High-Temperature Perturbation of Starch Synthesis Is Attributable to Inhibition of ADP-Glucose Pyrophosphorylase by Decreased Levels of Glycerate-3-Phosphate in Growing Potato Tubers

doi:10.1104/pp.117.4.1307

High-Temperature Perturbation of Starch Synthesis Is Attributable to Inhibition of ADP-Glucose Pyrophosphorylase by Decreased Levels of Glycerate-3-Phosphate in Growing Potato Tubers¹

Peter Geigenberger^*, Michael Geiger, and Mark Stitt

Botanisches Institut, Im Neuenheimer Feld 360, D-69120 Heidelberg, Germany

ABSTRACT

Top
Abstract
Introduction
Methods
Results
Discussion
References

To investigate the short-term effect of elevated temperatures on carbon metabolism in growing potato (Solanum tuberosum L.)tubers, developing tubers were exposed to a range of temperaturesbetween 19°C and 37°C. Incorporation of [¹⁴C]glucose (Glc) into starch showed a temperature optimum at 25°C.Increasing the temperature from 23°C or 25°C up to 37°C led todecreased labeling of starch, increased labeling of sucrose (Suc)and intermediates of the respiratory pathway, and increased respirationrates. At elevated temperatures, hexose-phosphate levels wereincreased, whereas the levels of glycerate-3-phosphate (3PGA)and phosphoenolpyruvate were decreased. There was an increasein pyruvate and malate, and a decrease in isocitrate. The amountof adenine diphosphoglucose (ADPGlc) decreased when tubers wereexposed to elevated temperatures. There was a strong correlationbetween the in vivo levels of 3PGA and ADPGlc in tubers incubatedat different temperatures, and the decrease in ADPGlc correlatedvery well with the decrease in the labeling of starch. In tubersincubated at temperatures above 30°C, the overall activities ofSuc synthase and ADPGlc pyrophosphorylase declined slightly, whereassoluble starch synthase and pyruvate kinase remained unchanged.Elevated temperatures led to an activation of Suc phosphate synthaseinvolving a change in its kinetic properties. There was a strongcorrelation between Suc phosphate synthase activation and thein vivo level of Glc-6-phosphate. It is proposed that elevatedtemperatures lead to increased rates of respiration, and the resultingdecline of 3PGA then inhibits ADPGlc pyrophosphorylase and starchsynthesis.

INTRODUCTION

Top
Abstract
Introduction
Methods
Results
Discussion
References

Potato (Solanum tuberosum L.) yield is limited by high temperatures, which restricts the use of this plant in the tropics(Awan, 1964; Burton, 1986), the optimum temperature for tubergrowth being around 22°C (Burton, 1986). Several factors couldbe responsible for this phenomenon. Elevated temperatures leadto (a) increased photorespiration and inhibition of net photosynthesisin leaves (Berry and Björkman, 1980); (b) increased respirationrates and therefore a considerable loss of photosynthate in growingsinks such as roots (Farrar and Williams, 1991); and (c) a reductionof Suc import into storage sinks such as potato tubers (Wolf etal., 1990).

However, several studies provide evidence that the reduced carbon import into potato tubers at high temperature is attributableto reduced Suc mobilization in the tuber itself, and not justto a shortage of photosynthate supply (Kraus and Marschner, 1984;Mohabir and John, 1988; Wolf et al., 1991). There are two linesof evidence. First, inhibition of potato tuber growth at elevatedsoil temperatures is accompanied by increased Suc levels in thetubers as well as in the leaves, indicating a block of Suc breakdownand starch synthesis in the tubers (Wolf et al., 1991; Midmoreand Prange, 1992). Second, compared with other cellular processessuch as respiration, which increase with temperature up to 40°C,the optimum temperature for starch synthesis is relatively low(Mohabir and John, 1988). Short-term experiments with [¹⁴C]Suc supplied to discs of growing potato tubers (Mohabir andJohn, 1988) demonstrated a sharp temperature optimum for starchsynthesis at approximately 21.5°C. Increasing the temperatureto 30°C led to a 50% reduction of starch synthesis, whereas respirationrates were increased 2-fold. This was also confirmed in long-termexperiments (Kraus and Marschner, 1984). When individual tubersof a potato plant were subjected to 30°C for 6 d, incorporationof ¹⁴C-labeled assimilates into starch, as well as the starch contentand the growth rate of the tubers, were significantly reduced,whereas the incorporation of ¹⁴C-labeled assimilates into the sugar fraction was not affectedby high tuber temperature.

The reasons for this decrease in starch synthesis at elevated temperatures are not clear. Decreased starch synthesis at elevatedtemperatures could be caused by (a) a direct inhibition of starchbiosynthetic enzymes in the plastid (i.e. increased heat-stresssusceptibility or thermolability of enzyme activities) and/or(b) a decrease in the levels of precursors caused by increasedrespiration or decreased Suc mobilization. Elevated temperaturesled to a decrease in AGPase activity when individual tubers ofa potato plant were subjected to 30°C for 6 d (Kraus and Marschner,1984), or to a reduction of AGPase and SuSy activities in thetubers when whole potato plants were transferred from 19/17°Cto 29/27°C (day/night) for 14 d (Lafta and Lorenzen, 1995), indicatingthat the site responsible for this temperature-induced responseis associated with AGPase or SuSy. Short-term studies, however,indicate that the temperature sensitivity of starch synthesisis caused by an interaction with processes in the cytosol becausea temperature shift from 21 to 31°C perturbed starch synthesisin tissue slices but not in cell-free amyloplasts of potato tubers(Mohabir and John, 1988).

At present, interpretation of changes in respiration, starch, and Suc metabolism at elevated temperature in potato tubersis limited by a lack of detailed information about changes inthe levels of metabolites and nucleotides. This information isnecessary to decide at which site(s) inhibition of starch synthesisoccurs and to elucidate possible regulation mechanisms. In thisarticle, our aim was to identify the enzymatic step(s) at whichfluxes are being regulated in response to a short-term increasein temperature. To do this, we incubated growing potato tubersat different temperatures from 19°C to 37°C, measured the fluxof [¹⁴C]Glc to starch, Suc, or glycolysis, and investigated changesin the levels of metabolites in the pathway from Suc to starch,as well as glycolytic intermediates, organic acids, and nucleotides.To elucidate a possible regulatory mechanism, we also investigatedseveral enzyme activities, including AGPase, soluble starch synthase,SuSy, and SPS.

	MATERIALS AND METHODS

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Potato (Solanum tuberosum L., cv Desirée) plants (Saatzucht Fritz Lange, Bad Schwartau, Germany) were grown in a growth chamber(350 µmol photons m² s¹, 20°C, 50% RH) in 5-L pots in soil supplemented with Hakaphosgrün (100 g/230 L soil; BASF, Ludwigshafen, Germany) under a14-h/10-h day/night regime. Growing tubers (about 2-4 g freshweight) from 6- to 8-week-old daily-watered plants were used forthe experiments. The tubers had high activities of SuSy, whichis taken as an indicator of rapidly growing tubers (Merlo et al.,1993).

Labeling Experiments and Fractionation of ¹⁴C-Labeled Tissue Extract

Labeling experiments were carried out with intact, growing tubers taken from fully photosynthesizing plants. Immediately afterharvest, tubers (approximately 2-4 g fresh weight) were incubatedin wet sand at temperatures from 19°C to 37°C. In parallel experiments,the temperature was measured inside of the tubers and it couldbe documented that the treatment described above increased tubertemperature from 19°C to 37°C within 15 to 20 min (data not shown).After 15 min, high-specific-activity [¹⁴C]Glc (12.5 GBq/mmol) was injected into a fine borehole throughthe middle of the tuber as described by Geigenberger et al. (1994)

,and tubers were incubated for another 45 min at the appropriatetemperature until a concentric cylinder (8 mm in diameter) aroundthe borehole was harvested and frozen in liquid nitrogen. Labeledtissue was extracted with 80% (v/v) ethanol at 80°C and reextractedin two subsequent steps with 50% (v/v) ethanol, and the combinedsupernatants were dried under an air stream at 40°C, taken upin 1 mL of water (soluble fraction), and separated in Suc, Glc,Fru, and ionic components by TLC as described by Geigenbergeret al. (1997)

. The insoluble material left after ethanol extractionwas homogenized, taken up in 4 mL of water, and counted for starch.In growing tubers starch accounts for more than 90% of the labelin the insoluble fraction (Geigenberger et al., 1994

Metabolite Analysis

Tubers were incubated in parallel for metabolite analysis. After 45 min of incubation in wet sand at temperatures from 19°Cto 37°C, tubers were harvested and cut into small discs (1-2 mmthick), which were placed into liquid N₂ immediately. The samplingprocedure lasted only a few seconds. The frozen material was homogenizedunder liquid nitrogen using a mortar and pestle. An aliquot ofthe frozen powder (approximately 0.5 g fresh weight) was extractedwith TCA (Jelitto et al., 1992), and hexose phosphates, 3PGA,PEP, pyruvate, pyrophosphate, and malate were measured as describedby Merlo et al. (1993)

; isocitrate was measured according to themethod of Beutler (1985)

. The recovery of small, representativeamounts of each metabolite through the extraction, storage, andassay procedures has been documented (Hajirezaei and Stitt, 1991

;Jelitto et al., 1992). Nucleotides, including UDPGlc, ADPGlc,ATP, and ADP, were measured in TCA extracts by HPLC using a chromatograph(Kontron Instruments, Eching, Germany) fitted with a Partisil-SAXanion-exchange column as described by Geigenberger et al. (1997)

.Recovery of a small representative amount of ADPGlc during extraction,storage, and analysis has been documented by Geigenberger et al.(1994)

Analysis of Enzyme Activities

Aliquots of the frozen powder (see above) were extracted and spin desalted, and SPS was immediately assayed via the anthronetest as described by Geigenberger et al. (1997)

. Aliquots of theextract were snap frozen in liquid nitrogen and assayed for SuSy,PK, and AGPase as described by Merlo et al. (1993)

, and for solublestarch synthase according to the method of Jenner et al. (1994)

Respiration Measurements

Immediately after being cut from a growing tuber attached to the plant, potato tuber discs (2 mm thick, 8 mm in diameter)were transferred into the temperature- controlled measuring chamberof an oxygen electrode (Hansatech, King's Lynn, Norfolk, UK) containing1 mL of buffer solution (10 mM Mes-KOH, pH 6.5), to measure oxygenconsumption at 16°C, 21°C, 25°C, 30°C, 33°C, and 37°C.

	RESULTS

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Elevated Temperatures Inhibit Starch Synthesis and Stimulate Respiration and Suc Resynthesis

Growing tubers (2-4 g fresh weight) were taken from 6-week-old plants and incubated at 19°C, 25°C, 30°C, and 37°C in wet sand.To measure fluxes, high-specific-activity [¹⁴C]Glc was injected into the tubers for 45 min, and the incorporationof label into starch, Suc, and ionic components (cations plusanions) was analyzed. The results are expressed as percentageof the total ¹⁴C injected (Fig. 1, A-D). With increasing temperature, an increasingamount of label was metabolized (Fig. 1A). Incorporation of labelinto starch showed a temperature optimum at 25°C (Fig. 1B), decreasingby 25% and 38% when temperature was increased to 30°C and 37°C,respectively. Compared with this, labeling of ionic components(mainly phosphate ester and organic and amino acids), which isan estimate of flux in glycolysis and respiration, increased withtemperatures up to 37°C in a linear manner (Fig. 1C). This wasconfirmed by an independent approach in which oxygen electrodeswere used to measure oxygen consumption in freshly cut potatotuber discs at different temperatures. Oxygen consumption (measuredin nmol g¹ fresh weight min¹) was 20.7 ± 1.9, 28.2 ± 1.1, 40.2 ± 3.9, 53.4 ± 1.8, 55.1 ± 1.0,and 62.7 ± 4.5 in discs incubated at 16°C, 21°C, 25°C, 30°C, 33°C,and 37°C, respectively (data are means ± SE, n = 4). These dataresemble those found in previous work using potato tuber discs(Mohabir and John, 1988

), in which an optimum for starch synthesisat 21.5°C was observed, whereas respiration increased in a linearmanner up to 30°C.

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Figure 1. Metabolism of [¹⁴C]Glc injected into tubers incubated at 19°C, 25°C, 30°C, and 37°C. Growing tubers (2-4 g fresh weight) were taken from 6-week-old plants that had just started to flower, and were incubated immediately in wet sand at different temperatures. After 15 min of preincubation at the temperatures indicated, [¹⁴C]Glc was injected into a fine borehole in the middle of the tuber, and tubers were sampled after another 45 min to analyze label remaining in Glc (A), and incorporation of label into starch (B), anions plus cations (glycolysis) (C), and Suc (D). In parallel experiments, the temperature was measured inside the tubers and it could be documented that the above treatment increased tuber temperature from 19°C to 37°C between 15 and 20 min (data not shown). Data are means ± SE of four individual tubers.

In potato tubers net Suc degradation is regulated by a cycle of Suc degradation and resynthesis (Geigenberger and Stitt, 1993).To investigate the rate of Suc resynthesis, incorporation of labelinto Suc was measured (Fig. 1D). Incorporation was low (about0.8% of total) at 19°C, increased when temperature was increasedto 25°C and 30°C, and showed an overproportional increase whentubers were incubated at 37°C. An overproportional increase inthe flux back to Suc is indicative of an induction of Suc cyclingand reduced net Suc degradation.

Changes of Metabolites

To identify potential sites for regulation, metabolites were measured in tubers of the same experiment (see Fig. 1) incubatedin parallel. As the temperature was increased from 19°C to 37°C,Glc-6-P levels increased progressively from 140 to 290 nmol g¹ fresh weight (Fig. 2B). 3PGA levels were low at 19°C, peakedat 25°C, and decreased again in tubers incubated at 37°C (Fig.2D). The decrease in starch synthesis at elevated temperatureswas therefore accompanied by an increase of hexose phosphatesand by a decrease of 3PGA (compare Fig. 1B with Fig. 2, B andD). Hexose phosphates are the immediate substrate and 3PGA isa potent activator of potato tuber ADPGlc pyrophosphorylase (Preiss,1988

). No consistent changes were observed in the levels of ATPand ADP (Fig. 3, A and B), UDPGlc (Fig. 2A), or PPi (data notshown).

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Figure 2. Metabolite levels in tubers incubated at 19°C, 25°C, 30°C, and 37°C. Tubers incubated in parallel to those used for radiolabel analysis (see Fig. 1, A-D) were sampled after 45 min for metabolite analysis. A, UDPGlc; B, Glc-6-P; C, Fru-6-P; and D, 3PGA. Data are means ± SE of four individual tubers. FW, Fresh weight.

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Figure 3. Levels of adenine nucleotides in tubers incubated at 19°C, 25°C, 30°C, and 37°C. ATP (A), ADP (B), and ADPGlc (C) were measured in the same extracts as in Figure 2. Data are means ± SE of four individual tubers. FW, Fresh weight.

Glycolytic and TCA-cycle intermediates were investigated in more detail in a second experiment in which tubers were incubatedat 23°C, 32°C, and 37°C (Table I). Labeling data for this experimentalso confirmed a decrease in the labeling of starch by 61% and65% at 32°C and 37°C. Decreased starch synthesis was again accompaniedby a 1.6-fold increase in hexose phosphates and an approximately50% decrease in 3PGA. There was also a 30% decrease in PEP, aslight increase of pyruvate and malate, and a decrease in isocitratefrom 21% to 44%. As a result, the PEP/pyruvate ratio declinedby 50%. This decrease was accompanied by increased fluxes to carbondioxide (see above). Together, these results show that there isa direct stimulation of the final respiratory reactions, leadingto a drain of TCA-cycle intermediates and a stimulation of reactionsconverting PEP to pyruvate (PK) or malate (PEPC).

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Table I. Levels of glycolytic intermediates and organic acids, metabolism of [¹⁴C]Glc, and enzyme activities in tubers incubated at 23°C, 32°C, and 37°C

Data are means ± SE of four to five individual tubers.

The observed increase in hexose phosphates (Fig. 2, B and C; Table I) indicates a block in starch synthesis. To distinguishbetween a block at ADPGlc pyrophosphorylase or at the final polymerizingreactions (i.e. starch synthases or branching enzyme) we measuredthe levels of ADPGlc (Fig. 3C). The level of ADPGlc increasedslightly when the temperature was increased to 25°C. ADPGlc decreasedby 23% and 45% in tubers incubated at 30°C and 37°C, respectively,which corresponds to the inhibition of starch synthesis at thesetemperatures (compare Figs. 3C and 1B). Similar trends were obtainedin a second experiment (Table I), in which ADPGlc decreased by78% and 85% in tubers incubated at 32°C and 37°C, respectively.Obviously, inhibition of starch synthesis is not accompanied byan accumulation of ADPGlc, which would be expected if solublestarch synthase were the regulatory site. The observed decreaseof ADPGlc was paralleled by a corresponding increase in hexosephosphates, which indicates that the temperature-sensitive siteis associated with AGPase.

Enzyme Activities

There were no marked changes in the maximal extractable activities of SuSy, AGPase, soluble starch synthase, or PK measuredin tubers incubated for 45 min at 19°C, 25°C, and 30°C (Fig. 4,A-D). At 37°C, however, a 40% decline of SuSy (Fig. 4A) and a27% decrease of AGPase activity (Fig. 4B) were observed. Theseresults were confirmed in a second experiment with a differentset of plants (Table I), in which AGPase activity decreased by32% to 50%, and SuSy activity decreased by 40% in tubers incubatedat 32°C and 37°C, whereas soluble starch synthase and PK did notchange significantly. In this experiment, tubers were used fromolder plants (8 weeks old) that had lower levels of enzyme activitiescompared with the plants from the experiment shown in Figure 4.

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Figure 4. Enzyme activities in tubers incubated at 19°C, 25°C, 30°C, and 37°C. SuSy (A), AGPase (B), soluble starch synthase (C), PK (D), and SPS (E-G) were measured in the same tubers as in Figure 2. SPS was measured under two different assay conditions: (E) V_max assay (12 mM Fru-6-P, 36 mM Glc-6-P, and 6 mM UDPGlc) or (F) V_sel assay (2 mM Fru-6-P, 6 mM Glc-6-P, 6 mM UDPGlc, and 5 mM Pi). G shows the ratio between the two activities. Data are means ± SE of four individual tubers. FW, Fresh weight.

To investigate whether the enhanced resynthesis of Suc was caused by stimulation of SPS, we also determined SPS activity.Activity was measured in two different assay conditions: (a) withsaturating hexose phosphates (termed V_max) to determine changesin maximal activities, and (b) with limiting hexose phosphatesand inhibitor Pi (termed V_sel) to determine whether the activationstate of the enzyme is modified by covalent modification (Sieglet al., 1990; Huber et al., 1992). Incubation of tubers at elevatedtemperatures did not have any consistent effect on SPS activitywhen it was assayed in the presence of saturating hexose-phosphateconcentrations (termed the V_max assay, with 12 mM Fru-6-P, 36mM Glc-6-P, and 6 mM UDPGlc; Fig. 4E and Table I). However, increasingthe temperature up to 37°C led to a 1.5- to 2-fold increase ofactivity when SPS was assayed in the presence of limiting substrates(termed the V_sel assay, with 2 mM Fru-6-P, 6 mM Glc-6-P, 6 mMUDPGlc, and 5 mM phosphate [Pi]; Fig. 4F and Table I). The increasein V_sel activity was especially marked in tubers exposed to 37°D,and coincided with the stimulation of Suc synthesis and the increasein hexose-phosphate levels (compare Figs. 4F, 1D, and 2B). TheV_sel-to-V_max ratio increased by 1.5- to 1.8-fold (Fig. 4G).

	DISCUSSION

Top Abstract Introduction Methods Results Discussion References

In short-term experiments, increasing the temperature from 23°C or 25°C up to 37°C leads to increased respiration, decreasedstarch synthesis, and increased resynthesis of Suc in growingpotato tubers. Similar changes of fluxes in response to elevatedtemperature were also seen in previous studies on potato tuberdiscs (Mohabir and John, 1988), but these earlier studies didnot provide in vivo information about the changes of metabolitesto allow the reasons for the inhibition of starch synthesis tobe identified.

Elevated Temperatures Lead to Increased Respiration, with the Resulting Decline in 3PGA Leading to Inhibition of AGPase and Starch Synthesis

The increase in respiration at high temperatures was accompanied by a 30% to 50% decrease of PEP and 3PGA, and a 50% decreasein the PEP-to-pyruvate ratio (Fig. 2; Table I). The increasedrate of glycolysis can therefore be attributed to activation ofPK and/or PEPC. Similar results have been obtained when respirationincreased in response to other factors, including increased carbohydratelevels (Geigenberger and Stitt 1991a

; Hatzfeld and Stitt, 1991

;Geiger et al., 1998

), addition of Gln or ammonia (Geigenbergerand Stitt, 1991b

), or addition of uncouplers (Hatzfeld and Stitt,1991

Potato tuber AGPase is allosterically activated by 3PGA (Sowokinos, 1981; Sowokinos and Preiss, 1982). The decrease in thelevel of 3PGA should therefore lead to an inhibition of AGPase.In agreement, the decrease in 3PGA at high temperature led toa decrease in ADPGlc and to an inhibition of starch synthesis(Fig. 5, A and B). We conclude that after activation of glycolysiscaused by increased respiration, a decrease of 3PGA leads to inhibitionof AGPase, and restricts the rate of starch synthesis. It mustbe noted, however, that the reported 3PGA levels are overall levelspresent in both the cytoplasm and the amyloplasts. Direct measurementsof subcellular metabolite levels will be needed to confirm ourinterpretation.

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Figure 5. Relation between 3PGA and ADPGlc (A) and ADPGlc and starch synthesis (B) in tubers exposed to different temperatures. Data are taken from Figures 1-3 and Table I, and are means ± SE of four individual tubers. FW, Fresh weight; Expt., experiment.

Hexose phosphates increased at elevated temperatures (Fig. 2; Table I), demonstrating that the inhibition of starch synthesisis caused by a direct inhibition of AGPase, rather than to a shortageof a substrate (i.e. via a block in Suc degradation). The declineof PEP and 3PGA (see above) would be expected to activate phosphofructokinase(Dennis and Greyson, 1987) and Fru-6-P2-kinase, leading to increasedFru-2,6-bisP and activation of PFP (Stitt, 1990), and this shouldstimulate the entry of hexose phosphates into glycolysis. Thefinding that hexose phosphates increase implies that the regulatoryloop leading to the stimulation of phosphofructokinase and PFPis not strong enough to lead to a decrease in hexose-phosphatelevels when respiration and glycolysis is stimulated by increasingtemperature. A similar result was obtained when respiration andglycolysis increased in response to an increased supply of carbohydrates(Geigenberger and Stitt, 1991a; Hatzfeld and Stitt, 1991; Geigeret al., 1998), addition of Gln or ammonia (Geigenberger and Stitt,1991b), or addition of uncouplers (Hatzfeld and Stitt, 1991).An alternative explanation for the increased hexose-phosphatelevels would be that starch degradation is stimulated in responseto high temperatures. Further studies are needed to investigatethe role of starch turnover in the regulation of starch synthesisin potato tubers.

Our results do not reveal the reasons for the stimulation of respiration at high temperatures. When temperature is increased,a general increase in the velocity of enzyme activities or chemicalreactions is to be expected and could lead to increased flux intothe respiratory pathways (Lambers, 1985). On the other hand, elevatedtemperatures will lead to increased membrane permeability, whichimpairs transport processes and increases energy costs to maintainmembrane gradients. However, there were no consistent changesin the overall levels of ATP or ADP in the tubers in responseto temperature that could be indicative of a stimulation of respirationattributable to an increased demand for ATP (Fig. 3). Increasedrespiration led to decreased isocitrate levels in the mitochondria(Table I), indicating a drain in TCA cycle intermediates causedby stimulation of the final oxidation process at the mitochondrialmembrane in response to high temperatures. This was accompaniedby activation of PK and/or PEPC and increased supply of substratesfor the TCA cycle. Accumulation of pyruvate and malate could alsoindicate that transport of substrates into the mitochondria isa limiting factor at elevated temperatures.

There was a 28% to 50% decrease in AGPase and a 40% to 50% decrease in SuSy activity measured under optimal conditions inextracts from tubers exposed to high temperatures (Fig. 4; TableI). Similar results were also obtained in previous experimentswith potato tubers (Kraus and Marschner, 1984; Lafta and Lorenzen,1995). It is very unlikely that the 50% decrease in the amountof AGPase or SuSy activities is responsible for the short-terminhibition of starch synthesis, since a similar decrease in enzymeactivity in tubers with reduced expression of AGPase (Müller-Röberet al., 1992) or SuSy (Zrenner et al., 1995) due to antisensedid not alter starch accumulation. However, changes in the amountof enzymes could amplify the effect of fine control mechanismsacting in parallel, leading to a higher degree of metabolic control.More studies are needed to elucidate the mechanisms leading tothe high-temperature-induced decrease in enzyme activity and todetermine if they lead to a further inhibition of starch synthesisduring a more prolonged exposure to high temperatures.

Inhibition of Starch Synthesis Is Accompanied by a Stimulation of Suc Synthesis Caused by Increased Hexose-Phosphate Levels and Activation of SPS

The inhibition of starch synthesis was accompanied by an accumulation of hexose phosphates (Fig. 2, B and C; Table I) andan overproportional increase of Suc resynthesis (Fig. 1D). Twofactors could be responsible for the stimulation of Suc synthesis.First, potato tuber SPS is subject to allosteric activation byGlc-6-P and inhibition by Pi (Reimholz et al., 1994

). Second,elevated temperatures led to increased activation of SPS, whichis expressed as a change in its kinetic properties, which allowshigher SPS activity in the presence of limiting substrate concentrations(Fig. 4, F and G). This resembles the effect of increased ratesof photosynthesis on leaf SPS phosphorylation (Huber and Huber,1996

). In the leaf system SPS is activated by dephosphorylationand SPS kinase is shown to be inhibited by hexose phosphates (McMichaelet al., 1995

). As shown in Figure 6, the increase in SPS activityassayed under selective conditions correlates with increased Glc-6-Plevels in potato tubers incubated at different temperatures. Accumulationof hexose phosphates in response to decreased starch synthesiswas also observed in tubers with reduced expression of AGPasevia antisense (R.N. Trethewey, P. Geigenberger, A. Hennig, H.Notter-Fleisch, and L. Willmitzer, unpublished results). Alsoin this case, a 2-fold increase in hexose phosphates was accompaniedby a 2-fold increase in SPS activation (Geigenberger et al., 1995

;P. Geigenberger, unpublished results). In potato tubers Suc mobilizationis regulated by a cycle of Suc synthesis and degradation (Geigenbergerand Stitt, 1993

; Geigenberger et al., 1995

, 1997

). The overproportionalincrease of Suc resynthesis at 37°C (Fig. 1D; Table I) is indicativeof an induction of Suc cycling and reduced net Suc degradation.This was paralleled by a 40% decrease in SuSy activity measuredin tubers incubated at 37°C (Fig. 4A; Table 1).

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Figure 6. Relation between the Glc-6-P level and the activity of SPS measured in the V_sel assay with limiting substrates and phosphate. Data are taken from Figures 2A and 4F and Table I, and are means ± SE of four individual tubers. FW, Fresh weight; Expt., experiment.

Role of AGPase in the Control of Starch Synthesis in Potato Tubers

In potato tubers an 80% to 95% reduction of AGPase expression led to decreased rates of starch accumulation (Müller-Röberet al., 1992

), whereas recent studies indicate that reducing solublestarch synthase to 20% of the wild-type level has no effect onstarch accumulation (Marshall et al., 1996

). This indicates theimportance of AGPase, rather than soluble starch synthase, incontrolling the rate of starch synthesis under normal growth conditionsin potato tubers. Under extreme water stress, the effect of starchsynthases on the flux to starch increases, which is indicatedby changes in ADPGlc levels (Geigenberger et al., 1997

). This,however, does not seem to be the case at high temperatures intubers (see above).

Our data indicate the importance of metabolic fine control of AGPase for the regulation of starch synthesis in potato tubers.A similar interaction of 3PGA with AGPase activity and starchsynthesis is found in transgenic potato tubers with decreasedexpression of PFP (Hajirezaei et al., 1994) or of NAD-malic enzyme(H.L. Jenner, B.M. Winning, C.J. Leaver, and S.A. Hill, unpublisheddata), and in wild-type tubers in response to moderate water stress(Geigenberger et al., 1997), or in leaves in response to waterstress (Quick et al., 1989) or a decreased availability of fixedcarbon (Stitt, 1990). This confirms previous studies on potatotubers overexpressing native and mutated Escherichia coli AGPase(Stark et al., 1992), demonstrating the significance of the allostericproperties of AGPase for the rate of starch accumulation.

The Effect of High Temperature on Starch Accumulation in Cereals

High temperature during the grain-filling process is also yield limiting in cereals, leading to a reduction in starch depositionand grain size (Chowdhury and Wardlaw, 1978

) caused by an impairedconversion of Suc to starch (Bhullar and Jenner, 1986

; MacLeodand Duffus, 1988

). The reasons for this adverse effect of temperatureon starch synthesis have been extensively studied in wheat endosperm.

In short-term experiments, isolated grains were heated at temperatures up to 40°C for 1 to 4 h (Jenner et al., 1993) or 3h (Keeling et al., 1993) to analyze enzyme activities and theflux of [¹⁴C]Suc or Glc to starch. In the study by Jenner et al. (1993),a sharp decline of soluble starch synthase was observed after30 min of exposure to 35°C, and a further but smaller reductionoccurred after 2 and 4 h. After 2 h at 35°C a significant butsmaller reduction of AGPase was also observed, whereas SuSy activityremained unchanged. A similar decrease of soluble starch synthasewas also observed by Keeling et al. (1993), although in this studyno significant changes in AGPase, SuSy, or UGPase were observedin the 3-h incubation period. In both of these studies, the decreaseof extracted soluble starch synthase observed at elevated temperatureswas highly correlated with the decrease in the rate of starchsynthesis (Jenner et al., 1993; Keeling et al., 1993). High temperaturesalso led to a marked change in the kinetic properties of starchsynthase extracted from wheat endosperm, leading to a loss ofcooperativity between glucans and ADPGlc (Jenner et al., 1995).

This decrease in starch synthase activity was also seen in long-term experiments. When wheat ears were exposed to 35°C for1 to 9 d, soluble starch synthase activity was reduced by morethan 50% and AGPase was decreased by about 26% (Hawker and Jenner,1993). In a previous study (Jenner, 1991), metabolite levels wereanalyzed in wheat ears exposed to elevated temperatures for upto 7 d to identify temperature-sensitive steps in the conversionof Suc to starch. Increasing the temperature from 16°C/21°C to25°C/35°C (night/day) resulted in a decrease in the levels ofmetabolites (hexose phosphates, UDPGlc, and ADPGlc), whereas theSuc content of the endosperm was either not affected or increased(Jenner, 1991). Hexose phosphates declined by 50% after 1 d andremained at a constant low level for the next 6 d. UDPGlc andADPGlc decreased more gradually during the entire time interval,being significantly reduced by 28% and 13%, respectively, comparedwith the low-temperature control. The overall decrease in metabolitelevels in wheat during long-term exposure to heat indicates thatthere may be additional factors besides an inhibition of starchsynthase that contribute to the small increase in starch depositionwith increasing temperature.

In potato tubers elevated temperatures lead to a decrease in the extracted amounts of SuSy and AGPase, and to inhibition ofAGPase due to decreased levels of 3PGA (see above), both mechanismsacting in concert and leading to an inhibition of starch synthesis.In wheat, however, inhibition of starch synthesis at elevatedtemperatures is associated with a decrease in the extracted amountof soluble starch synthase (see above). This might reflect differentroles of AGPase and starch synthases in controlling flux to starchin cereals such as wheat or barley compared with potato (Jennerand Hawker, 1993). In wheat or barley endosperm, for example,AGPase is less sensitive to 3PGA activation than in potato tubers(Jenner and Hawker, 1993; Kleczkowski et al., 1993), and at leastfor barley it could be shown that a considerable part of the AGPaseactivity is located outside of the plastid (Thorbjornsen et al.,1996).

	FOOTNOTES

¹ This work was supported by the Deutsche Forschungsgemeinschaft (SFB 199).
^* Corresponding author; e-mail pgeig{at}botanik1.bot.uniheidelberg.de; fax 49-6221-545859.

Received February 2, 1998; accepted May 1, 1998.

ABBREVIATIONS

Abbreviations: ADPGlc, adenine diphosphoglucose. AGPase, adenine diphosphoglucose pyrophosphorylase. PEPC, PEP carboxylase. PFP, pyrophosphate:Fru-6-P phosphotransferase. 3PGA, glycerate-3-phosphate. PK, pyruvate kinase. SPS, Suc phosphate synthase. SuSy, Suc synthase. UDPGlc, uridine diphosphoglucose. UGPase, uridine diphosphoglucose pyrophosphorylase.

	ACKNOWLEDGMENT

We are grateful to Steven Hill (Oxford, UK) for discussions and for making unpublished data available.

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High-Temperature Perturbation of Starch Synthesis Is Attributable to Inhibition of ADP-Glucose Pyrophosphorylase by Decreased Levels of Glycerate-3-Phosphate in Growing Potato Tubers1

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High-Temperature Perturbation of Starch Synthesis Is Attributable to Inhibition of ADP-Glucose Pyrophosphorylase by Decreased Levels of Glycerate-3-Phosphate in Growing Potato Tubers¹

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© 1998 American Society of Plant Physiologists