intracellular compartmentalization or cellular heterogeneity that one metabolic pathway exclusively provides ATP to the pump. To examine this we performed several types of experiments. In one, the coupling between the rate of transport and the rate of oxidation of¹⁴C-labeled substrates was studied. We found that there was coupling between H⁺ transport and glucose, butyrate, oleate, and -OH-butyrate oxidation. In another set of experiments we depleted turtle bladders of their endogenous substrates and tested the effect of a number of substrates on the rate of transport. We found that glucose, pyruvate, lactate, actetate, butyrate and -OH butyrate all stimulated H⁺ transport. In a third set of experiments we found no coupling between H⁺ transport and lactate production. Finally, we found that reduction of H⁺ transport by mucosal acidification resulted in an increase in epithelial cell ATP concentrations and a decrease in ADP levels.These results suggest that the H⁺ pump receives its ATP from carbohydrate and fatty acid oxidation. The changes in ATP and ADP levels provide an initial explanation for the coupling of H⁺ transport to the rate of cellular oxidative metabolism.     

Stoichiometry of H+-linked dopamine transport in chromaffin granule ghosts

A proton-translocating adenosinetriphosphatase in adrenal medullary chromaffin granule ghosts can generate either a membrane potential (inside positive) or a pH gradient (inside acid). Dopamine uptake occurs in response to both the membrane potential and the pH gradient. The natural logarithm of the dopamine concentration gradient [In (Din/Dout)] is linearly related to the membrane potential with a slope of F/(RT). This dependence is not affected by the pH of the medium. In (Din/Dout) is linearly dependent on In ([H+]in/[H+]out) with a slope of 2. These results indicate that dopamine is taken up via an exchange diffusion or antiport mechanism. The stoichiometry of this exchange is two H+/dopamine cation and is independent of pH.     

A novel method to quantify H+-ATPase-dependent Na+ transport across plasma membrane vesicles

To prevent sodium toxicity in plants, Na(+) is excluded from the cytosol to the apoplast or the vacuole by Na(+)/H(+) antiporters. The secondary active transport of Na(+) to apoplast against its electrochemical gradient is driven by plasma membrane H(+)-ATPases that hydrolyze ATP and pump H(+) across the plasma membrane. Current methods to determine Na(+) flux rely either on the use of Na-isotopes ((22)Na) which require special working permission or sophisticated equipment or on indirect methods estimating changes in the H(+) gradient due to H(+)-ATPase in the presence or absence of Na(+) by pH-sensitive probes. To date, there are no methods that can directly quantify H(+)-ATPase-dependent Na(+) transport in plasma membrane vesicles. We developed a method to measure bidirectional H(+)-ATPase-dependent Na(+) transport in isolated membrane vesicle systems using atomic absorption spectrometry (AAS). The experiments were performed using plasma membrane-enriched vesicles isolated by aqueous two-phase partitioning from leaves of Populus tomentosa. Since most of the plasma membrane vesicles have a sealed right-side-out orientation after repeated aqueous two-phase partitioning, the ATP-binding sites of H(+)-ATPases are exposed towards inner side. Leaky vesicles were preloaded with Na(+) sealed for the study of H(+)-ATPase-dependent Na(+) transport. Our data implicate that Na(+) movement across vesicle membranes is highly dependent on H(+)-ATPase activity requiring ATP and Mg(2+) and displays optimum rates of 2.50 microM Na(+) mg(-1) membrane protein min(-1) at pH 6.5 and 25 degrees C. In this study, for the first time, we establish new protocols for the preparation of sealed preloaded right-side-out vesicles for the study of H(+)-ATPase-dependent Na(+) transport. The results demonstrate that the Na(+) content of various types of plasma membrane vesicle can be directly quantified by AAS, and the results measured using AAS method were consistent with those determined by the previous established fluorescence probe method. The method is a convenient system for the study of bidirectional H(+)-ATPase-dependent Na(+) transport with membrane vesicles.