Phenylarsine Oxide Inhibits the Fusicoccin-Induced Activation of Plasma Membrane H+-ATPase

doi:10.1104/pp.122.2.463

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Phenylarsine Oxide Inhibits the Fusicoccin-Induced Activation of Plasma Membrane H⁺-ATPase¹

Claudio Olivari,^* Cristina Albumi, Maria Chiara Pugliarello, and Maria Ida De Michelis

Dipartimento di Biologia dell'Università degli Studi di Milano, Centro di Studio del Consiglio Nazionale delle Ricerche per la Biologia Cellulare e Molecolare delle Piante, via G. Celoria 26, I-20133 Milano, Italy.

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

To investigate the mechanism by which fusicoccin (FC) induces the activation of the plasma membrane (PM) H⁺-ATPase, we used phenylarsine oxide (PAO), a known inhibitor ofprotein tyrosine-phosphatases. PAO was supplied in vivo in theabsence or presence of FC to radish (Raphanus sativus L.) seedlingsand cultured Arabidopsis cells prior to PM extraction. Treatmentwith PAO alone caused a slight decrease of PM H⁺-ATPase activity and, in radish, a decrease of PM-associated 14-3-3proteins. When supplied prior to FC, PAO drastically inhibitedFC-induced activation of PM H⁺-ATPase, FC binding to the PM, and the FC-induced increase ofthe amount of 14-3-3 associated with the PM. On the contrary,PAO was completely ineffective on all of the above-mentioned parameterswhen supplied after FC. The H⁺-ATPase isolated from PAO-treated Arabidopsis cells maintainedthe ability to respond to FC if supplied with exogenous, nonphosphorylated14-3-3 proteins. Altogether, these results are consistent witha model in which the dephosphorylated state of tyrosine residuesof a protein(s), such as 14-3-3 protein, is required to permitFC-induced association between the 14-3-3 protein and the PM H⁺-ATPase.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

The H⁺-ATPase is the most important ion pump in the plant plasma membrane (PM), playing a crucial role in several aspects ofplant physiology; it is regulated in vivo by several endogenousand environmental factors (Marré et al., 1993; Palmgren, 1998).One of the best characterized modulators to date is the phytotoxinfusicoccin (FC), which rapidly and strongly stimulates electrogenicproton extrusion in a variety of higher plants (Marré, 1979;Marré et al., 1992; Palmgren, 1998). The FC-induced activationof H⁺-ATPase causes a shift in the pH optimum of the enzyme towardmore alkaline values and a decrease in the apparent K_m for thesubstrate Mg-ATP (Rasi-Caldogno and Pugliarello, 1985; Rasi-Caldognoet al., 1986, 1993; De Michelis et al., 1991; Johansson et al.,1993; Olivari et al., 1993; Lanfermeijer and Prins, 1994).

Different experimental approaches have allowed the identification of a C-terminal autoinhibitory domain on the H⁺-ATPase of higher plants. This domain is involved in FC-inducedactivation of the H⁺-ATPase, which depends on a conformational modification of theenzyme, leading to the displacement of the C terminus (Palmgrenet al., 1990, 1991; Johansson et al., 1993; Rasi-Caldogno et al.,1993; Regenberg et al., 1995).

It has recently been shown that the activation of the PM H⁺-ATPase by FC is caused by the FC-induced association between theC-terminal domain of the enzyme and member(s) of the 14-3-3 proteinfamily (Oecking et al., 1997; Baunsgaard et al., 1998; Fulloneet al., 1998; Piotrowsky et al., 1998; Oecking and Hagemann, 1999).On the other hand, the C-terminal domain of the PM H⁺-ATPase does not contain any sequence similar to the known 14-3-3binding motifs RSX_1,2pSXP (Muslin et al., 1996; Yaffe et al.,1997) in which the phosphorylation of the Ser residue is crucialfor the binding of 14-3-3 to target proteins. Recent data suggestthat in spinach, the phosphorylation of Thr-948 localized at theC terminus could modulate the FC-induced association between 14-3-3proteins and the C terminus domain of PM H⁺-ATPase (Olsson et al., 1998). However, 14-3-3 proteins also bindto the H⁺-ATPase independently of FC (Fullone et al., 1998), and this FC-independentbinding is phosphorylation dependent and also occurs in a truncatedH⁺-ATPase lacking the C-terminal domain (Jahn et al., 1998).

To understand the physiological factors modulating the interaction between the PM H⁺-ATPase and 14-3-3 proteins, we used an inhibitor of Tyr-specificprotein phosphatase (PTP) to investigate the possible involvementof phosphorylation-dephosphorylation of Tyr residues. We showthat in vivo treatment of radish (Raphanus sativus L.) seedlingsand cultured Arabidopsis cells with phenylarsine oxide (PAO),a known inhibitor of PTPs (Garcia-Morales et al., 1990; Heimovaara-Dijkstraet al., 1996; Knetsch et al., 1996), inhibits the formation ofthe FC-H⁺-ATPase-14-3-3 complex and thus the FC-induced activation of thePM H⁺-ATPase.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Plant Material and in Vivo Treatments

The method for germination of radish (Raphanus sativus L. cv Tondo Rosso Quarantino, Ingegnoli, Milan) seeds was previouslypublished (De Michelis et al., 1996). In vivo treatments withFC (5 µM, final concentration) and/or PAO were performed after21 h of germination for the times specified in the figure legends.After the treatments the seedlings were frozen at $-$ 80°C. PAO wasdissolved in dimethyl sulfoxide (DMSO) (10 mM stock solution),and supplied at the final concentrations indicated in the figurelegends.

Cell-suspension cultures of Arabidopsis ecotype Landsberg were grown as described in Curti et al. (1993). In vivo treatmentswith FC and/or PAO were performed by adding the two effectorsto the culture medium at the final concentrations and for thetimes specified in the figure legends. At the end of the treatmentsthe cells were collected by centrifuging the samples twice at1,000g for 5min.

Isolation of PM

A PM-enriched fraction from germinating radish seedlings was obtained by an aqueous two-phase partitioning system, as previouslydescribed (Rasi-Caldogno et al., 1995).

Arabidopsis cells harvested from 6-d-old subcultures were homogenized in ice-cold extraction medium (2 mL/1 g of fresh weight);a microsomal fraction was obtained essentially as previously described(Rasi-Caldogno et al., 1995). A highly purified PM fraction wasobtained by a two-step aqueous two-phase partitioning system containing6.2% (w/w) Dextran T500 (Pharmacia Biotech, Piscataway, NJ), 6.2%(w/w) PEG 3350 (Sigma-Aldrich, St. Louis), 11% (w/w) Suc, 5 mMpotassium phosphate buffer (pH 7.8), and 1 mM or 5 mM KCl in thefirst- and second-phase systems, respectively. The final upperphase was diluted 5-fold with 1 mM Bis-Tris propane-4-(2-hydroxyethyl)-1-piperazineethanesulfonicacid (BTP-HEPES), pH 7.0, 0.1 mM EGTA, 3 mM dithiothreitol (DTT),10% (v/v) glycerol, 1 mM phenylmethylsulfonyl fluoride (PMSF),and 0.1 mg mL¹ polyoxyethylene 20 cetyl ether (Brij 58), and centrifuged at48,000g for 35 min. The obtained pellets were resuspended in 10%(v/v) glycerol, 0.5 mM DTT, and 1 mM 3-(N-morpholino)-propanesulfonicacid (MOPS)-KOH (pH 7), and frozen at $-$ 80°C. Membrane proteinswere assayed according to the method of Markwell et al. (1978).

PM H⁺-ATPase Activity

The PM H⁺-ATPase activity of PM isolated from cultured Arabidopsis cells was assayed in 0.2 mM EGTA, 50 mM KNO₃, 3 mM MgSO₄,5 mM (NH₄)₂SO₄, 0.1 mM ammonium molybdate, 1 µg mL¹ oligomycin, 0.1 mg mL¹ Brij 58, 5 µM carbonyl cyanide p-(trifluoromethoxy)phenyl-hydrazone,40 mM BTP-2-(N-morpholino)-ethanesulfonic acid (BTP-MES) (pH 6.0-6.7),or BTP-HEPES (pH 6.8-7.5), 2 units mL¹ pyruvate kinase, 1 mM phosphoenolpyruvate (PEP), and 1 mM ATP(unless otherwisespecified).

The PM H⁺-ATPase activity of PM isolated from germinating radish seedlings was assayed in the same assay medium without pyruvatekinase or PEP but with 3 mM ATP and 5 mM MgSO₄.

PMs (5-20 µg of protein) were incubated in 250 µL of assay medium and the reaction was carried out for 60 min at 30°C. ReleasedPi was determined as described in De Michelis and Spanswick (1986).The PM H⁺-ATPase activity was evaluated as the difference between totalactivity and that measured in the presence of 100 µMvanadate.

FC Radioimmunoassay

Antiserum against bovine serum albumin (BSA)-conjugated dideacetyl-FC was kindly supplied by P. Aducci and M. Marra (Dipartimentodi Biologia, Università di Roma Tor Vergata, Rome). [³H]FC (0.7 kBq pmol¹) was a generous gift of Prof. G. Randazzo (Università di Napoli,Italy). The FC radioimmunoassay was performed as previously described(De Michelis et al., 1996).

FC Binding

FC binding was assayed essentially as described in Rasi-Caldogno et al. (1993), except that membranes (100 µg of protein)were incubated in 1 mM MOPS-KOH, pH 7, 10% (v/v) glycerol, 0.5mM DTT, 5 mM MgSO₄, and 0.1 mg mL¹ Brij 58 (200 µL of final volume) in the presence of 5 nM [³H]dihydrofusicoccin ([³H]FC). Unspecific binding, evaluated in the presence of 10 µMunlabeled FC, was subtracted from all of the binding values toobtain specificbinding.

SDS-PAGE

Samples were treated as reported in Rasi-Caldogno et al. (1993). SDS-PAGE was performed essentially according to the methodof Laemmli (1970). About 10 to 20 µg of protein were loaded ontoa 4% to 20% gradient polyacrylamide Tris-Gly Ready Mini Gel (catalogno. 161-0903, Bio-Rad Laboratories, Hercules, CA), and subjectedto electrophoresis under standardconditions.

Western-Blot Analysis

After SDS-PAGE, the polypeptides were electrophoretically transferred to a 0.2-µm nitrocellulose membrane (reference no. 401391, Schleicher & Schull, Keene, NH). The blot was incubated for2 h with anti-N terminus H⁺-ATPase polyclonal antibody diluted 1:1,000 (Olivari et al., 1998)or with anti-14-3-3 polyclonal antibody diluted 1:1,000 (Marraet al., 1994), kindly supplied by P. Aducci and M. Marra (Dipartimentodi Biologia, Università di Roma Tor Vergata, Rome). Immunodecorationwas performed with anti-rabbit IgG conjugated with alkaline-phosphatase(Sigma-Aldrich) for H⁺-ATPase and with anti-rabbit IgG conjugated with horseradish peroxidase(catalog no. 170-6463, Bio-Rad) for 14-3-3 proteins. Detectionof the PM H⁺-ATPase was performed by using 5-bromo-4-chloro-3-indolyl phosphate-nitrobluetetrazolium (BCIP-NBT) alkaline phosphatase substrate (B-5655,Sigma-Aldrich). Detection of the 14-3-3 proteins was performedwith an enhanced chemiluminescence system (RPN 2209, Amersham-PharmaciaBiotech,Uppsala).

Statistics

Data reported in the figures are the results from one experiment with three replicates, representative of at least two experiments,each performed on an independent PM preparation; SE of the assaysdid not exceed 3% of the measuredvalues.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Effect of PAO on PM H⁺-ATPase Activity

In a first set of experiments, we tested the effect of PAO supplied in vivo to radish seedlings and cultured Arabidopsis cellson the PM H⁺-ATPase activity. Figure 1 shows the H⁺-ATPase activity (measured at pH 6.4) in PM isolated from bothplant materials after 3 h of incubation in the presence of differentconcentrations of PAO. In both plant materials, treatment withPAO caused a partial decrease of PM H⁺-ATPase activity. In radish, the highest concentration of PAOtested (100 µM) decreased the enzyme activity by about 30%, whilein Arabidopsis the same concentration of PAO decreased the PMH⁺-ATPase activity by less than 20%. PAO supplied in vitro to PMisolated from both plant materials was completely ineffective(data not shown).

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Figure 1. Effect of increasing concentrations of PAO on the PM H⁺-ATPase activity. Radish seedlings ( $open circle$ ) and cultured Arabidopsis cells ( $triangle$ ) were treated with PAO for 180 min prior to PM isolation. PM H⁺-ATPase activity, assayed at pH 6.4, is expressed as a percentage of that measured in the absence of PAO (0.30 µmol min¹ mg¹ protein for radish seedlings; 1.40 µmol min¹ mg¹ protein for Arabidopsis).

Effect of PAO on FC-Induced Activation of the PM H⁺-ATPase

In all plant materials tested, FC fed in vivo strongly stimulated the PM H⁺-ATPase. This activation causes a shift in the pH optimum of theenzyme toward more alkaline values and a decrease in the apparentK_m for the substrate Mg-ATP (Rasi-Caldogno and Pugliarello, 1985;Rasi-Caldogno et al., 1986; Schulz et al., 1990; De Michelis etal., 1991; Johansson et al., 1993; Olivari et al., 1993). Thus,FC-induced stimulation of the PM H⁺-ATPase is much stronger when the enzyme activity is assayed atpH values typical of the cytoplasm of a plant cell (pH 7.5) thanat the relatively acidic pH optimum for enzyme activity (pH 6.4-6.6).Therefore, the ratio between the activity measured at pH 6.4 andthat measured at pH 7.5 (pH ratio) is lower in PM isolated fromplant material treated in vivo with FC compared with that measuredin untreated tissue, and the pH ratio is an useful parameter withwhich to monitor the activation state of the PM H⁺-ATPase (Olivari et al., 1998).

We determined whether PAO affected the FC-induced activation of the PM H⁺-ATPase. Radish seedlings and cultured Arabidopsis cells wereuntreated or treated in vivo with PAO alone, 5 µM FC alone, orpretreated with PAO followed by FC. The pH dependence of the enzymeactivity in isolated PMs was then analyzed. Figure 2 shows thatin both plant materials pretreatment with 100 µM PAO completelyprevented the FC-induced increase of PM H⁺-ATPase activity at pHs above the optimum, so that the pH curveof PMs from PAO-pretreated cells became similar to that of controlPMs. This is highlighted by the pH ratio values (inserts to Fig.2), which become similar to those of control PM in radish seedlings(Fig. 2A), and even higher in cultured Arabidopsis cells (Fig.2B). Figure 2 also shows that, even in the absence of a treatmentwith FC, the inhibition of the PM H⁺-ATPase activity caused by pretreatment with 100 µM PAO slightlyincreased with the increase of pH, so that the pH ratio for theH⁺-ATPase activity of PMs from PAO-pretreated cells becomes higherthan that of control PMs. These results suggest that treatmentwith PAO, aside from inhibiting FC-induced activation of the PMH⁺-ATPase, also decreases its basal activation state.

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Figure 2. Effect of PAO on the pH dependence of the PM H⁺-ATPase activity. PM was isolated from radish seedlings (A) and cultured Arabidopsis cells (B) untreated ( $open circle$ , C), pretreated with 100 µM PAO for 180 min (

, PAO), pretreated with 5 µM FC for 120 min ( $triangle$ , FC), or pretreated with 100 µM PAO for 60 min followed by a treatment with 5 µM FC for 120 min ( $black-triangle$ , PAO,FC). PM H⁺-ATPase activity is expressed as a percentage of that measured at pH 6.2 for radish seedlings (C = 0.31; PAO = 0.21; FC = 0.28; PAO,FC = 0.21 µmol min¹ mg¹ protein) and at pH 6.0 for Arabidopsis (C = 0.56; PAO = 0.46; FC = 0.46; PAO,FC = 0.27 µmol min¹ mg¹ protein).

Figure 3 shows the dose-response plot of the PM H⁺-ATPase activity assayed at pH 6.4 and 7.5 (and the correspondent pH ratios).Radish seedlings (Fig. 3A) and cultured Arabidopsis cells (Fig.3B) were pretreated in vivo with different concentrations of PAOfollowed by treatment with 5 µM FC. In both plant materials, thedecrease of the PM H⁺-ATPase activity was more dramatic when assayed at pH 7.5 at allconcentrations of PAO tested, so that the pH ratio progressivelyincreased with PAO concentration. The inhibition of FC-inducedactivation of the PM H⁺-ATPase was half maximal at about 30 µM PAO, a concentration onlyslightly higher than those used to inhibit Tyr phosphorylationin animal cells or plant protoplasts (Garcia-Morales et al., 1990;Heimovaara-Dijkstra et al., 1996; Knetsch et al., 1996).

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Figure 3. Inhibiting effect of PAO on FC-induced activation of the PM H⁺-ATPase. PM H⁺-ATPase activity was measured at pH 6.4 (gray bars) or pH 7.5 (white bars) in PM isolated from radish seedlings (A) and cultured Arabidopsis cells (B) treated with increasing concentrations of PAO for 60 min, followed by a treatment with 5 µM FC for 120 min. Numbers on top of the white bars represent the corresponding pH ratios.

We then evaluated whether FC was able to prevent the effect of PAO. Figure 4 shows the effect of PAO supplied to culturedArabidopsis cells prior to or after FC on the PM H⁺-ATPase activity assayed at pH 6.4 and 7.5 and on the correspondingpH ratios. The results indicate that, when supplied after FC,PAO was unable to reverse the FC-induced activation of the PMH⁺-ATPase.

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Figure 4. PAO is unable to revert FC-induced activation of the PM H⁺-ATPase. PM H⁺-ATPase activity was measured at pH 6.4 (gray bars) or pH 7.5 (white bars) in PM isolated from cultured Arabidopsis cells pretreated with 5 µM FC for 180 min (FC), pretreated with 100 µM PAO for 60 min followed by a treatment for 120 min with FC (PAO,FC), or pretreated with 5 µM FC for 60 min followed by a treatment for 120 min with 100 µM PAO (FC,PAO). Numbers on top of the white bars represent the corresponding pH ratios.

Effect of PAO on FC Binding to the PM

To better investigate which step of the mechanism leading to FC-induced activation of the PM H⁺-ATPase was affected by PAO, we tested the effect of the inhibitoron FC binding to the PM upon in vivo and in vitro treatment withFC. Figure 5 shows the effect of pretreatment with increasingconcentrations of PAO on FC binding to the PM upon treatment ofradish seedlings with 5 µM FC. Data obtained indicate that pretreatmentwith PAO inhibited FC binding to the PM with the same concentrationdependence as monitored for FC-induced activation of the PM H⁺-ATPase (compare with Fig. 3A). Moreover, in PM isolated fromcultured Arabidopsis cells treated with PAO, the binding of FCsupplied in vitro to PM was almost completely inhibited comparedwith that measured on control PM: 0.21 pmol FC mg¹ protein versus 1.46 pmol FC mg¹ protein, respectively.

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Figure 5. Effect of PAO on FC binding to the PM. PM was isolated from radish seedlings treated with increasing concentrations of PAO followed by a treatment with 5 µM FC. The amount of FC bound to PM upon in vivo treatment was evaluated by FC radioimmunoassay.

It has been shown that FC binding to the PM involves an interaction between the C terminus of the H⁺-ATPase and members of the 14-3-3 protein family (Oecking et al.,1997; Baunsgaard et al., 1998; Fullone et al., 1998; Piotrowskyet al., 1998; Oecking and Hagemann, 1999) and that FC stronglyenhances the amount of PM-associated 14-3-3 proteins (De Micheliset al., 1996; Jahn et al., 1997; Oecking et al., 1997, Olivariet al., 1998). Thus, we checked the effect of PAO on the amountof 14-3-3 proteins associated with the PM. Figure 6 shows westernanalysis of PM isolated from radish seedlings or cultured Arabidopsiscells untreated or treated with PAO alone, FC alone, or PAO suppliedprior to or after the treatment with FC. The blots were immunodecoratedwith polyclonal antibodies raised against the N-terminal domainof the PM H⁺-ATPase (Olivari et al., 1998) or against 14-3-3 proteins (Marraet al., 1994). In the first case, the antibody identified a singleband of 100 kD, the intensity of which was similar in the differentlanes, indicating that PAO had no major effect on the PM H⁺-ATPase amount. In radish, the intensity of the band at 30 kD,identified by the anti-14-3-3 antibody, was reduced by treatmentwith PAO supplied in vivo alone, indicating that PAO decreasesthe association of 14-3-3 proteins with the PM. In Arabidopsis,the band at 30 kD was barely affected by the same treatment. Asreported for different plant materials (Korthout and de Boer,1994; Oecking et al., 1994; Jahn et al., 1997; Baunsgaard et al.,1998; Fullone et al., 1998; Olivari et al., 1998), FC stronglyincreased the amount of 14-3-3 associated with the PM both ofradish and moreso of Arabidopsis. Pretreatment with PAO completelyprevented the FC-induced increase of PM-associated 14-3-3 proteinsin both plant materials. On the contrary, when supplied afterFC, PAO was unable to reverse the FC-induced increase of 14-3-3proteins associated with the PM.

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Figure 6. Effect of PAO on the amount of PM-associated 14-3-3 proteins. PM was isolated from radish seedlings or cultured Arabidopsis cells untreated (C), pretreated with 100 µM PAO (PAO), pretreated with 5 µM FC (FC), pretreated with 100 µM PAO followed by a treatment with 5 µM FC (PAO,FC), or with 5 µM FC followed by a treatment with 100 µM PAO (FC,PAO). After SDS-PAGE and western blotting, immunodecoration was performed with an anti-N-terminal H⁺-ATPase polyclonal antibody and with an anti-14-3-3 polyclonal antibody.

Effect of PAO on the Activation of the PM H⁺-ATPase of Arabidopsis by GF 14-6 14-3-3 and FC

All data presented so far indicate that PAO abolishes the FC-induced activation of the PM H⁺-ATPase by hampering the association between 14-3-3 proteins andthe enzyme. The simplest hypothesis to explain these data is thatPAO affects the phosphorylation state of relevant Tyr residueslocated on the amino acid sequences of the PM H⁺-ATPase or of 14-3-3 proteins. The availability of recombinant14-3-3 (Fullone et al., 1998) allowed us to determine whetherthe PM H⁺-ATPase from Arabidopsis cells pretreated with PAO maintainedthe capability to respond to FC when supplied with 14-3-3. Figure7 shows the PM H⁺-ATPase activity of control PM and PM from PAO-treated cells measuredin the presence or absence of 5 µM FC alone or supplied with 20µg mL¹ GF 14-6 14-3-3. The data indicate that, as for several plantmaterials (Blum et al., 1988; Olivari et al., 1993), in vitroaddition of FC essentially did not stimulate the H⁺-ATPase activity, while the simultaneous supply of GF 14-6 14-3-3and FC to control PM caused a dramatic activation: by about 100%,of the H⁺ATPase, which is similar to that reported in yeast expressingArabidopsis PM H⁺-ATPase AHA2 (Baunsgaard et al., 1998). In PM from PAO-treatedcells, the simultaneous supply of GF 14-6 14-3-3 and FC causedthe activation of the H⁺ATPase to a similar extent monitored for control PM, suggestingthat PAO treatment does not affect the H⁺ATPase responsiveness to FC. The addition of GF 14-6 14-3-3 aloneslightly increased the activity of the enzyme of PM from bothcontrol and PAO-treated cells.

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Figure 7. Effect of recombinant GF 14-6 and FC on the PM H⁺-ATPase activity of PM isolated from cultured Arabidopsis cells untreated (hatched bars) or treated with 100 µM PAO (white bars). PMs (1.5 µg of proteins) were incubated with or without 5 µM FC and with or without 2 µg of GF 14-6 in 50 µL of assay medium (pH 7.3) without ATP, PK, and PEP at 30°C for 30 min. The volume was adjusted to 100 µL with assay medium added with pyruvate kinase, PEP, and ATP (0.3 mM final concentration); the reaction was carried out for 60 min at 30°C.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

In this paper we have shown that PAO, a known inhibitor of PTPs (Garcia-Morales et al., 1990; Heimovaara-Dijkstra et al.,1996; Knetsch et al., 1996), supplied in vivo to radish seedlingsor cultured Arabidopsis cells, completely prevents the FC-inducedactivation of PM H⁺-ATPase. In fact, the pH dependence of H⁺-ATPase activity of PM from cells treated first with PAO thenwith FC becomes similar to that of control PM (Fig. 2). This revealsan increasing effect at pH values above the optimum of the H⁺-ATPase activity, where the FC-induced activation is much strongerand more relevant is the autoinhibitory effect of C-terminal domain(Rasi-Caldogno and Pugliarello, 1985; Rasi-Caldogno et al., 1986;Schulz et al., 1990; De Michelis et al., 1991, 1993; Johanssonet al., 1993; Olivari et al., 1993, 1998). The effect of PAO isdue to the inhibition of FC binding to PM (Fig. 5); in fact, bothFC binding and inhibition of the FC-induced activation of H⁺-ATPase show the same dose-response relationship, being completelyabolished by 100 µM PAO (Figs. 3 and 5). Treatment with 100 µMPAO also suppressed the FC-induced increase of PM-associated 14-3-3proteins (Fig. 6). Our results indicate that PAO prevents theFC-induced association between 14-3-3 proteins and the C terminusof the H⁺ATPase.

Treatment with PAO also caused a slight general decrease of PM H⁺-ATPase activity, which was particularly evident in the absenceof FC (Fig. 1). This effect, which requires PAO concentrationshigher than those effective on FC-induced activation of the enzyme,may reflect some nonspecific action of PAO on metabolism (Gibsonet al., 1989), which would require further investigation. It isnoteworthy, however, that in the absence of FC, PAO also causesa decrease of the activation state of the PM H⁺-ATPase (compare the pH ratios of PM from PAO-treated cells withthat of control PM in Fig. 2) and, at least in radish, this correlateswith a reduced amount of 14-3-3 proteins associated with the PM(Fig. 6). This result suggests that the association of 14-3-3proteins may be important in regulating the PM H⁺-ATPase activity independently ofFC.

The inhibitory effect of PAO was completely prevented when it was supplied after FC (Fig. 4), suggesting that once the FC-inducedactivation of H⁺-ATPase is established, the modulatory site(s) inhibited by PAOis no more accessible or becomes lessrelevant.

One simple interpretation of these results is that PAO affects the phosphorylation state of relevant Tyr residues locatedon the sequences of the PM H⁺-ATPase, of the 14-3-3 proteins, or both. The availability ofa recombinant, nonphosphorylated GF 14-6 14-3-3 isoform allowedus to show that in PM from Arabidopsis cells pretreated with PAO,the H⁺-ATPase maintains the capability to respond to FC when suppliedin vitro with 14-3-3 (Fig. 7). This result suggests that the phosphorylationstate of Tyr residues located on the PM H⁺-ATPase may not be involved in the association of 14-3-3 withthe enzyme, and that the dephosphorylation of 14-3-3-located specificTyr residues would be required to permit the FC-induced activationof the PM H⁺-ATPase. Searching Tyr-kinase phosphorylation site motifs on the14-3-3 protein sequence in several isoforms of different plantmaterials using the consensus pattern [RK]-X(2,3)-[DE]-X(2,3)-Y(Hunter, 1982; Patschinsky et al., 1982; Cooper et al., 1984),we found a highly conserved putative Tyr kinase phosphorylationsite KMKGDYYRY, which was also completely conserved in the 14-3-3GF14-6 isoform from maize (Fullone et al., 1998). It is temptingto speculate that de-phosphorylation of this site may be requiredto allow the FC-induced association between 14-3-3 proteins andthe PM H⁺-ATPase C terminus. However, we cannot rule out the possibilitythat PAO modifies a third partner protein, which, directly orindirectly, modifies 14-3-3 proteins. Work is in progress to discriminatebetween thesepossibilities.

Phosphorylation of Tyr residues is an ubiquitous, highly conserved modulatory mechanism involved in mitogen-activated proteinkinase (MAPK) cascade among eukaryotes (Anderson et al., 1990;Posada et al., 1991). In animal and yeast systems, PTPs play importantroles in a number of signal tranduction pathways involving themodulation of MAPKs (Neel and Tonks, 1997). In higher plants,recent results have shown that Tyr phosphorylation is criticalfor the activation of MAPKs involved in a variety of signal transductionpathways (Suzuki and Shinshi, 1995; Hirt, 1997; Zhang and Klessing,1997). In barley, PAO prevents the activation of a MAPK in responseto abscisic acid (Knetsch et al., 1996), indicating that a PTPis involved in the MAPK pathway in plants. Recently, an ArabidopsiscDNA clone has been isolated that encodes a PTP (AtPTP1) thatmay function in stress responses (Xu et al., 1998). Molecularcharacterization of PTPs in Arabidopsis, pea, and soybean hasbeen recently published (Fordham-Skelton et al., 1999), suggestingthat their role may not be as MAPK phosphatases and indicatingthat the function of these PTPs in higher plants is still unclear.The PAO-inhibited PTPs involved in FC-induced activation of PMH⁺-ATPase could be the final step of a signal transduction pathwaythat modulates the association between 14-3-3 proteins and theH⁺-ATPase, by affecting the phosphorylation state of Tyr residuesof the enzyme or, more likely, of 14-3-3proteins.

Modulation of PM H⁺-ATPase by modification of its phosphorylation state has been reported to occur both in vivo and in vitro;however, to date, only Ser and Thr residues have been involved(Sussman, 1994; Xing et al., 1996; Lino et al., 1998; Olsson etal., 1998). In particular, different phosphorylation sites identifiedin the H⁺-ATPase sequence have been shown to be involved in the interactionwith the 14-3-3 proteins. The activation of the PM H⁺-ATPase by FC is determined by the FC-induced association betweenthe C-terminal domain of the enzyme and member(s) of the 14-3-3protein family (Oecking et al., 1997; Baunsgaard et al., 1998;Fullone et al., 1998; Piotrowsky et al., 1998; Oecking and Hagemann,1999). The C-terminal domain of the PM H⁺-ATPase does not contain any sequence similar to the known 14-3-3-bindingmotifs RSX_1,2pSXP (Muslin et al., 1996; Yaffe et al., 1997), inwhich the phosphorylation of the Ser residue is crucial for thebinding of 14-3-3 to target proteins. Recent data suggest thatin spinach the phosphorylation of Thr-948 localized at the C terminuscould modulate the FC-induced association between 14-3-3 proteinsand the C-terminal domain of PM H⁺-ATPase (Olsson et al., 1998). However, 14-3-3 proteins also bindto the H⁺-ATPase independently of FC (Fullone et al., 1998), and this FC-independentbinding is phosphorylation dependent and occurs in a truncatedH⁺-ATPase lacking the C-terminal domain (Jahn et al., 1998). Recently,Marra et al. (2000) identified a sequence of the PM H⁺-ATPase highly conserved in different isoforms of different plantsand localized in the cytosolic stretch connecting transmembranesegments 8 and 9, which mimics the known 14-3-3 binding motif(Muslin et al., 1996; Yaffe et al., 1997). A phosphopeptide correspondingto such a sequence bound a 14-3-3 protein and inhibited FC bindingand FC-induced activation of the PM H⁺-ATPase; all of these effects were dependent on the phosphorylationof a Serresidue.

The physiological roles of such a complex modulation of the PM H⁺-ATPase involving phosphorylation mechanisms requires the dissectionof the single steps of the putative cascade and the identificationand characterization of the enzyme activitiesimplicated.

	ACKNOWLEDGMENTS

The authors are grateful to Patrizia Aducci (Dipartimento di Biologia, Università di Roma Tor Vergata, Rome) and Mauro Marra(Università degli Studi del Sannio, Benevento, Italy) for thegenerous gift of antisera anti-FC and anti-14-3-3 and of recombinantGF 14-6.

	FOOTNOTES

Received July 19, 1999; accepted October 28, 1999.

¹ This work was supported by Ministero per le Risorse Agricole, Alimentari e Forestali in the frame of the "Piano Nazionaleper le BiotecnologieVegetali."

^* Corresponding author; e-mail claudio.olivari{at}unimi.it; fax 39-02-26604399.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Phenylarsine Oxide Inhibits the Fusicoccin-Induced Activation of Plasma Membrane H+-ATPase1

Phenylarsine Oxide Inhibits the Fusicoccin-Induced Activation of Plasma Membrane H⁺-ATPase¹