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Plant Physiology 133:47-62 (2003) © 2003 American Society of Plant Biologists Differential Regulation of Glucose-6-Phosphate Dehydrogenase Isoenzyme Activities in Potato1
Pflanzenphysiologie, FB5 Biologie/Chemie, Universität Osnabrück, Barbarastra
In plants, Glc-6-phosphate dehydrogenase (G6PDH) isoenzymes are present in the cytosol and in plastids. The plastidic enzymes (P1 and P2) are subject to redox regulation, but mechanisms that adjust cytosolic G6PDH activity are largely unknown. We adopted a leaf disc system for monitoring the effects of various conditions on G6PD isoform expression and enzyme activities in potato (Solanum tuberosum). Cytosolic G6PDH activity remained constant during water incubation in the dark. In continuous light or in the presence of metabolizable sugars in the dark, cytosolic G6PDH activity increased 6-fold within 24 h. Cycloheximide incubation demonstrated that enhanced cytosolic G6PDH activity depends on de novo protein synthesis. Osmotic change, phosphate sequestration, or oxidative stress did not affect cytosolic G6PDH activity. Furthermore, enzyme activity and protein contents closely followed the corresponding mRNA levels. Together with the fact that multiple SURE elements are present in the promoter region of the gene, these results suggest that cytosolic G6PDH activity is regulated by sugar availability at the transcriptional level. Plastidic G6PDH activity stayed constant during water incubation in the light and dropped to minimal levels within 6 h in the dark. Conversely, plastidic G6PDH activity of leaf discs incubated on Paraquat rose to 10-fold higher levels, which was not prevented by cycloheximide. Similar increases were found with nitrite, nitrate, or sulfate. No major changes in protein or mRNA contents of the plastidic P1 and P2 isoforms were registered. Km (Glc-6-phosphate) values of plastidic G6PDH activity differed between samples incubated on water or Paraquat, suggesting posttranslational modification of the plastidic enzyme(s). Immunoprecipitation of 32P-labeled samples with P1 isoform-specific antibodies showed that the chloroplast enzyme is subject to protein phosphorylation. Obviously, in extended dark periods, G6PDH activity in the stroma is restricted but can be stimulated in response to high demands for NADPH.
Glc-6-phosphate dehydrogenases (G6PDHs, EC 1.1.1.49) catalyze the oxidation of Glc-6-phosphate (G6P) to 6-phosphogluconolactone concomitant with reducing NADP to NADPH. The product 6-phosphogluconolactone is first converted to 6-phosphogluconate by 6-phosphogluconolactonase (EC 3.1.1.31) and then decarboxylated by 6-phosphogluconate dehydrogenase (6PGDH, EC 1.1.1.44), yielding another mole of NADPH and ribulose-5-phosphate. The first enzyme, G6PDH, controls the flux through this nonreversible limb of the oxidative pentose phosphate pathway (OPPP; Williams, 1980  ; Copeland and Turner, 1987). In higher plants, G6PDH isoenzymes reside in two compartments, the cytosol and plastids (Heber et al., 1967; Schnarrenberger et al., 1973). Reducing power (NADPH) generated by the OPPP sustains reductive biosyntheses (e.g. fatty acids, isoprenoids and aromatic amino acids) in the dark and nitrogen assimilation in heterotrophic tissues (Bowsher et al., 1992). In addition, OPPP intermediates are continuously withdrawn to fuel other metabolic pathways. For example, erythrose-4-phosphate, produced by the Calvin cycle in the light and by the OPPP in the dark, is a substrate of the shikimate pathway and, thus, needed as precursor of aromatic amino acids, cell wall polymers, phytoalexins, and pigments. All enzymatic steps of the shikimate pathway up to chorismate are confined to plastids (Schmid and Amrhein, 1995). Schnarrenberger et al. (1995) postulated that in plants, only the irreversible reactions of the OPPP might be present in the cytosol. This has recently been supported by the work of Eicks et al. (2002), who characterized a pentose phosphate translocator of the inner chloroplast membrane from Arabidopsis. Bioinformatic analyses of the Arabidopsis genome revealed that genes for both cytosolic and plastidic isoforms of Rib-5-phosphate isomerase and ribulose-5-phosphate-3-epimerase are present, but for transketolase and transaldolase, cytosolic isoforms are missing. Thus, the oxidative branch of the OPPP in the cytosol probably operates in close connection with the complete pathway in plastids.
Sequences coding for NADP-dependent G6PDH enzymes exist in all organisms except for Archaebacteria (Wendt et al., 1999
Information on in planta regulation of G6PD isoforms is limited. Several studies in the past describing conditions that stimulate G6PDH activity (pathogen attack and elicitation) did not distinguish between the different isoenzymes nor analyze possible regulatory mechanisms involved (Endo and Veech, 1969
In heterotrophic tissues, plastidic G6PDH (and 6PGDH) activities provide reductive power (NADPH) for nitrogen assimilation. Several situations are known to modify metabolic fluxes through the plastid-localized OPPP: Oji et al. (1985 This work aimed at elucidating factors that result in changes of cytosolic and plastidic G6PDH activity. We adopted a leaf disc system to examine the effects of various treatments (feeding metabolites, inhibitors, etc.) on G6PD isoforms in potato. We determined maximal G6PDH activities (by differential inactivation of plastidic G6PDH with DTTred), protein abundance (with isoenzyme-specific antibodies), and transcript levels (using isoform-specific cDNA probes) and sequenced the promoter region of a genomic DNA fragment coding for the cytosolic isoform. Based on the obtained results, we suggest that discrete mechanisms contribute to the regulation of cytosolic and plastidic G6PDH isoenzyme activity in planta.
Rational for the Method of Choice We chose incubation experiments to study short-term influences of water-soluble substances on G6PDH-isoenzyme activities in potato leaf tissue. Activities were determined in leaf disc extracts after different incubation times in the dark and in the light. In addition, mRNA levels of the different G6PD isoforms were analyzed by northern-blot hybridization and protein contents by immunodetection on western blots. Leaf surface served as reference to account for deviations in protein content that result from degradation of Rubisco during long-term incubations in the dark. In this way, dark- and light-incubated samples and also different experimental series can be compared.
Cytosolic G6PDH activity remained constant during water incubation of leaf discs in the dark (Figs. 1, 2, 3). In the light, activities increased 5- to 7-fold compared with water controls in the dark (Figs. 1 and 3). Within 48 h, cytosolic G6PDH activity increased steadily and then remained at a constant level. Comparable stimulation was also triggered by incubation of leaf discs on 50 mM Glc in the dark (Figs. 1, 2, 3). Incubation on 50 mM mannitol or 100 mM KCl did not affect G6PDH activity, demonstrating that the observed increases are not due to osmotic or salt effects (data not shown). Presence of the electron-consuming herbicide Paraquat (5 µM methylviologen) or an inhibitor of photosynthetic electron transport (100-500 µM DCMU) in the light had no effect, indicating that oxidative stress and light as such are not responsible for the activity increases.
The following experiments demonstrate the effects of different sugars on cytosolic G6PDH activity. Leaf discs were incubated either on Suc, Fru, Glc, or Man, respectively. Incubation on Suc (25 mM) or Fru (50 mM) in darkness reproducibly led to higher increases of cytosolic G6PDH activity and corresponding mRNA levels compared with Glc (Fig. 2, A and B). Stimulation by Fru was always higher than by Suc. Hybridization of total RNA isolated from leaf discs incubated on water or different sugars, using cDNA fragments of the cytosolic isoform (von Schaewen et al., 1995 Chx (1 mM) inhibited both the increase of cytosolic G6PDH activity in water-incubated samples in the light (not shown) and upon feeding Glc in the dark (Fig. 3A). Water incubation in the light was always equivalent to Glc incubation in the dark, although here Glc in the dark stimulates cytosolic G6PDH activity to higher levels compared with water in the light (compare with Fig. 1). Western-blot analyses using a polyclonal antiserum specific for cytosolic G6PDH revealed that elevated protein contents correspond to the observed increases in activity and mRNA levels. Because Chx prevents de novo synthesis of cytosolic G6PDH protein (Fig. 3B), elevated activity of this isoform seems to result from regulation at the transcriptional level, most likely triggered by accumulation of metabolizable sugars in the cytosol.
Similar to Paraquat, incubation of potato leaf discs in the presence of hydrogen peroxide (H2O2; 0.05, 0.1, and 10 mM), iron (100 µM FeIIICl3), ammonium (20 mM NH4Cl), NO2- (20 mM NaNO2), NO3- (20, 40, 100, and 250 mM NaNO3), or sulfate (SO42-; 50, 100, and 250 mM KSO4) had no influence on cytosolic G6PDH activity. Incubation with phosphatase inhibitors (50 µM Endothall, 0.5 µM Okadaic acid, or 20-100 mM NaF) also had no effect.
Incubation of leaf discs in the presence of Paraquat (methylviologen) in the dark has been described previously to induce oxidative stress (Bowler et al., 1991
Interestingly, stimulation of DTTred-sensitive G6PDH activity was not inhibited by Chx (Fig. 4A). Concomitantly, protein contents of the P1 isoform remained unchanged in Paraquat- or water-incubated samples (Fig. 4B). Hybridization of total RNA isolated from leaf discs incubated on water or Paraquat, using cDNA fragments of the plastidic P1 isoform (von Schaewen et al., 1995 To assess kinetic parameters, Km and Vmax values were determined in extracts prepared from leaf discs incubated on water or Paraquat, respectively. The results are shown in Table I. The values for cytosolic G6PDH activity did not change considerably (and can be regarded as internal control). However, for the redox-sensitive plastidic enzyme(s), the Km for binding substrate (G6P) was about 10 times lower upon Paraquat incubation, with no dramatic change in Km for binding cosubstrate (NADP). The Vmax values for G6P remained more or less unchanged, whereas those for NADP doubled in Paraquat-incubated samples.
Because stimulation of DTTred-sensitive G6PDH activity was not accompanied by increased protein contents of the plastidic enzymes, nevertheless resulting in a Km (G6P) change for binding substrate, we examined whether posttranslational modification, e.g. phosphorylation, could account for the observed effect. Dark incubation of leaf discs on either water or Paraquat was conducted in the additional presence of 500 µCi 32P-orthophosphate. Protein extracts of labeled leaf discs were immunoprecipitated with antibodies specific for the P1 isoenzyme (von Schaewen et al., 1995 Unlike for the cytosolic enzyme, incubation of leaf discs with 50 mM Glc in the dark had no effect on DTTred-sensitive G6PDH activity (Fig. 4A). Combined incubation on Paraquat plus Glc in the dark did not influence the stimulation found with Paraquat alone. Incubation of leaf discs on Paraquat plus 500 µM DCMU in the light led to a 6-fold stimulation of DTTred-sensitive G6PDH activity, whereas Paraquat in the light alone had no effect (data not shown). Increased DTTred-sensitive G6PDH activity was also observed for NO2- incubations in the dark (NO2-, Fig. 5A) and similar time courses also for NO3- (data not shown), either alone or in combination with Glc. High concentrations (100 mM) led to significant stimulation of DTTred-sensitive G6PDH activity, and simultaneous feeding of Glc sustained the effect. For SO42- (Fig. 5B), the extent of stimulation depended on the additional presence of sugar (acceptor carbon skeletons). Incubation on equimolar salt solution (KCl served as a control) did not result in altered plastidic G6PDH activities (data not shown). In summary, G6PDH activity in chloroplasts of dark-held leaf tissue is rapidly inactivated at the posttranslational level, probably via phosphorylation of the existing enzyme pool. Conversely, enhanced activity of plastidic G6PDH would be triggered by dephosphorylation in situations imposing high demands for NADPH in the stroma.
Conditions Stimulating Cytosolic G6PDH Activity
During incubation of potato leaf discs, cytosolic G6PDH activity was stimulated about 5- to 7-fold above the initial value on either water in the light or upon feeding sugar in the dark. Blocking photosynthetic electron transport by DCMU in the light prevented the effect, which demonstrates that stimulation of cytosolic G6PDH activity is not due to light as such, but results from translocation of photosynthate (sugar) into the cytosol. In the leaf disc system, export of endogenously synthesized sugars via active phloem loading is unlikely because, after excision, sieve elements are rapidly clogged by callose deposition (Müller-Röber et al., 1990
According to the Chx and western-blot experiments, increases in cytosolic G6PDH activity require de novo protein synthesis. Northern-blot analyses showed that the mRNA levels correlate well with enhanced enzyme activities and protein amounts of cytosolic G6PDH. These results prompted us to examine the 5' region of the corresponding gene. A clone hybridizing to the cDNA sequence of cytosolic G6PDH (Graeve et al., 1994
The promoter of the cytosolic G6PD gene harbors several conserved elements in identical or slightly modified form known to be present in promoters of genes that are regulated by carbohydrate availability (Fig. 6). Among others, SURE1 and SURE2 motifs of patatin (Mignery et al., 1988
Several systems involved in sugar-mediated gene regulation are currently discussed (for review, see Koch, 1996
Due to the results of various sugar feeding studies, the response pattern of cytosolic G6PDH activity can be compared with the regulation of genes encoding enzymes of the glyoxylate pathway (described for suspension cultures of Cucumis sativus; Graham et al., 1994
In the leaf disc system, enhanced cytosolic G6PDH activity (resulting from increased gene expression) is also induced by Man. In the past, Man was frequently used to induce phosphate sequestration (Brouquisse et al., 2001
A considerable part of photosynthate is deposited as transitory starch in the stroma and can exit the chloroplast in two ways: (a) as triosephosphate (upon phosphorolytic starch breakdown via G6P) using the triose-phosphate/3-phosphoglycerate/phosphate anti-porter (Fliege et al., 1978 Here, we demonstrate that water incubation of leaf discs in the light has the same effect as sugar incubation in the dark, and, thus, can be considered a metabolic sink situation. We did not observe an additive effect of Glc and light incubation (data not shown). Supposedly, the responsible sugar sensor in the cytosol cannot differentiate between Glc imported across the plasma membrane and Glc exported from chloroplasts. Hexose accumulation could be sensed by hexokinase (or a yet unknown downstream sensor), and further signaling leads to up-regulation of the gene encoding cytosolic G6PDH in the nucleus.
The results are summarized in a model of G6PDH regulation in potato leaf tissue (Fig. 7). Substrate availability, i.e. hexoses accumulating in the cytosol (either upon export of Glc from the chloroplasts or supplied exogenously), is perceived via stimulation of an intracellular sugar sensor—possibly by hexokinase or a yet unknown downstream sensor (Huijser et al., 2000
Because incubation of leaf discs on FeIIICl3, Paraquat, H2O2, Endothall, Okadaic acid, NO2-, NO3-, or SO42- did not alter cytosolic G6PDH activity, we predict that compounds known to cause oxidative stress (FeIIICl3, Paraquat) or defense reactions (H2O2) do not influence cytosolic G6PDH activity directly but act through changes in the cellular carbohydrate state known to switch from "source" to "sink" under these conditions.
Increased demand for reductant triggered either by Paraquat, NO2-, NO3-, or SO42- in the dark led to rapid posttranslational stimulation of DTTred-sensitive G6PDH activity. Thus, regulation of the plastidic enzyme(s) completely differs from the cytosolic counterpart. Conditions stimulating cytosolic G6PDH did not affect plastidic activity; conversely, sugar availability (the stimulus leading to upregulation of the cytosolic isoform) had no effect on DTTred-sensitive G6PDH activity. This is surprising and demonstrated best by two graphs that are based on the same incubation experiment (compare Fig. 1 with Fig. 4A). Glc in the dark stimulates only the cytosolic isoform, and Paraquat in the dark only stimulates plastidic G6PDH activity. Substrate for plastid-localized G6PDH in the dark is most likely provided by mobilization of transitory starch. This was shown previously by Thom and Neuhaus (1995
The herbicide Paraquat, a bipyridin derivative (1,1'-dimethyl-4,4'bipyridin) is known to act as strong electron acceptor of PSI in the light and of NADPH in the dark, mediated by either FNR or ferredoxin (Brian, 1964
The stimulation of chloroplast G6PDH activity triggered by an increased stromal demand for electrons in the dark prompted us to investigate the responsible regulatory mechanism. First, the increase in DTTred-sensitive G6PDH activity induced by Paraquat in the dark was not inhibited by Chx. Simultaneous incubation on Glc, Paraquat, and Chx led to stimulation of only plastidic but not cytosolic G6PDH activity (data not shown), which proved that the chosen Chx concentration inhibited translation of nuclear-encoded mRNA without toxic effects on the tissue. Second, for the incubation period studied (72 h), we demonstrate that regulation of cytosolic and plastidic G6PDH activities operate independently. The two identified stimuli (Glc for the cytosolic isoform, increased demand for NADPH in case of the plastidic enzyme[s]) do not influence each other, despite a possible interaction between cytosolic and plastidic OPPP at the level of C5 sugar phosphates via the recently characterized pentosephosphate translocator (Eicks et al., 2002 In contrast to cytosolic G6PDH, stimulation of plastidic G6PDH activity did not depend on de novo protein synthesis. Independent of Chx inhibition, DTTred-sensitive G6PDH activity increased about 4-fold (when compared with the initial value) and 10-fold (when compared with water controls incubated in parallel, see Figs. 4 and 5). Protein amounts detected on western blots using isoform-specific antibodies for P1 (Fig. 4B) or P2 (data not shown) did not change and, hence, cannot be responsible for the rapid stimulation of DTTred-sensitive G6PDH activity.
The differences in apparent Glc6P of DTTred-sensitive G6PDH activity indicated that Paraquat incubation probably influences the plastidic enzyme(s) by covalent modification. Km and Vmax were determined in crude extracts and, therefore, are difficult to compare with values previously reported for enriched or partially purified enzyme preparations. Kinetic comparisons must also take into account that the values published by Scheibe et al. (1989
The obtained results led to the conclusion that posttranslational modification of plastidic G6PDH is responsible for the rapid activity changes. An effect of redox state can be excluded because for both stimulated and unstimulated enzyme forms, G6PDH activity was determined as difference between samples pre-incubated with either buffer or DTTred. Incubation in the presence of 32P-labeled orthophosphate revealed that at least the P1 enzyme is subject to protein phosphorylation. Incorporation of label increased with time and was much less pronounced in Paraquat-incubated samples. In the dark, 32P-orthophosphate fed to plant cells must first enter the mitochondria for incorporation into ATP and is only then imported by plastids via counterexchange with ADP (Heldt, 1976
For plastid-encoded genes, redox modification and phosphorylation are known to play important regulatory roles (e.g. transcription factor, Tiller and Link, 1993
Tests intended to prevent Paraquat-mediated stimulation of plastidic G6PDH activity using the phosphatase inhibitors Endothall or Okadaic acid were unsuccessful (data not shown), possibly due to low uptake into intact leaf tissue (discs floating upside down on the solutions) where the cuticle forms a potential barrier for these substances. Another reason could be that to act, the inhibitors have to reach the chloroplast stroma, whereas they only need to cross the plasma membrane to contact potential cytosolic targets, as described in the work of Sheen (1993
Large variations of G6PDH activity in chloroplasts were reported earlier (see Schnarrenberger et al., 1995
It appears that chloroplast G6PDH is affected by the stromal redox state at three levels: (a) NADPH is known to act as a competitive inhibitor of G6PDH (Lendzian and Bassham, 1975 It remains to be shown whether there is hierarchy between redox regulation and phosphorylation in vivo. Phosphorylation could act either directly by influencing the catalytic properties of the enzyme or indirectly by interfering with redox regulation. We currently favor the idea that regulation by phosphorylation developed as a means to restrict plastidic G6PDH activity in the oxidized (dark-activated) state. In any case, the two posttranslational mechanisms ensure a quick and tight adaptation of plastidic G6PDH activity to alterations in stromal redox state simply by changing the kinetic properties of the enzyme.
The observation that plastidic G6PDH activity is stimulated by the demand for stromal NADPH prompted us to test other potential stimuli. The importance of plastidic electron transport for NO2- assimilation was reported earlier (Paneque et al., 1964 We observed stimulation of plastidic G6PDH by NO2-, NO3-, and also by SO42- plus Glc that were comparable with those seen with Paraquat. This shows that physiological electron acceptors can replace Paraquat in stimulating plastidic G6PDH activity in the dark. A major function of the OPPP in darkened leaves seems to be sustained provision of reducing equivalents for biosyntheses like nitrogen and sulfur assimilation. To our knowledge, this is the first direct experimental evidence for an interaction of the plastidic OPPP with SO42- reduction and proves that stimulation by Paraquat is not a result of unspecific tissue damage. The concentrations of NO3- or SO42- used in this study were fairly high but were chosen to provoke a clear response and to yield plastidic G6PDH activities comparable with those observed with Paraquat. Because equimolar KCl concentrations did not stimulate plastidic G6PDH activity, salt effects can be excluded. The leaf disc system seems to be rather insensitive to SO42- or NO3- feeding, which probably reflects absence of high-affinity uptake mechanisms in leaf tissue. The effect of NO2- in lower concentrations (20 mM) may be due to its high membrane permeability and/or toxicity and the resulting need for rapid reduction. It is important to note that feeding cytosolic electron acceptors (FeIIICl3 and NO3-) did not lead to increased cytosolic G6PDH activity, showing that this enzyme is not directly regulated by the demand for reductant. Our experiments clearly demonstrate interaction of carbohydrate metabolism with nitrogen and sulfur assimilation. Addition of Glc (50 mM) to NO2-, NO3-, or SO42- incubations resulted in higher plastidic G6PDH stimulation than with NO3-, NO2-, or SO42- alone because sugars provide the carbon backbone for ammonium and sulfide acceptors (Glu and O-acetyl-Ser, respectively). The finding that NO2-, NO3-, and SO42- exert the same effect as Paraquat in the dark demonstrates that up-regulation is not stimulus specific but a result of NADPH shortage in the stroma, which somehow influences the catalytic state of the plastidic enzyme(s). Thus, posttranslational regulation of chloroplast G6PDH can be summarized as follows: Redox modification via dithiol/disulfide interchange of two regulatory Cys in the cosubstrate binding domain represents a coarse "off/on" switch during light/dark transitions, and the phosphorylation state probably determines the extent of catalytic activity of the dark-activated (oxidized) enzyme.
The results suggest that regulation of G6PDH enzymes in the cytosol and in chloroplasts are governed by distinct mechanisms. Figure 7 shows a hypothetical model based on the elucidated regulation principles. High sugar levels in the cytosol trigger elevated transcription of the cytosolic G6PD gene via sugar-mediated signaling to the nucleus. Increased mRNA expression results in higher enzyme levels and G6PDH activity. C5 sugar phosphates formed in the cytosol can be used for nucleotide synthesis or are transported into plastids to replenish continuous withdrawals of R5P and E4P (by plastid-localized nucleotide synthesis and the shikimate pathway, respectively), which is especially important in metabolic sink situations (i.e. in darkness and in heterotrophic tissues). In contrast, G6PDH activity in plastids can be stimulated by low NADPH to NADP ratios (most likely via dephosphorylation of the existing enzyme pool) and is restricted in prolonged dark periods (probably via phosphorylation). This ensures quick adaptation of the OPPP to short-term NADPH shortage in the stroma and could help to poise the important but labile balance of stromal reduction charge in the night, when alternative mechanisms like the malate valve (Fickenscher and Scheibe, 1983 ) are inactive.
Harvest and Incubation of Potato (Solanum tuberosum L. cv Désirée) Leaf Discs Potato seed tubers stored at 16°C for approximately 6 months were planted in a soil:compost:sand mixture (3:3:1 [v/v]) and grown in climate chambers under controlled conditions (10 h of light, 200 µmol m-1 s-1 at 25°C; 14 h of dark at 20°C). When the plants were about 4 weeks old, discs were cut from both sides of the midrib using a cork borer (i.d. = 7 mm) of leaves numbered 3 to 5 (counted from the top, the first leaf measuring about 1 cm in length) always at the beginning of the light period. Up to 30 leaf discs were floated upside-down (to minimize anaerobic effects) on different solutions. Water served as a control. The following substances were tested alone or in combination: 50 mM Glc, Fru, Man, 3-O-MG, or mannitol, respectively; 25 mM Suc; 100 mM KCl; 50 mM KH2PO4; 5 mM 2-deoxy-Glc; 1 mM Chx; 0.1 mM DCMU; 5 µM Paraquat (methylviologen); KNO3 (20, 40, 100, and 250 mM); 20 mM NaNO2 (to avoid toxic effects); K2SO4 (50, 100, and 250 mM); KCl (100 and 250 mM); 50 µM Endothall; 0.5 µM Ocadaic acid; and NaF (20, 40, and 100 mM). All incubations were carried out on 20-mL volume in disposable petri dishes at room temperature for up to 72 h in the dark or in continuous light. After 6, 12, 24, 48, and 72 h, incubated leaf discs were removed from the solutions with forceps, briefly dried on filter paper, snap frozen, and stored in liquid nitrogen. To determine initial values of G6PDH activity (0 h of incubation), samples were directly harvested from the plants and frozen as above.
To reduce variations in the measurements due to the start material (discs cut from different regions of the leaf), we sampled three times two to three leaf discs and extracted them separately. Enzyme activities were determined twice from each of the three extracts. Thus, means ± SDs are based on six single values. The leaf disc extraction buffer consisted of 100 mM Trismaleate (pH 8), 5 mM
Total RNA was isolated with the RNeasy Plant Mini Kit (Qiagen, Hilden, Germany). Each sample consisted of six to eight leaf discs. Isolated RNA (15 µg each) was separated in denaturing agarose gels and blotted on nylon membranes (Hybond N+, Amersham Pharmacia Biotech, Freiburg, Germany). Blots were hybridized with radiolabeled cDNA fragments, washed, and exposed with x-ray film as described in von Schaewen et al. (1995
To label phosphoproteins, leaf discs were incubated in the additional presence of 500 µCi of H332PO4 (specific activity 9,000 Ci mmol-1; NEN, Meckenheim, Germany) diluted in 100 µM KH2PO4 (5-mL total volume). Extraction of radiolabeled leaf discs was in 1 mL of Tris-maleate buffer (also used for enzyme measurements and western blots; Graeve et al., 1994
A genomic potato DNA library cloned in
DNA fragments of isolated phage clones were ligated to compatible restriction sites of plasmid vector pBluescript SK (Stratagene, Heidelberg) using standard procedures (Sambrook et al., 1989
The authors thank Monika Nietschke for excellent technical assistance and the gardeners of the Plant Physiology Department in Osnabrück for continuous provision of healthy plants. They gratefully acknowledge the group of Uwe Sonnewald (IPK Gatersleben, Germany) for providing the genomic potato library and the helpful initial advice of Andrea Polle (Universität Göttingen, Germany) on setting up a leaf disc incubation system for potato. Received April 17, 2003; returned for revision April 23, 2003; accepted May 5, 2003.
1 This work was supported by the Deutsche Forschungsgemeinschaft (Scha 541/3). 
2 Present address: Institut für Pflanzenkrankheiten, Universität Bonn, Nu
3 Institut für Botanik, Universität Münster, Schlo * Corresponding author; e-mail Schaewen{at}uni-muenster.de; fax 49-251-83-23823.
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ABSTRACT
RESULTS
EMBL3 (kindly provided by the group of Uwe Sonnewald, IPK Gatersleben, Germany) was screened using the entire radiolabeled NotI-cDNA fragment of the cytosolic G6PD isoform as a probe (Graeve et al., 1994
