From the Departamento de Bioquímica, Biología Celular y Molecular de Plantas, Estación Experimental del Zaidín, CSIC, Apartado 419, 18080-Granada, Spain
Received for publication, October 22, 2002 , and in revised form, April 14, 2003.
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ABSTRACT |
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INTRODUCTION |
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The role and concentration of K+ in other endomembrane organelles in plants are largely unknown. Apart from a specific K+ requirement, secondary ion transporters might rely on K+ for pH regulation in these organelles. It was shown that apart from the vacuole, V-type H+-transporting ATPase is found in various membranes of the secretory system where vesicle acidification is important for ligand-receptor binding and protein modification, trafficking, and sorting (4, 5). In animal cells, the pH gradient from neutral to acidic along organelles from both the secretory and endocytic pathways is suggested to be under tight control by the operation of secondary ion transporters providing proton leak pathways (6, 7, 8). Second, solute uptake energized by the pH gradient might be required to generate the osmotic pressure needed for vesicle fusion (5). In view of the abundance of K+ in the cell, K+/H+ exchangers are likely candidates to be involved in pH and osmoregulation of intracellular compartments as well as active uptake of K+ into vacuoles (3) although the biochemical evidence for the existence of such antiporters is scarce (9, 10).
In contrast to the limited information available on K+/H+ antiporters, many reports have indicated the existence of vacuolar Na+/H+ antiporters in plants (11). The first vacuolar Na+/H+ exchanger AtNHX1 was identified recently (12), and it was shown that overexpression of this gene in plants enhances salt tolerance (13, 14, 15). A family of six genes was identified in Arabidopsis (AtNHX1 to AtNHX6) that shows sequence homology to mammalian and yeast NHE or NHX exchangers (16, 17). It was demonstrated however that AtNHX1 could catalyze both Na+/H+ and K+/H+ exchange (14, 18). A similar ion specificity was reported for the human NHE7 isoform. It was shown that this isoform is expressed in the trans-Golgi network, indicating that regulation of pH and ionic composition of intracellular compartments by K+/H+ or Na+/H+ exchange is an important task of these antiporters (7). This notion was strengthened by the observation that the NHX1 protein is essential for osmotolerance and endosomal protein trafficking in yeast (19, 20). Indeed, plant NHX genes were shown not only to be involved in salinity tolerance, but also in vacuolar pH regulation (21, 22), and to be induced by NaCl, KCl, and osmotic stress (12, 16, 2326), or even heat shock (27).
We have identified the first NHX proteins in tomato. One isoform, LeNHX2 is relatively distant from the AtNHX1 protein. In this study we describe this isoform, and analyze its function by heterologous expression in yeast. The LeNHX2 protein turns out to be the first intracellular K+/H+ antiporter protein in plants, which enables the maintenance of higher K+ concentrations in intracellular compartments under conditions of salt stress when expressed in yeast. These data show that plants contain different NHX genes with different ionic specificities regulating K+, Na+, and H+ ion homeostasis in intracellular compartments.
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EXPERIMENTAL PROCEDURES |
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Plant Growth ConditionsTomato seeds (L. esculentum Mill, cv. Pera) were surface-sterilized and then germinated and grown for 5 weeks in sterile vermiculite under a light irradiance of 150 µmol m2 s1 (16-h photoperiod) at 26 °C and 6065% relative humidity. One-tenth strength Hoagland's nutrient solution (30) was applied from emergence of the first leaf and raised to quarter-strength (2 weeks after sowing) thereafter, every 3 days. Plants were treated for 0, 1, 6, and 24 h with 130 mM NaCl or for 1 h with 100 µM abscisic acid, before harvesting root, stem, and leaf tissues.
RNA Blot AnalysisA DNA probe for LeNHX2 was made by amplification of a 415-bp fragment of the C-terminal coding region using gene-specific forward and reverse primers. Total RNA from different tissues was isolated and purified according to Logemann et al. (31). RNA for all blots (15 µg) was run on 1.2% denaturing formaldehyde agarose gels and blotted onto nylon membranes (HybondTM N+, Amersham Biosciences) (32). The DNA probes were radioactively labeled with [-32P]dCTP by random priming using the RediprimeTMII kit (Amersham Biosciences). Nylon filters were prehybridized and hybridized at 65 °C in hybridization buffer containing 7% (w/v) SDS, 300 mM sodium phosphate, pH 7.0, and 1 mM EDTA (33). Blots were washed twice in 4x SSC, 0.1 (w/v) SDS, and once in 0.4x SSC, 0.1 (w/v) SDS, at 65 °C for 15 min each. Membranes were rehybridized with a tomato 18 S rDNA gene probe to monitor RNA loading quantity (a gift from Dr. N. Ferrol, Est. Exp. Zaidín, CSIC, Granada, Spain). Nylon filters were exposed to a Phosphorimager screen (BioRad Molecular Imager System) and/or exposed to X-Omat AR5 film (Kodak), where hybridization signal was recorded with a Phosphorimager analyzer (BioRad Molecular Imager System) or digitized with a BioRad imaging analyzer, respectively. Transcript amount was determined by quantification of band signal intensities of digitized images and relativized to the respective ribosomal signals using Scion Image software (version 3.62a; www.scioncorp.com).
Yeast Strains and Growth ConditionsAll Saccharomyces cerevisiae strains used were derivatives of W303-1B (Mat leu2-13 112 ura3-1 trp1-1 his3-11, 15 ade2-1 can1-100). Strains WX1 (
nhx1::TRP1), ANT3 (
ena14::HIS3
nha1::LEU2), and AXT3 (
ena14::HIS3
nha1::LEU2
nhx1::TRP1) were gifts from Drs. F. J. Quintero and J. M. Pardo (IRNA Sevilla, Spain). Cells were grown at 30 °C in YPD (1% yeast extract, 2% peptone, 2% glucose) or APD (10 mM arginine, 8 mM phosphoric acid, 2% glucose, 2 mM MgSO4, 1 mM KCl, 0.2 mM CaCl2, trace minerals and vitamins, Ref. 34). For induction of antiporter expression in cells carrying plasmids with antiporter genes under the control of the GAL1 promoter, glucose (2%) was replaced by galactose (2%) in the growth media. For growth curves or drop tests, a preculture was made by growing the strains in selective APD medium to saturation (OD660 nm of 45). In drop tests, the preculture was diluted 50-fold, after which 10 µl of serial (101) dilutions were spotted on YPD plates with 0, 10, or 25 µg/ml hygromycin B. Growth curves were made in a total volume of 50 ml using a 250-ml cell culture vessels stirred at 80 rpm under continuous aeration. Growth was started by diluting the preculture to OD660 nm of 0.006 in APD medium (pH 6.0) with or without 20 mM NaCl. Samples were taken at the indicated time points to determine OD660 nm.
Determination of Total Intracellular Ion ContentCells were grown in liquid APG medium (APD medium with galactose instead of glucose) supplemented or not with 20 mM NaCl as indicated. 50-ml fractions were taken when the cells reached an OD660 nm of 0.25 ± 0.01 and centrifuged (2 min at 3000 x g). Cells were washed twice with 10 ml of ice-cold 10 mM MgCl2, 10 mM CaCl2, 1 mM HEPES. Washed cells were resuspended in 2 ml of the same buffer and the cell density determined from the optical density at 660 nm. Separately the relationship between OD660 nm and yeast dry weight was determined. Intracellular ions were extracted by addition of HCl to a final concentration of 0.4% and incubation for 20 min at 95 °C. After removal of cell debris by centrifugation, potassium and sodium ion content was determined with an atomic absorption spectrometer.
Determination of Vacuolar and Cytoplasmic Ion ContentThe vacuolar and cytoplasmic Na+ and K+ content was determined by treating the cells with cytochrome c that selectively permeabilizes the plasma membrane (35, 36). Cells were grown and washed as above and resuspended in 50 µl of 2% cytochrome c, 18 µg/ml antimycin, 1 mM HEPES, 10 mM MgSO4, 10 mM CaCl2 and 5 mM 2-deoxy D-glucose. After incubation for 20 min at room temperature, the cells were centrifuged and washed three times with 2 ml of the same solution without cytochrome c. The supernatants containing the ions released by the cytochrome c treatment were pooled to determine cytoplasmic ion content. The remaining ions, corresponding to the vacuolar fraction, were extracted by addition of HCl to a final concentration of 0.4% in a total volume of 2 ml and incubation for 20 min at 95 °C. Potassium and sodium ion content was determined with an atomic absorption spectrometer as above.
Yeast Membrane FractionationMicrosomal membranes were isolated as described (18) The microsomal membrane pellet (2 ml) was layered on a linear (28 ml) 2055% sucrose gradient prepared in 10 mM Tris-HCl, pH 7.5, 1 mM EDTA, 1 mM dithiothreitol, and 30 µl of protease inhibitor mixture (Sigma), and centrifuged 18 h at 100,000 x g in a Beckman SW28 swinging bucket rotor. 2-ml fractions were collected, and sucrose density and protein content determined.
Tomato Cell Membrane FractionationMicrosomal membranes were obtained from Tomato calli (L. esculentum Mill. cv. Pera) as previously described (37). Microsomal membranes were layered on a linear (14 ml) 2040% sucrose gradient and centrifuged as described above. 1-ml fractions were collected, and sucrose density and protein content determined.
Marker Enzyme AnalysisIn tomato cell membrane fractions latent UDPase activity (Golgi) (38) Antimycin A-insensitive NADH-cytochrome c reductase (ER)1 (39) and nitrate-sensitive ATPase (Tonoplast) (40) was measured. The LeNHX2 protein was detected by immunoblot analysis using the affinity-purified polyclonal antibody raised against the LeNHX2 c-terminal peptide EPIMHSSRRAGYDGH (Sigma-Genosys). In yeast membrane fractions marker enzyme proteins were detected by immunoblot analysis. The distribution of ER membranes was assayed by determination of NADPH-cytochrome c oxidoreductase activity (41). SDS-PAGE and Western blotting were performed as described (18) using a monoclonal antibody raised against the 100-kDa subunit of the vacuolar proton ATPase VPH1, a monoclonal antibody against the late Golgi protein vps10p, and a monoclonal antibody against the endosomal/prevacuolar protein pep12p (Molecular Probes). The recombinant LeNHX2 protein in yeast was detected using a monoclonal antibody raised against the RGSH4 epitope (Qiagen).
Purification of LeNHX2:H10 Protein by Ni2+ Affinity ChromatographyThe LeNHX2 protein was purified essentially as described for the AtNHX1 protein (18) with some modifications. Cells were grown in APG medium to an OD660 nm of 1.0. Microsomal membranes were isolated as described (18) after which the microsomal membrane fraction (4 ml, 10 mg of protein/ml in 100 mM Tris-HCl, pH 7.5, 20% glycerol, 0.1 mM dithiothreitol, and 0.1 mM EDTA) was mixed with 40 ml of solubilization buffer (50 mM KH2PO4, pH 7.4, 500 mM NaCl, 10 mM imidazole, 20% glycerol, 0.5% n-dodecyl--D-maltoside) supplemented with 200 µl of protease inhibitor mixture (Sigma) and incubated for 30 min at 4 °C under gentle shaking. Unsolubilized material was removed by centrifugation for 30 min at 30,000 x g (Sorvall SS34 rotor). The supernatant was mixed with 1 ml of Ni-nitrilotriacetic acid; resin (Qiagen) and incubated overnight at 4 °C. The resin was then poured into a polypropylene column and prewashed with an imidazole step-gradient of 8-ml fractions containing 20, 50, 75, and 100 mM imidazole (pH 7.4) in 50 mM KH2PO4 (pH 7.4), 500 mM NaCl, 10% glycerol, 0.075% n-dodecyl-
-D-maltoside, 2 µg/ml pepstatin, 0.2 mM phenylmethylsulfonyl fluoride. Finally, bound protein was washed with 4 ml of 20 mM BTP-Mes (pH 7.4), 100 mM imidazole, 10% glycerol, 0.075% n-dodecyl-
-D-maltoside, 2 µg/ml pepstatin, and 0.2 mM phenylmethylsulfonyl fluoride and eluted slowly in 10 x 0.5 ml of 20 mM BTP-Mes pH 7.4, 500 mM imidazole (pH 7.4), 10% glycerol supplemented with 2 µg/ml pepstatin, and 0.2 mM phenylmethylsulfonyl fluoride. The third fraction would normally contain 5075 µg of purified antiporter protein, corresponding to 65% of totally eluted antiporter protein. This fraction was frozen in liquid nitrogen and stored at 80 °C, until use for subsequent experiments.
Reconstitution of LeNHX2:H10 Protein and Measurement of Cation/H+ Exchange in VitroReconstitution was performed by elimination of detergent using Sephadex G-50 (fine; Amersham Biosciences) spin columns, and Biobeads (SM-2; Bio-Rad) as previously described (18) using 5 µg of protein and in the presence of ammonium sulfate. In order to encapsulate pyranine during the reconstitution, it was essential to preload the G-50 spin column with 200 µl of 2.5 mM pyranine (BTP salt) in reconstitution buffer, as the pyranine present in the liposome-protein-detergent mixture was eliminated by >99% at the top of the column. This shows that the reconstitution takes place along the passage of the sample through the column, allowing also an efficient elimination of imidazole or traces of KCl and NaCl in the protein sample. An inside acid pH gradient was created by diluting the proteoliposomes 50-fold in (NH4)2SO4-free medium. Cation/H+ exchange activity was monitored by measuring the rise in fluorescence of encapsulated pyranine in the presence of various monovalent cations as previously described (18). For measurement of antiporter activity in the absence of a preimposed pH gradient, ammonium sulfate in the reconstitution was replaced by Cs2SO4, pH during reconstitution was adjusted to 7.2, and measurements were made in the same buffer containing equilibrium Cs2SO4 concentration.
Affinity Purification of the LeNHX2 Polyclonal AntibodyA rabbit polyclonal antibody was raised against a peptide corresponding to the C-terminal 15 amino acids of the LeNHX2 protein (Sigma-Genosys). The antibody was purified from the serum by affinity purification using the LeNHX2 protein. 10 µg of purified protein was separated by SDS-gel electrophoresis and transferred to a polyvinylidene difluoride membrane. The band containing the protein was cut from the membrane, blocked, and incubated for 3 h with the serum at a 1:20 dilution in 1.5 ml of 20 mM K-phosphate, pH 7.5, 150 mM NaCl, 0.1% bovine serum albumin. After washing, the antibody was eluted with 750 µl of 0.2 M glycine, pH 2.7, 1 mM EGTA and neutralized with an equal volume of 0.2 M Tris-HCl, pH 8.0, 0.2% bovine serum albumin, 0.02% NaN3. The purified antibody solution was used at a 1:10 dilution in Western blot experiments.
Protein DeterminationProtein was determined by the method of Schaffner and Weissmann (42) with bovine serum albumin as standard.
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RESULTS |
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Expression Studies in PlantsPlant and yeast NHX genes are proposed to be involved in salinity or osmotolerance (13, 16, 23, 45). To test the involvement of the LeNHX2 protein in these processes we subjected tomato plants of 5-week-old grown in vermiculite to a shock of 130 mM NaCl. The LeNHX2 gene showed a rapid induction by salt stress or the stress hormone abscisic acid in leaves, but was constitutively expressed in stems and roots (Fig. 3), indicating a role of this protein in the salt or osmotic stress response.
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Yeast Complementation StudiesDisruption of the NHX1 gene in S. cerevisiae confers a strong hygromycin B sensitivity to the cells (Fig. 4C), as has been reported by others (12, 23, 46). LeNHX2 could efficiently complement this sensitivity. The effect on salt sensitivity of NHX1 disruption and complementation by the plant gene was studied using a yeast strain with additional disruptions in the plasma membrane Na+ efflux systems ENA1-4 and NHA1 (23). An effect of the NHX1 disruption on NaCl sensitivity was observed already at 20 mM NaCl (Fig. 4B). The tomato gene could partly compensate for NHX1 disruption in this strain. We could not demonstrate any effect of LeNHX2 expression on Li+ sensitivity (data not shown).
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Effect of LeNHX2 Expression on Intracellular Na+ and K+ Content in YeastIn normal growth conditions no effect of NHX1 disruption or complementation by the LeNHX2 gene on intracellular K+ concentrations could be observed (Fig. 5A). K+ content was however much lower in NHX1-disrupted cells as compared with the wild-type cells or cells expressing LeNHX2 when intracellular K+ content was compromised by growing the cells in 20 mM NaCl (Fig. 5B). Intracellular Na+ content was similar for all strains tested in these conditions, indicating that the NHX1 or LeNHX2 protein does not contribute to Na+ accumulation (Fig. 5B). To determine whether the loss in K+ was due to a diminution of the cytoplasmic or vacuolar K+ concentration, we treated the cells with cytochrome c, which selectively permeabilizes the plasma membrane (35, 36). Cytoplasmic K+ content was very similar for all strains, but the control strain or the strain expressing LeNHX2 had 23-fold higher vacuolar K+ content (Fig. 5C).
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Detection of LeNHX2 in Membrane Fractions of Yeast CellsA sequence encoding a C-terminal RGSH10 epitope tag was added to LeNHX2 after which it was inserted in vector pYes (Invitrogen) harboring the GAL1 promoter. The presence of the tagged LeNHX2 protein in AXT3 cells conferred resistance to hygromycin and NaCl when cells were grown on galactose-containing media and still resulted in higher levels of intracellular K+, but not Na+ (data not shown), indicating that the protein was functional. The tagged LeNHX2 protein was readily detected in microsomal membranes isolated from galactose-grown cells using a monoclonal antibody raised against the RGSH4 epitope. In a linear sucrose gradient, the LeNHX2 protein equilibrated in low density sucrose fractions corresponding to vacuolar or endomembranes, and clearly separated from higher density mitochondrial or plasma membrane markers (data not shown). In more detail, the LeNHX2 protein had a distribution pattern similar to the late Golgi marker vps10p and, to a lesser extent, the endosomal/prevacuolar marker pep12p. The vacuolar marker VPH1 equilibrated at slightly higher sucrose densities (17) (Fig. 6).
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Detection of LeNHX2 in Membrane Fractions of Tomato CellsTo detect the LeNHX2 protein in plant membrane fractions, we obtained a polyclonal antibody raised using a peptide corresponding to the extreme C-terminal 15 amino acids (Sigma-Genosys). In yeast, this antibody detected a 50-kDa protein only in cells expressing the LeNHX2 protein (data not shown). After fractionation of tomato cell microsomes on a linear sucrose gradient, the LeNHX2 protein comigrated with the markers for Golgi and vacuolar membranes (Fig. 7).
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Purification of His-tagged LeNHX2 Protein and Cation/H+ Antiport ActivityThe tagged LeNHX2 protein was purified by Ni2+ affinity chromatography (Fig. 8A) and reconstituted in proteoliposomes containing the pH indicator pyranine. After creation of an inside acid pH gradient, the capacity of monovalent cations to dissipate the pH gradient was assayed (Fig. 8B). In the presence of K+ a significant internal alkalinization could be observed, especially at concentrations above 100 mM. The exchange reaction was much less efficient in the presence of Na+. In the presence of Li+ or Cs+ only a residual activity was observed. The exchange reaction showed sigmoidal kinetics as a function of substrate concentration, indicating allosteric effects (Fig. 8C). The same ionic specificity was observed when the exchange reaction was assayed in the absence of a preimposed pH gradient although the exchanger was much less efficient in these conditions (Fig. 9A). The exchange reaction was only slightly inhibited by the amiloride analogs EIPA and Benzamil (Fig. 9B).
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DISCUSSION |
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Expression Studies in PlantsIn Arabidopsis, 6 isoforms of the NHX family were described (16). The LeNHX1 protein is closely related to proteins AtNHX1 to AtNHX3 while the LeNHX2 protein is closely related to a different subgroup of plant NHX proteins and shows highest sequence homology to the AtNHX5 protein (Fig. 1). The LeNHX2 gene is ubiquitously expressed but we could show a modest increase in transcript levels in aerial parts of tomato plants by short term NaCl stress or treatment with the plant stress hormone abscisic acid, indicating a role for this protein in osmotic stress in plants (Fig. 3). The AtNHX5 gene was also shown to be induced by NaCl stress in Arabidopsis seedlings (16), but not by abscisic acid treatment. This would indicate that similar isoforms are under control of differential regulatory pathways in different plant species. Such discrepancies were also suggested from studies comparing the expression of isoforms from halophytic species like Mesembryanthemum crystallinum and Atriplex gmelini with those of Arabidopsis and rice (13, 2326).
Yeast Complementation StudiesIn yeast NHX1 is the only member of the intracellular antiporter family (16). A role for NHX1 in yeast salinity tolerance was demonstrated, but for unknown reasons the protein is also involved in conferring resistance to other toxic cations like hygromycin B (12, 45). We show that the plant LeNHX2 gene can complement the salt- and hygromycin-sensitive phenotypes caused by NHX1 disruption (Fig. 4).
Yeast achieves salt tolerance mainly through exclusion of toxic sodium ions at the plasma membrane through the operation of a plasma membrane Na+ pump and Na+/H+ antiporter (23, 47). A disruption of these plasma membrane Na+ efflux systems results in a dramatic increase in the intracellular Na+/K+ ratio when the cells are grown in the presence of NaCl (48, 49). An effect of NHX1 gene disruption on salt sensitivity is most clearly demonstrated in this yeast strains. However, even in these conditions a role of NHX1 in salt tolerance can only be observed when cells are grown at low K+ concentrations (23), indicating that potassium ion homeostasis is important for the observed phenotype.
We now show that under salt stress conditions in this strain, intracellular K+ concentrations are strongly affected by the disruption of the NHX1 gene, which can be complemented by the tomato antiporter LeNHX2 (Fig. 5B). Under the mild NaCl stress conditions used we could not detect any effect on intracellular Na+ concentrations (Fig. 5B). Similar results were obtained recently studying the effects of AtNHX1, 2 and 5 in yeast (16). A minor increase in Na+ concentration could be observed only in yeast cells expressing AtNHX1, while no increases were observed in cells expressing AtNHX5. On the contrary, all isoforms caused a very significant increase of intracellular K+ concentrations as compared with the NHX1-disrupted strain, the most efficient being AtNHX5. By treating the cells with cytochrome c, we could show that in salt stress conditions the NHX1 disruption and complementation by LeNHX2 affects K+ concentrations in vacuolar or intracellular compartments, while cytoplasmic K+ concentrations remain similar (Fig. 5C). This suggests that the accumulation of K+ in intracellular compartments by NHX1 or LeNHX2 plays an important role for growth at limiting cytoplasmic K+ concentrations. On the other hand, we did not obtain evidence for the involvement of LeNHX2 in the active accumulation of K+ inside vacuoles in the absence of salt stress (Fig. 5A).
It has been proposed that in plants Na+ ions can replace K+ ions for osmotic adjustment in the vacuolar pool upon conditions of salt stress (1). Also in yeast, the accumulation of salt in vacuoles by the ScNHX1 protein would reduce the concentration of toxic Na+ ions in the cytoplasm, thereby improving salt tolerance (12, 17, 23). Our data show that K+ homeostasis of intracellular compartments is an additional toxicity target of salt stress in plants and yeast. Essential cellular processes like regulation of pH in organelles of the secretory pathway might rely on the presence of K+/H+ antiporters at these organelle using the readily available K+, while vacuolar pH and Na+ concentrations are controlled by distinct Na+/H+ antiporters. It was indeed shown that disruption of NHX1 in yeast does not abolish pH-dependent Na+/H+ antiport activity in vacuolar vesicles (50). In summary, our data indicate that the physiologically significant activity of NHX1 and LeNHX2 is K+/H+ and not Na+/H+ antiport.
Biochemical Characterization of LeNHX2Accumulation of K+ in intracellular compartments is consistent with the observed distribution of the LeNHX2 protein in a linear sucrose gradient (Figs. 6 and 7). Furthermore, we demonstrated that the purified LeNHX2 protein specifically transports K+, exhibiting very low activities with other monovalent cations (Figs. 8B and 9A). Previously, we showed that the AtNHX1 protein is a less specific monovalent cation/H+ antiporter, with similar affinities for K+ and Na+ (18). These data are consistent with the effect of AtNHX1, but not LeNHX2 or AtNHX5 on intracellular Na+ concentrations in yeast (16). In contrast to the AtNHX1 protein, that exhibited simple saturation kinetics with Km values for K+ or Na+ of around 40 mM, the LeNHX2 protein shows sigmoidal kinetics as a function of K+ concentration suggesting more than one K+ binding site that show positive cooperativity (Fig. 8C). This results in a strong dependence of the activity on K+ concentrations in the range from 50 to 150 mM K+, which is in accordance with the concentrations normally found in the cytoplasm of plant cells (3). The lower Km values obtained for the AtNHX1 protein strengthen a role for this enzyme in vacuolar Na+ accumulation, as cytoplasmic Na+ concentrations are suggested to be much lower. Allosteric kinetics with respect to Na+ were only reported for the mammalian isoform NHE4, while the majority of mammalian isoforms function at maximal turnover rates with respect to Na+, but exhibit allosteric kinetics with respect to H+ resulting in a strong activation by a decrease in cytoplasmic pH (51). At the same time, a variety of effector molecules or posttranslational modifications such a phosphorylation or dephosphorylation could modify the K+ activation profile. In the absence of a preimposed pH gradient, addition of KCl also induced the rapid formation of proton efflux from the vesicles (Fig. 9A). The LeNHX2 protein contains the typical motives that are suggested to be involved in amiloride binding and inhibition (Fig. 2) (5254). Nevertheless, unlike our previous results obtained with the reconstituted AtNHX1 protein (18), the LeNHX2 protein was only slightly inhibited by amiloride analogs (Fig. 9B). It has to be noted that in the reconstituted system we could not assay higher concentrations of inhibitors, as these compounds interfere with membrane permeability (18).
In conclusion, we have cloned two genes from the NHX antiporter family in tomato. The LeNHX2 gene encodes the first intracellular K+/H+ antiporter in plants, and our data indicate that the control of K+ concentrations and pH in intracellular compartments by this enzyme is important for ion homeostasis and salt tolerance in plants and yeast. Finally, the resemblance of the phenotype of cells expressing ScNHX1 with that of cells expressing LeNHX2 suggests that LeNHX2 might be the true functional homologue of the ScNHX1 gene.
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FOOTNOTES |
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To whom correspondence should be addressed. Tel.: 34-958-181600; Fax: 34-958-129600; E-mail: kev{at}eez.csic.es.
1 The abbreviations used are: ER, endoplasmic reticulum; Mes, 4-morpholineethanesulfonic acid; BTP, 1,3-bis[tris(hydroxylmethyl)-methylamino]propane; EIPA, ethylisopropyl-amiloride.
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ACKNOWLEDGMENTS |
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REFERENCES |
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