Metabolizable and Non-Metabolizable Sugars Activate Different Signal Transduction Pathways in Tomato

doi:10.1104/pp.010771

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Metabolizable and Non-Metabolizable Sugars Activate Different Signal Transduction Pathways in Tomato¹

Alok K. Sinha, Markus G. Hofmann, Ulrike Römer, Walter Köckenberger, Lothar Elling, and Thomas Roitsch^*

Lehrstuhl für Pharmazeutische Biologie, Julius-von-Sachs Institute, Julis-von-Sachs-Platz 2, Universität Würzburg, D-97082 Würzburg, Germany (A.K.S., M.G.H., T.R.); Heinrich-Heine-University Düsseldorf, Research Center Jülich, D-52426 Jülich, Germany (U.R., L.E.); and Magnetic Resonance Centre, School of Physics and Astronomy, University of Nottingham, Nottingham NG7 2RD, United Kingdom (W.K.)

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

To gain insight into the regulatory mechanisms of sugar signaling in plants, the effect of derivatives of the transport sugarsucrose (Suc), the Suc isomers palatinose and turanose, and theSuc analog fluoro-Suc were tested. Photo-autotrophic suspensionculture cells of tomato (Lycopersicon peruvianum) were used tostudy their effect on the regulation of marker genes of sourceand sink metabolism, photosynthesis, and the activation of mitogen-activatedprotein kinases (MAPKs). Suc and glucose (Glc) resulted in reverseregulation of source and sink metabolism. Whereas the mRNA levelof extracellular invertase (Lin6) was induced, the transcriptlevel of small subunit of ribulose bisphosphate carboxylase (RbcS)was repressed. In contrast, turanose, palatinose, and fluoro-Suconly rapidly induced Lin6 mRNA level, whereas the transcript levelof RbcS was not affected. The differential effect of the metabolizableand non-metabolizable sugars on RbcS mRNA regulation was reflectedby the fact that only Suc and Glc inhibited photosynthesis andchlorophyll fluorescence. The activation of different signal transductionpathways by sugars was further supported by the analysis of theactivation of MAPKs. MAPK activity was found to be strongly activatedby turanose, palatinose, and fluoro-Suc, but not by Suc and Glc.To analyze the role of sugars in relation to pathogen perception,an elicitor preparation of Fusarium oxysporum lycopersici wasused. The strong activation of MAPKs and the fast and transientinduction of Lin6 expresssion by the fungal elicitor resemblesthe effect of turanose, palatinose, and fluoro-Suc and indicatesthat non-metabolizable sugars are sensed as stress-relatedstimuli.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

In recent years, sugars have been recognized as important signal molecules that affect a variety of physiological responsesand in particular regulate genes involved in photosynthesis, sinkmetabolism, and defense response (Koch, 1996; Smeekens, 1998;Roitsch, 1999; Sheen et al., 1999). Whereas the effect of sugarson gene regulation is well established, the nature of the sugarsignal, and the molecular mechanisms involved in sugar perceptionand intracellular signal transmission, are largely unknown. Sucis the major form of translocated carbon in higher plants andwas shown to regulate a number of carbohydrate-responsive genes.Whereas in many cases the effects of Suc could be mimicked byhexoses, such as Glc and Fru, a few studies demonstrated the existenceof Suc-specific regulatory pathways (Chiou and Bush, 1998; Rooket al., 1998). In principle, a sugar signal could be generatedby extracellular recognition via a soluble or membrane-bound receptormolecule or by intracellular sensing at different stages of sugarmetabolism. For hexoses, a dual role of hexokinase in sugar sensingand glycolysis has been proposed (Jang and Sheen, 1997; Jang etal., 1997) that is a matter of a controversial debate (Halfordet al., 1999). Additional membrane-based sensing systems havebeen implied both for hexoses and Suc. Primary lines of evidenceare the finding that non-phosphorylatable Glc analogs can mimicthe effect of Glc on the regulation of specific genes (Godt etal., 1995; Roitsch et al., 1995) and transgenic studies with specificsubcellular targeting of a yeast (Saccharomyces cerevisiae) invertase(Herbers et al., 1996). Hexose transporters were shown to functionas membrane sugar sensors in yeast (Özcan et al., 1998) and adual function of plant sugar carriers in transport and sensingof sugars has been proposed (Lalonde et al., 1999). Additionalsensing mechanisms involving metabolism of sugars such as glycolysishave also been suggested (Koch et al., 2000). In summary, resultsobtained with various experimental approaches and systems indicatethe existence of different sensory mechanism and parallel sugarsignaling pathways in higher plants (Jang et al., 1997; Smeekensand Rook, 1997; Lalonde et al., 1999).

To gain insight into disaccharide-specific signal transduction pathways, derivates of the transport sugar Suc were used inthe present study. Turanose (3-O- $alpha$ -d-glucopyranosyl-Fru) and palatinose(6-O- $alpha$ -d-glucopyranosyl-Fru) are structural isomers of Suc composedof Glc and Fru with a different glycosidic linkage. They are notsynthesized in higher plants and cannot be cleaved or transportedby plant enzymes. Using these non-metabolizable Suc isomers, evidencefor extracellular sugar sensing has been obtained in barley (Hordeumvulgare) and potato (Solanum tuberosum) tubers (Loreti et al.,2000; Fernie et al., 2001).

A Suc analog that is not cleaved by invertase is 1'deoxy-1'fluro-Suc (1-deoxy-1-fluorofructofurano-syl $alpha$ -D-glucopyranosid,fluoro-Suc). Because this sugar analog is not commercially available,it was synthesized by an optimized protocol. Here, we report ahighly effective synthesis of fluoro-Suc with a recombinant Sucsynthase 1 from potato to address the possible signaling functionof this Sucanalog.

Acitvation of mitogen-activated protein kinases (MAPKs) was shown to be involved in the stress-induced signal transductionpathways (Zhang and Klessig, 1998; Zhang et al., 1998). Thus,we also studied the activation of MAPK by different Suc analogs.Pathogen infection is known to affect source/sink relations anddifferent lines of experimental evidence suggest a role of sugarsin plant defense responses (Herbers et al., 1996; Ehness et al.,1997).

Photo-autotrophic cultures proved to be useful to study various aspects of sugar regulation (Krapp and Stitt, 1994; Roitschet al., 1995; Godt and Roitsch, 1997). Sugar responses may beanalyzed without the necessity of a sugar depletion period requiredfor heterotrophic cultures and signal transduction events maybe related to photosynthetic gene expression or photosyntheticactivity as well as source/sink regulations. Using photo-autotrophicsuspension culture cells of Chenopodium rubrum, it has been shownthat source/sink relations and defense mechanisms are coordinatelyregulated both by sugars and stress-related stimuli (Ehness etal., 1997).

A photo-autotrophic culture of the model plant species tomato (Lycopersicon peruvianum; Beimen et al., 1992) was used in thepresent study to test the effect of Suc, Glc, and the non-metabolizableSuc derivatives turanose, palatinose, and fluoro-Suc on differentcellular responses. The results were compared with the effectof an elicitor preparation of the tomato pathogen Fusarium oxysporumlycopersici. Extracellular invertase is the key enzyme for phloemunloading via an apoplastic pathway and was used as a representativemarker gene for sink metabolism (Sturm, 1999; Roitsch et al.,2000). The analysis of the regulation of the mRNA for the smallsubunit of the Calvin cycle enzyme ribulose bisphosphate carboxylase(RbcS) was complemented by the measurement of the rate of photosyntheticoxygen evolution and chlorophyll fluorescence. The present studydemonstrates that metabolizable and non-metabolizable sugars activatedifferent signal transduction pathways. They were shown to differentiallyaffect photosynthesis as well as MAPK activation. In contrastto Suc and Glc, the Suc derivatives had no effect on RbcS expressionand photosynthesis but resulted in strong MAPK activation. Thefact that the non-metabolizable sugars, like the fungal elicitor,activate MAPKs and results in a fast induction of Lin6 expressionindicates that they are sensed as stress-related stimuli ratherthan extracellular carbohydratesignals.

	RESULTS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Inverse Regulation of mRNAs for Extracellular Invertases Lin6 and RbcS by Suc and Glc

The time course of the regulation of mRNAs for the sink-specific extracellular invertase Lin6 and the photosynthetic markergene RbcS by metabolizable sugars was analyzed by the additionof 50 mM Glc or Suc to autotrophically growing tomato cell cultures.Samples were taken before the addition of the sugars, and after1, 4, 9, 24, and 48 h, mRNA levels were determined by RNA gel-blotanalysis.

The low level of mRNA for extracellular invertase Lin6 was already elevated after 1 h in response to both Glc and Suc, furtherincreased up to 24 h, and then declined (Fig. 1A). In contrast,the mRNA level of the photosynthetic protein was inversely regulated.The high steady state of RbcS mRNA was repressed already after4 h by both sugars and further declined up to 48 h. Addition of50 mM mannitol to the cultures as an osmotic control did not resultedeither in the induction of LIN6 or repression of RbcS transcriptlevel (data not shown).

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Figure 1. Differential effect of metabolizable sugars, Suc isomers, and an elicitor preparation of F. oxysporum lycopersici (E-FOL) on mRNA regulation and photosynthetic parameters. A, Regulation of mRNAs for extracellular invertase Lin6 and RbcS. Thirty micrograms of total RNA was separated on formaldehyde agarose gels, blotted onto nitrocellulose, and probed with random primer labeled cDNA fragments. Equal loading of RNA was confirmed by ethidium bromide staining of the rRNA (data not shown). The data presented are representative of five independent sets of experiments. B, Regulation of the rate of oxygen evolution (

) and effective photochemical yield Y ( $open circle$ ). The data represent the mean values of five independent experiments.

Differential Uptake of Hexoses, Suc, and the Suc Isomers Turanose and Palatinose by Tomato Suspension Culture Cells

It has been shown previously that the Suc isomers turanose and palatinose are neither recognized nor transported by Suc transportersof soybean (Glycine max) cotyledons and broad bean (Vicia faba)leaves (M'Batchi and Delrot, 1988; Li et al., 1994). To rule outa possible uptake of these two Suc derivatives by the tomato suspensioncultures used for the experiments, 50 mM of these sugars was addedto the suspension culture cells and the concentration of the twoSuc isomers in the culture supernatant were determined duringa 48-h incubation period. Figure 2A demonstrates that the extracellularconcentration of palatinose and turanose did not change even aftera prolonged incubation time of 48 h compared with the initialconcentration determined. No Glc could be detected during thecourse of the experiment. These results demonstrate that the twoSuc isomers are neither cleaved nor taken up by the tomato suspensionculture cells. In comparison, control incubations with 50 mM Glcor Suc demonstrate a fast decrease of the concentrations of thesesugars in the culture supernatant. Figure 2A shows that the Glcconcentration starts to decrease after 1 h and further declinesto 11 mM after 48 h. The concentration of Suc gradually declinesto 0.3 mM at 48 h (Fig. 2B). Determination of the Suc cleavageproducts revealed a differential accumulation of Glc and Fru.Glc can be detected only after 24 h and the peak concentrationof 12.7 mM at 24 h decreases to 9.4 mM at 48 h. In contrast, Frustarts to accumulate after 1 h, which further increases up to29 mM at 48 h.

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Figure 2. Time course of changes in external sugar concentrations. Suspension cultures cells were treated with 50 mM of the indicated sugars and the remaining concentration in the culture supernatant was determined at the given time points. A, Suspension cultures were treated with Glc ( $open circle$ ), palatinose ( $black-triangle$ ), or turanose ( $triangle$ ). B, Suspension cultures were treated with Suc and the concentration of Suc (

), Glc ( $open circle$ ), and Fru (

) in the same supernatant were determined. The data represent the mean values of six independent measurements.

Suc Isomers Differentially Affect the mRNAs for Extracellular Invertases Lin6 and RbcS

The time course of the regulation of mRNAs for the sink-specific extracellular invertase Lin6 and the photosynthetic markergene RbcS by metabolizable sugars was analyzed by the additionof 50 mM turanose and palatinose to autotrophically growing tomatocell cultures. Samples were taken before the addition of the sugarsand after 1, 4, 9, 24, and 48 h, and mRNA levels were determinedby RNA gel-blotanalysis.

A fast and strong induction of the Lin6 gene could be observed in response to both Suc isomers. The low level of mRNA forLin6 was highly induced already after 1 h and the elevated leveldeclined after 24 h (Fig. 1A). In contrast, neither turanose norpalatinose had an effect on the high RbcS mRNA level throughoutthe 48-h experiment. Thus addition of the two non-metabolizableSuc isomers turanose and palatinose results in a differentialeffect on the source- and sink-specific marker enzymestested.

The Differential Effect of Glc, Suc, and Suc Isomers on RbcS mRNA Is Reflected by the Rate of Photosynthetic Oxygen Evolution and Chlorophyll Fluorescence

In further experiments, it has been addressed whether the differential effect of the metabolizable and non-metabolizable sugarson the mRNA level of the photosynthetic gene RbcS is reflectedby physiologicalparameters.

The rates of oxygen evolution were measured with the help of a liquid phase oxygen electrode. Glc treatment results in animmediate decrease of the rate of oxygen evolution, which furtherdeclines up to 48 h (Fig. 1B). Suc treatment also resulted ina pronounced reduction of the rate of oxygen evolution althoughwith a different time course. An initial lag phase of 4 h wasfollowed by a constant decline to result in a final reductionto values comparable with the Glc-treated cultures. In contrast,the non-metabolizable Suc analogs palatinose and turanose didnot reduce the rate of oxygen evolution throughout theexperiment.

To analyze whether the photosynthetic apparatus is also differentially affected by the metabolizable sugars and the Suc analogs,chlorophyll fluorescence measurements were carried out with aPAM 2000 portable fluorometer as described in "Materials and Methods."The F_v/F_m values, reflecting the maximal photochemical quantumefficiency of PSII reaction centers of dark-adapted samples, remainedunchanged by all the treatments (data not shown). Photochemicalyield Y, an indicator of effective photochemical quantum efficiencyof illuminated sample, was differentially affected by the metabolizableand non-metabolizable sugars. Glc and Suc resulted in a constantdecline of the photochemical yield Y with comparable low valuesafter 48 h (Fig. 1B). In contrast, the photochemical yield remainedunchanged in turanose- and palatinose-treatedcultures.

Fast, Transient, and Inverse Regulation of mRNAs for Extracellular Invertase Lin6 and RbcS by an Elicitor Preparation of F. oxysporum lycopersici

Using photo-autotrophic cultures of C. rubrum, it has been shown that during a short incubation time of 6 h, the mRNA foran extracellular invertase and RbcS are coordinately regulatedboth by Glc and the fungal elicitor chitosan (Ehness et al., 1997).These findings were reevaluated and extended in the present studyby comparing the effect of sugars with a fungal elicitor on theautotrophic tomato suspension culture over a 48-h period. F. oxysporumlycopersici is a wilt-inducing pathogenic fungus specific fortomato (Armstrong and Armstrong, 1981). An elicitor preparationof this fungus (E-FOL), shown to elicit secondary metabolite productionin the photo-autotrophic tomato suspension culture line used forthe experiments (Beimen et al., 1992), was used to address theregulation of Lin6 and RbcS in response to this stress-relatedstimulus.

Treatment of the tomato suspension culture with 150 µg mL¹ E-FOL resulted in fast and transient effects on the levels of mRNAsfor Lin6 and RbcS (Fig. 1A). After 1 and 4 h, the Lin6 mRNA washighly induced, then declined to a low level again. The transienteffect on RbcS mRNA showed a similar time course. The high levelof mRNA for RbcS was most strongly repressed at 4 h and then increasedagain to the normallevel.

E-FOL treatment resulted in a fast and pronounced decrease of the rate of oxygen evolution after 1 h that recovered after24 h, although values were still reduced compared with the controlcultures (Fig. 1B). In contrast to the oxygen production, photochemicalyield Y was not affected in the cultures treated with E-FOL (Fig.1B).

MAPK Activity Is Induced Only by Non-Metabolizabable Sugars and an Elicitor Preparation of F. oxysporum lycopersici, But Not by Metabolizable Sugars

MAPKs play a key role in signal transduction cascades of animals and yeast. They are rapidly and transiently activated andcharacterized by phosphorylating the model substrate myelin basicprotein (MBP) in an in-gel assay. There is also accumulating evidencefor the importance of MAPKs in the transduction of various, inparticular stress-related, stimuli in higher plants. Therefore,we have compared the effect of Suc, Glc, and the Suc derivativeswith the effect of the fungal elicitor E-FOL on MAPKactivation.

Tomato suspension culture cells were treated with the different stimuli for 5 min and crude extracts were analyzed for MAPKactivity by in-gel kinase assays with the model substrate MBP.The dose response shown in Figure 3 demonstrates that concentrationsof up to 100 mM of either Glc or Suc had no effect on MAPK. Onlya concentration of 200 mM of the two metabolizable sugars resultedin a weak MAPK activity. Control incubations demonstrate thatmannitol also resulted in weak MAPK activation at a concentrationof 200 mM. This finding indicates that the weak MAPK activationby 200 mM Glc and Suc represents an osmotic effect rather thana specific effect of the two sugars applied. In contrast to thetwo metabolizable sugars, both palatinose and turanose resultedin strong MAPK activation. The dose response shown in Figure 3demonstrates that concentrations of 25 mM of both Suc isomerswere sufficient to result in MAPK activation that further increasesat concentration of up to 100 mM (Fig. 3A). The elicitor preparationE-FOL also strongly activated MAPK, even at the lowest concentrationof 0.1 µg mL¹ tested (Fig. 3B). The observed differential effect of metabolizableand non-metabolizable sugars on MAPK activation further supportsthe activation of different signal transduction pathways.

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Figure 3. Differential effect of metabolizable sugars, Suc isomers, and an elicitor preparation of F. oxysporum lycopersici (E-FOL) on activation of MAPK. Cells were harvested exactly after 5 min after the addition of stimuli. A, Study of activation of MAPK by different sugars. Mannitol was taken as osmotic control for the different concentrations of sugars used. B, Activation of MAPK by different amount of E-FOL. The data presented in A and B are representative of five independent sets of experiments.

Synthesis of the Suc Analog Fluoro-Suc

In further experiments, the question has been addressed whether the differential effects of the Suc isomers and Suc and Glcare related to the fact that turanose and palatinose are not transported.Fluoro-Suc was used as a Suc analog that is not subject to invertasehydrolysis, only slowly metabolized (Hitz et al., 1985) but efficientlytransported into plant cells (Thom and Maretzki, 1992). We foundthat 80% to 85% of fluro-Suc was taken up by the cell culturewithin 6 h ofincubation.

Because fluoro-Suc is not commercially available, it was synthesized by an optimized procedure. Card and Hitz (1984) previouslysynthesized fluoro-Suc by using a Suc synthase from barley seedswith an overall yield of 59% (507 mg). In the present paper, wecould improve the synthesis with reference to the enzyme productivityby repetitive use of recombinant Suc synthase and alkaline phosphatase(Fig. 4). The synthesis yield after three batches was 100% withreference to the acceptor substrate. After purification, an overallyield of 85% (860.5 mg) for fluoro-Suc was obtained. The analysisby NMR confirmed the structural integrity of the product as describedpreviously (Card and Hitz, 1984).

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Figure 4. Enzymatic synthesis of 1'-deoxy-1'-fluoro-Suc with a recombinant Suc synthase (SuSy) from potato and alkaline phosphatase (AP).

The Suc Analog Fluoro-Suc Differentially Affects the Regulation of mRNAs for Extracellular Invertases Lin6 and RbcS and Activates MAPKs

Because of the limited amount of fluoro-Suc available, the regulation of the mRNAs for the marker enzymes Lin6 and RbcS wasanalyzed only at one time point, 6 h after the addition of theSuc analog. Figure 5A shows that 20 mM fluoro-Suc strongly inducesLin6 mRNA, whereas the level of the RbcS mRNA was not affected.Thus, fluoro-Suc, like the Suc isomers, specifically affects onlythe expression of the sink-specfic extracellular invertase incontrast to the metabolizable sugars that also repress RbcS mRNAlevel.

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Figure 5. A, Regulation of mRNAs of extracellular invertase Lin6 and RbcS by fluoro-Suc and Suc. Suspension culture cells were treated with 20 mM fluoro-Suc and 50 mM Suc for 6 h. Thirty micrograms of total RNA was separated on formaldehyde agarose gels, blotted onto nitrocellulose, and probed with random primer-labeled cDNA fragments of extracellular invertase Lin6 or RbcS. Equal loading of RNA was confirmed by ethidium bromide staining of the rRNA (data not shown). B, Activation of MAPK by fluoro-Suc and Suc. The cell cultures were incubated with 20 mM fluoro-Suc and 50 mM Suc and harvested exactly after 5 min for the MAPK assay. The data presented in A and B are representative of three independent sets of experiments.

To further substantiate the similar effect of fluoro-Suc and the Suc isomers, MAPK activation was tested. The in-gel assayshown in Figure 5B demonstrates that addition of 20 mM fluoro-Sucfor 5 min also results in strong MAPK activation, whereas Sucwas inactive. Thus, the ability of fluoro-Suc to activate MAPKactivity also resembles the effect of turanose and palationseshownabove.

Control experiments were carried out to rule out intracellular cleavage of fluoro-Suc by Suc synthase. Crude extracts of fluoro-Suc-treatedcells were analyzed by ¹⁹F-NMR. The ¹⁹F-NMR spectra revealed that fluoro-Suc was taken up by the tomatosuspension culture cells, but that this Suc analog has not undergoneany change in structure under the experimental conditions used(data notshown).

	DISCUSSION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Although sugar-mediated signal transduction pathways have been recognized to be important to regulate a variety of physiologicalresponses, the analysis in particular of the effect of the transportsugar Suc is complicated by the fact that it is readily cleavedby extracellular invertase. To circumvent this problem, the non-metabolizableSuc derivatives turanose and palatinose have been used to addressdisaccharide-specific signaling (Loreti et al., 2000; Fernie etal., 2001). The present study demonstrates that metabolizablesugars and non-metabolizable Suc derivatives activate distinctlydifferent signal transduction pathways in photo-autotrophic tomatosuspension culture cells. The data indicate that different disaccharide-specificpathways exist and that non-metabolizable Suc derivatives aresensed as stress-relatedstimuli.

Photo-autotrophic suspension culture cells of the model plant species tomato and Suc derivatives were used to get furtherinsight in the mechanisms that mediate sugar recognition and signaltransduction. Turanose and palatinose are isomers of Suc thatdiffer in their glycosydic linkage between Glc and Fru. Thesetwo Suc isomers were shown to be neither cleaved nor taken upby the tomato suspension culture cells used. These data supportprevious findings that turanose and palatinose are not recognizedor transported by Suc transporter (M'Batchi et al., 1984; M'Batchiand Delrot, 1988; Li et al., 1994). Fernie et al. (2001) alsorecently showed very poor absorption of palatinose by slices ofpotato tubers. The analysis was further complemented by the useof fluoro-Suc, a Suc derivative that is not subject to invertasehydrolysis but efficiently transported into plant cells (Thomand Maretzki, 1992). It was synthesized by optimizing the protocolof Kragl et al. (1993) using a recombinant Suc synthase. The resultsobtained with metabolizable sugars (Glc and Suc) and non-metabolizablesugars (turanose, palatinose, and fluro-Suc) were compared withthe effect of an elicitor preparation of the tomato pathogenicfungus F. oxysporum lycopersici (E-FOL) as a specific and physiologicalstress-relatedstimulus.

Metabolizable Sugars and Non-Metabolizable Suc Derivatives Result in Differential Gene Regulation

In the present study, the regulation of mRNAs for extracellular invertase Lin6 and RbcS, chosen as representative marker enzymesfor sink and source metabolism, have been analyzed over a 48-hincubation time. The metabolizable sugars Glc and Suc induce theexpression of Lin6, whereas RbcS was repressed. This finding confirmsresults obtained with various experimental systems involving bothmonocotyledonous and dicotyledonous species showing that metabolizablesugars in general seem to repress photosynthetic genes, whereassink-specific enzymes are induced (Ehness et al., 1997; Roitsch,1999; Sheen et al., 1999; Pego et al., 2000). Whereas turanoseand palatinose resulted in a strong, fast, and transient inductionof extracellular invertase Lin6, the level of RbcS mRNA was notaffected. Likewise, the Suc analog fluro-Suc, tested only withan incubation time of 6 h because of the limited amount available,also showed a fast induction of Lin6 transcript level, whereasRbcS transcript level was not affected. Palatinose was also shownto stimulate Suc degradation in discs of growing potato tubers(Fernie et al., 2001). The differential effect of the metabolizablesugars and the non-metabolizable Suc isomers on RbcS expressionindicate that they activate distinctly different signal transductionpathways. The fungal elicitor E-FOL resulted in fast and transientrepression of RbcS and induction of Lin6 mRNA. Induction of Lin6pathway seems to be activated by all the stimuli tested, althoughat different time courses. The Suc derivatives and stress stimuliresulted in faster activation than the metabolizable sugars. Inaddition, the effect of the Suc isomers was transient like theelicitor, although it was not consumed likeSuc.

The differential effect of the metabolizable sugars and the Suc isomers on RbcS expression is substantiated by the analysisof two physiological photosynthetic parameters. The correlationbetween the regulation of RbcS mRNA, the rate of oxygen evolution,and the photochemical yield Y supports the use of RbcS mRNA asan appropriate marker for photosynthesis. The regulation of RbcSmRNA by E-FOL is also reflected by a transient decrease of therate of oxygen evolution, whereas photochemical yield Y is notaffected.

Metabolizable Sugars and Non-Metabolizable Suc Derivatives Results in Differential MAPK Activation

The differential effects of sugar analogs and metabolizable sugars were further substantiated by the study of activation ofMAPK, which is an important enzyme in a number of signal transductioncascades. MAPKs have been reported to be activated by severalstresses in plants such as elicitors (Zhang et al., 1998), wounding(Stratmann and Ryan, 1997), cold and drought stress (Jonak etal., 1996), salinity (Munnik et al., 1999), and endogenous signals(Zhang and Klessig, 1997). In the present studies from the suspensioncell cultures of tomato, MAPK was found to activated not onlyby the fungal elicitor E-FOL, but also by the sugar analogs, turanose,palatinose, and fluoro-Suc. In contrast, Suc and Glc did not resultin MAPK activation at the corresponding concentrations. Theseresults suggest that the perception of non-metabolizable Suc analogsand metabolizable sugars and transduction of the correspondingsignals follow differentpathways.

Implications for the Analysis of Sugar Signal Transduction Pathways

The finding that the metabolizable sugars and the different non-metabolizable Suc derivatives tested, turanose, palationose,and fluoro-Suc, activate distinctly different signal transductionpathways further supports the complexity and importance of carbohydrate-mediatedsignal transduction in higherplants.

The differential effect of the non-metabolizable Suc isomers and Suc on a very fast signal transduction event, the activationof MAPK, indicates the existence of distinctly different disaccharidespecific pathways. Within the very short incubation time of 5min, cleavage of Suc by extracellular invertase can be neglected.Thus, the observed difference between Suc and the non-metabolizableSuc may not be because of conversion of Suc into the hexose monomers.Using the Suc isomers turanose and palatinose, Loreti et al. (2000)also have demonstrated that both Glc and disaccharide-sensingmechanisms modulate the expression of $alpha$ -amylase mRNA in barleyembryos. Because effects on gene regulation have been analyzed,incubation times of at least several hours were required. Theresulting Suc/Glc interconversion ruled out the comparison betweenthe effect of Suc and the Sucisomers.

The finding that neither turanose nor palatinose is transported supports an extracellular recognition of these carbohydratesignals, which has been suggested before (Loreti et al., 2000;Fernie et al., 2001). Because the transportable fluoro-Suc elicitedthe same responses as turanose and palatinose, the correspondingeffects are independent of the lack of a transport system. Bothwith respect to the time course of Lin6 mRNA induction and MAPK,the effect of the non-metabolizable Suc derivatives resemble theeffect of the fungal elicitor E-FOL. These observations indicatethat these Suc derivatives that are not naturally occurring inplants are sensed as stress signals rather than metabolic signals.The physiological significance of this assumption is supportedby the fact that phytopathogens such as specific strains of Erwiniaspp. are able to transform Suc into palatinose (Huang et al.,1998). By this mechanism, Suc is retrieved from the plants andconverted to a form unavailable for the plant metabolism. Thus,the presence of unusual Suc derivatives may be signals for thepresence of a pathogen. Therefore, these sugar analogs may notbe appropriate tools to address extracelluar and disaccharide-specificsensing mechanism in plants perse.

Non-metabolizable Suc derivatives were shown to activate different signal transduction pathways than metabolizable sugars,thus demonstrating the complexity of carbohydrate-mediated regulatorymechanisms. Distinct sugar-sensing mechanisms and parallel signaltransduction pathways may be a central part of a complex regulatorynetwork of higher plants to integrate metabolism with developmentand defenseresponses.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Growth of Suspension Culture Cells

Photo-autotrophic suspension cell culture cells of tomato (Lycopersicon peruvianum) were established by Beimen et al. (1992)These cell cultures are being subcultured every 2 weeks in Murashigeand Skoog medium and are incubated shaking under continuous lightconditions with an atmosphere containing 2% (w/v) CO₂.

Preparation of an Elicitor from Fusarium oxysporum lycopersici

The pathogenic fungus F. oxysporum lycopersici Schlecht. Fr. f. sp. lycopersici (Sacc.) was obtained from the Centraalbureauvoor Schimmelcultures (Baarn, The Netherlands). The fungus wascultured in a medium containing 50 g L¹Glc, 8 g L¹casamino acids, 0.5 g L¹yeast (Saccharomyces cerevisiae) extract, 0.2 g L¹MgSO₄and FeSO₄ each, 20 mg L¹CaCl₂, and 1.5 mg L¹MnSO₄ and Na₂MoO₄ each in 25 mM potassium phosphate at pH 7.5.After 4 d of shaking at 28°C, the culture was autoclaved, dialyzedagainst water, and lyophilized. For the induction of stress response,150 mg L¹of the dried hyphae was added to a tomato cell suspensionculture.

Extraction of mRNA and RNA Gel-Blot Analysis

For the isolation of RNA, cells were harvested by centrifugation, snap frozen in liquid nitrogen, and ground in the presenceof liquid nitrogen. Total RNA was isolated according to the methodsof Chomczynski and Sacchi (1987). Northern-blot analysis was carriedout as described previously (Godt and Roitsch, 1997).

Determination of Sugars

The concentrations of Glc were determined by a commercially available test system (GOD test, Roche, Mannheim, Germany). Forthe determination of Suc concentrations, the Suc present in thesamples were hydrolyzed by 100 units of yeast invertase (GradeVII, Sigma, St. Louis) incubated at 30°C for 1 h. Glc concentrationwas determined before and after hydrolysis by invertase and thedifference between these values was taken as the actual amountof Suc in the sample. The supernatant of Suc treated cells wereused to estimate the build up of hexoses, Glc, and Fru. Glc wasestimated by the GOD test, whereas Fru was estimated as describedby Bernt and Bergmeyer (1970). Turanose and palatinose concentrationswere determined according to Dubois et al. (1956).

In-Gel Kinase Assay for MAPK

The enzyme was extracted from the ground tissue in an extraction buffer consisting of 100 mM HEPES, pH 7.5; 5 mM EDTA; 5 mMEGTA; 10 mM dithiothreitol; 10 mM Na₃VO₄; 10 mM NaF; 50 mM glycerophosphate;0.1 mM phenylmethylsulphonyl fluoride; 1 mM bezamidine; and 0.1µg mL¹ antipain. The crude extract was centrifuged at 4°C at 20,000rpmfor 10 min and an aliquot of supernatant equivalent to 40 µg ofprotein analyzed by Bradford assay (Bradford, 1976) was used forin-gel kinase assay. Polyacralymide gel (10% [w/v]) embedded with0.3 mg mL¹ of MBP (Upstate Biotechnology, Lake Placid, NY) as substratewas used for the kinase assay. For control, MBP was substitutedwith histone or casein. After electrophoresis, proteins were renaturedand assayed for kinase assay as described by Zhang and Klessig(1997). Activity were visualized by autoradiography and phosphorimager (Cyclone Phosphor Storage Systems, Perkin Elmer, Madison,WI).

Measurement of Rate of Oxygen Evolution

Rate of oxygen evolution of the cell cultures were measured using a liquid phase oxygen electrode (Frank Bros Ltd., Cambridge,UK) in the presence of saturating light provided by a halogenlamp projector. The cells in the sample cuvette were first allowedto respire for 1 min in the dark and then exposed to light forthe measurement of oxygen evolution. Equal volumes of cells wereused each time and immediately after the measurements, the cellswere taken out to determine the fresh weight. The rate of oxygenevolution was calculated on the basis of fresh weight and representedas relativeunits.

Chlorophyll Fluorescence Measurements

Modulated chlorophyll fluorescences of the tomato cell suspension culture were measured using a PAM 2000 chlorophyll fluorometer(Heinz Walz, Effeltrich, Germany). Maximum PSII quantum yieldof a dark-adapted sample (F_v/F_m) and effective PSII quantum yieldof illuminated sample (Y; for nomenclature, see van Kooten andSnel, 1990) were measured on cells dark adapted for 15 min asdescribed by Schreiber et al. (1986). The preprogrammed protocol(Standard Run 3) was used for the determination of F_v/F_m and Yin a special cuvette designed for the purpose. The steady-statevalues obtained at the end of Run 3 were reported as the valuesofY.

Synthesis of 1-Deoxy-1-Fluoro-Fru

1-Deoxy-1-fluoro-D-Fru was obtained by the reaction described by Card and Hitz (1984). In brief, the readily available 2,3:4,5-di-o-isopropylidene-D-fructopyranosewas converted into the trifylate by the procedure described byBinkley et al. (1980). Trifylate was fluorinated by Tris (dimethylamino)sulfur(trimethylsilyl)difluoride (Sigma-Aldrich, Saint-Quentin-Fallavier,France) in refluxing tetrahydrofuran. After removal of the isopropylideneprotection groups, 1-deoxy-1-fluoro-D-Fru was obtained as a syrupin 75% yield. The synthesis of 1'-deoxy-1'-fluoro-Suc was carriedout by the repetitive batch technique (Kragl et al., 1993). Thereaction mixture (100 mL) containing 0.96 mmol 1-deoxy-1-fluoro-Fru(176 mg) and 1 mmol UDP- $alpha$ -D-Glc (Sigma, Deisenhofen, Germany)in 200 mM HEPES buffer, pH 8.0, was gently stirred at 30°C afterthe addition of 40 units of recombinant SuSy 1 from potato (Solanumtuberosum; Zervosen et al., 1998; Zervosen and Elling, 1999),and 200 units of alkaline phosphatase (Roche Diagnostics). Thecourse of reaction was controlled by HPLC analysis of the productwith an Aminex HPX-87C column (300 × 7, 8 mm, Bio-Rad, Munich)by elution with distilled water at 85°C. After 48 h, the enzymeswere recovered by ultrafiltration and used in a second and thirdbatch, respectively, by the addition of newsubstrates.

The yield of the combined product solutions was 2.9 mmol (100%) for 1'-deoxy-1'-fluoro-Suc. For isolation, the product solutionwas adjusted to pH 8.6 and loaded onto an anion exchanger column(HCOO form) filled with AG 1-X8 resin (100-200 mesh, 122-mL bed volume,Bio-Rad), which was equilibrated with distilled water. Elutionwith distilled water (linear flow rate: 56.5 cm h¹) gave a product pool, which was concentrated by in vacuoevaporationto a final volume of 5 mL. The disaccharide was further purifiedby chromatography on an AG 50W-X8 resin column (200-400 mesh,Ca²⁺ form, 1,532-mL bed volume, Bio-Rad). Elution with distilled water(linear flow rate: 3 cm h¹) gave the fractions containing the disaccharide, which were pooledand lyophilized. The dry product was dissolved in 10 mL of absolutemethanol and crystallized at 25°C. 1'-deoxy-1'-fluoro-Suc wasobtained in an overall yield of 85% corresponding to 2.5 mmol(860.5 mg) with an HPLC purity of 89%. NMR spectroscopy (11.7Tesla) of 1'-deoxy-1'-fluoro-Suc revealed the typical couplingsbetween ¹⁹F and ¹H or ¹³C: ¹H-NMR(D₂O): H_1' $delta$ ' 3a.39 ppm, m, J_1H-19F: 46.6 Hz, J_1H-1H:10.4 Hz; ¹⁹F-NMR(D₂O): $delta$ _CFCl3: $-$ 229.4 ppm, m, J_19F-1H: 46.6Hz.; ¹³C-NMR(D2O): C_1' $delta$ :80.7 ppm, d, J_13C-19F: 174.2Hz; C_2' $delta$ :101.8ppm, d, J_13C-19F: 19.6Hz.

	ACKNOWLEDGMENTS

W.K. is grateful for the support and advice of Drs. Claude Roby, Jacques Defaye, and André Gadelle (Commissariat à l'EnergieAtomique, Grenoble, France) during the synthesis of fluoro-Fru.T.R. and A.K.S. would like to thank Werner Kremer (Institut fürBiophysik und Physikalishe Biochemie, Regensburg, Germany) forthe NMR analysis of tomato samples, and Dr. Ulrch Schreiber (LehrstuhlsBotanik I, Würzburg, Germany) for providing the PAM 2000 portablefluorometer. Authors are grateful to Dr. Ludwig Lehle for thehelp with the sugar determinations, Vinzenz Link and Mark Goetzfor critically reading the manuscript, and Dr. Widmar Tanner forcontinuous interest and support (all from Lehrstuhl für Zellbiologieund Pflanzenphysiologie, Regensburg,Germany).

	FOOTNOTES

Received August 22, 2001; returned for revision October 20, 2001; accepted December 18, 2001.

¹ This work was supported by the Deutsche Forschungsgemeinschaft (grant no. SFB380, Teilprojekt B26 to L.E. and grant no. Ro4-1 to T.R.), by the Alexander von Humbold Foundation (to A.K.S.),and by the Studienstiftung des Deutschen Volkes (to M.G.H.).

^* Corresponding author; e-mail roitsch{at}biozentrum.uni-wuerzburg.de; fax 49-931-888-6182.

Article, publication date, and citation information can be found at www.plantphysiol.org/cgi/doi/10.1104/pp.010771.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
RESULTS
DISCUSSION
MATERIALS AND METHODS
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Metabolizable and Non-Metabolizable Sugars Activate Different Signal Transduction Pathways in Tomato1

Metabolizable and Non-Metabolizable Sugars Activate Different Signal Transduction Pathways in Tomato¹