Metabolite Control Overrides Circadian Regulation of Phosphoenolpyruvate Carboxylase Kinase and CO2 Fixation in Crassulacean Acid Metabolism

doi:10.1104/pp.121.3.889

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Metabolite Control Overrides Circadian Regulation of Phosphoenolpyruvate Carboxylase Kinase and CO₂ Fixation in Crassulacean Acid Metabolism¹

Anne M. Borland,^* James Hartwell, Gareth I. Jenkins, Malcolm B. Wilkins, and Hugh G. Nimmo

Department of Agricultural and Environmental Science, University of Newcastle, Newcastle upon Tyne NE1 7RU, United Kingdom (A.M.B.); and Plant Molecular Science Group, Institute of Biomedical and Life Sciences, University of Glasgow, Glasgow G12 8QQ, United Kingdom (J.H., G.I.J., M.B.W., H.G.N.)

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Phosphoenolpyruvate carboxylase (PEPc) catalyzes the primary fixation of CO₂ in Crassulacean acid metabolism plants. Fluxthrough the enzyme is regulated by reversible phosphorylation.PEPc kinase is controlled by changes in the level of its translatablemRNA in response to a circadian rhythm. The physiological significanceof changes in the levels of PEPc-kinase-translatable mRNA andthe involvement of metabolites in control of the kinase was investigatedby subjecting Kalanchoë daigremontiana leaves to anaerobic conditionsat night to modulate the magnitude of malate accumulation, orto a rise in temperature at night to increase the efflux of malatefrom vacuole to cytosol. Changes in CO₂ fixation and PEPc kinaseactivity reflected those in kinase mRNA. The highest rates ofCO₂ fixation and levels of kinase mRNA were observed in leavessubjected to anaerobic treatment for the first half of the nightand then transferred to ambient air. In leaves subjected to anaerobictreatment overnight and transferred to ambient air at the startof the day, PEPc-kinase-translatable mRNA and activity, the phosphorylationstate of PEPc, and fixation of atmospheric CO₂ were significantlyhigher than those for control leaves for the first 3 h of thelight period. A nighttime temperature increase from 19°C to 27°Cled to a rapid reduction in kinase mRNA and activity; however,this was not observed in leaves in which malate accumulation hadbeen prevented by anaerobic treatment. These data are consistentwith the hypothesis that a high concentration of malate reducesboth kinase mRNA and the accumulation of the kinaseitself.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

In plants with Crassulacean acid metabolism (CAM), phosphoenolpyruvate carboxylase (PEPc) (EC 4.1.1.31) catalyzes the nocturnalfixation of atmospheric CO₂ (as HCO₃) into oxaloacetate, which is subsequently reduced to malate andstored in the vacuole. During the day, the decarboxylation ofmalate released from the vacuole generates a high intercellularpartial pressure of CO₂, which results in stomatal closure andthe conservation of water. The fixation of this internally generatedCO₂ by Rubisco continues behind closed stomata until malate decarboxylationnears completion and the CO₂ partial pressure drops. Stomata maysubsequently re-open and atmospheric CO₂ can then be fixed directlyvia the Calvincycle.

The temporal separation of these C₄ and C₃ carboxylation processes, which distinguishes CAM from C₄ photosynthesis, requiresthat the activity of PEPc be reduced during the day to curtailfutile cycling of CO₂ from concurrent malate synthesis and breakdown.The day/night regulation of flux through PEPc is achieved by reversiblephosphorylation that reduces the sensitivity of the enzyme toinhibition by L-malate with the phosphorylated, malate-insensitive(active) form of PEPc present at night (Nimmo et al., 1984, 1986).The phosphorylation state of PEPc is determined by the presenceor absence of a specific Ca²⁺-independent protein kinase termed PEPc kinase (Carter et al.,1991; Li and Chollet, 1994). Recently, Hartwell et al. (1996)used a novel approach in which the products of in vitro translationof leaf RNA were assayed directly for PEPc kinase activity todemonstrate that the activity of PEPc kinase reflects changesin the level of its translatable mRNA. Thus, levels of kinasemRNA were approximately 20-fold higher at night than during thedaytime in leaves of the CAM plant Kalanchoë (Bryophyllum) fedtschenkoi(Hartwell et al., 1996).

While the levels of PEPc kinase mRNA in C₃ and C₄ plants appear to respond to photosynthesis and, thus, light-dark transitions,in CAM plants a circadian oscillator controls the levels of kinaseactivity and translatable mRNA under constant environmental conditions(Carter et al., 1991; Hartwell et al., 1996). This results ina circadian rhythm in the phosphorylation state of PEPc (Nimmoet al., 1987), which plays an important role in generating theendogenous rhythms of CO₂ exchange in CAM plants first describedby Wilkins (1959). To date, the exact nature of the circadianoscillator in CAM is unknown, but recent observations indicatethat the timing of PEPc activation/deactivation varies betweendifferent CAM species grown under identical environmental conditions(Borland and Griffiths, 1997).

Physiological manipulations of dark CO₂ uptake and malate accumulation have indicated that the storage capacity of the vacuolefor malate plays a key role in determining the timing of the inactivationof PEPc (Winter and Tenhunen, 1982; Fischer and Kluge, 1984; Borlandand Griffiths, 1997). Thus, in plants prevented from accumulatingmalate overnight in an atmosphere of N₂, flux through PEPc increasessubstantially at the start of the day in ambient air, and theinactivation of PEPc is delayed by 2 to 3 h (Borland and Griffiths,1997). Observations that the circadian rhythms of phosphorylationof PEPc and CO₂ exchange can be disrupted and re-initiated bytemperature changes have also pointed to a key role for the tonoplastin malate compartmentation, and for malate itself in the generationof the endogenous rhythm of PEPc activity (Wilkins, 1983; Carteret al., 1991; Grams et al., 1997). Malate inhibits PEPc kinaseby binding to PEPc (Carter et al., 1991; Li and Chollet 1993,1994), although it is not clear whether this effect is physiologicallysignificant. Malate or other metabolites might also affect thephosphorylation of PEPc by acting at steps closer to the circadianoscillator. Such effects on the output from the oscillator couldprovide CAM plants with the flexibility to adjust C flux in responseto changes in environmentalconditions.

The aim of the present work was to study the relationship between leaf malate content, PEPc kinase activity, and levels oftranslatable kinase mRNA in intact plants of Kalanchoë daigremontianaHamet et Perr. Physiological manipulations involving anaerobictreatments and temperature changes in the dark were used to modulatethe magnitude of dark CO₂ uptake and malate accumulation. Theresults highlight the physiological importance of changes in translatablePEPc kinase mRNA in the CAM cycle and suggest that metabolites,most likely malate, affect the phosphorylation of PEPc at severallevels.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Plant Material and Growth Conditions

Plants of Kalanchoë daigremontiana Hamet et Perr., which were approximately 1 year old and growing in 10-cm-diameter pots,were acclimated in the growth chamber for 4 weeks prior to experimentation.All measurements were conducted on the fourth leaf pair from thegrowingtip.

The plants were acclimated in a growth chamber (Fitotron, Sanyo Gallenkamp, Leicester, UK) programmed to provide gradual changesin temperature, humidity, and photsynthetic photon flux density(PPFD) at the start and end of the photoperiod in an attempt tomimic conditions found naturally at dawn and dusk. From 8:30 AMuntil 12 PM, PPFD was increased to a maximum of 530 µmol m² s¹ at leaf height, the temperature was increased from 19°C to 27°C,and the relative humidity (RH) was decreased from 80% to 60% (thevapor pressure deficit was increased from 1.8-2.9 kPa). Theseconditions were maintained until 4 PM, when PPFD was decreasedgradually until the lights were off at 7:30 PM, the temperaturewas decreased to 19°C, and the RH was increased to 80% (the vaporpressure deficit was 1.8 kPa). Over the 13-h dark period, thetemperature (19°C) and RH (80%) remainedconstant.

Manipulation of CAM

Previous studies on K. daigremontiana have indicated that exposure of the plants to CO₂-free air still permits the accumulationof malate (up to 25% of that observed in controls) through refixationof respiratory CO₂ by PEPc (A. Borland, unpublished data). Thus,in order to completely inhibit PEP carboxylation at night, individualleaves of intact plants were enclosed in an atmosphere of N₂ overnight,as described by Borland and Griffiths (1997), thereby preventingaccess to external CO₂ and inhibiting the release of internal(respiratory) sources of CO₂ (full N₂). Some leaves were enclosedin an atmosphere of N₂ for the first half of the dark period (until2 PM) and then exposed to ambient air for the remainder (halfN₂). Control leaves were exposed to the ambient atmosphere inthe growthchamber.

A set of plants, half of which were maintained in ambient air (control), and half with leaves enclosed in an atmosphere ofN₂ (half N₂), was subjected to an increase in temperature from19°C to 27°C in the middle of the dark period (2:30-3 AM). Theleaves enclosed in N₂ were subsequently exposed to ambient airfrom 3 AM onward, with the temperature maintained at 27°C andthe RH at 70%.

Gas Exchange Measurements

Rates of net CO₂ assimilation were measured continuously on the same leaf over 24 h. The leaf was enclosed in a porometerhead that tracked the environmental conditions in the growth chamberwith gas exchange parameters measured using an open infrared (IR)gas exchange system (H. Walz, GmbH Effeltrich, Germany) with agas analyzer (Binos, H. Walz). Gas exchange parameters were calculatedusing DIAGAS software supplied by H. Walz. Each gas exchange curvepresented is for a representative leaf from three replicatedeterminations.

Malate Content

Discs were punched from three replicate leaves, subjected to the various treatments at intervals over the dark and light periods,and immediately plunged into hot (80°C) methanol (80%, v/v). Themethanolic extracts were heated for 1 h at 70°C before being evaporatedto dryness, taken up in 100 mM N,N'-bis(2-hydroxyethylglycine)(Bicine), pH 7.8, and the malate content determined enzymaticallyusing malate dehydrogenase, as described by Hohorst (1965).

PEPc and PEPc Kinase Assays

Leaf extracts were prepared and desalted as described by Hartwell et al. (1996). The activity of PEPc was assayed and itsapparent K_i for L-malate estimated as described by Nimmo et al.(1984). PEPc kinase activity in desalted extracts was assayedaccording to the method of Carter et al. (1991) using purifieddephosphorylated PEPc from Kalanchoë fedtschenkoi as the substrate.Incubations were for 30 min at 30°C.

Assay of PEPc-Kinase-Translatable mRNA

Following the method of Hartwell et al. (1996), RNA was isolated and translated in vitro using a rabbit reticulocyte lysate,and a sample of the translation products was assayed for PEPckinase activity. The PEPc was isolated by immunoprecipitation,resolved by SDS gel electrophoresis, and the incorporation of³²P into PEPc was quantified by phosphor imaging. These values werecorrected to take into account any differences in the efficiencyof translation between the different samples, as estimated bythe incorporation of [³⁵S]Met into protein (Hartwell et al., 1996). The values are thereforeequivalent to data from northern blot analysis corrected for RNAloading. Control experiments in which [ $gamma$ -³²P]ATP was omitted from the kinase assays showed that when K. daigremontianaRNA was used, small amounts of [³⁵S]Met were incorporated into immunoprecipitated PEPc from de novosynthesis of PEPc during the translations. This incorporationwas less than the amount of ³²P incorporated into PEPc in controls using the products of translationswith no added RNA. The background incorporation of ³²P was as a result of trace contamination of the PEPc substratewith PEPc kinase. However, this was <4% of the maximum labelingobtained with samples containing RNA. All experiments were repeatedat least twice, with similar results, and the data presented arefrom representative individualexperiments.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Physiology of CAM and Manipulation by N₂

Figure 1A illustrates how the dark/light pattern of net CO₂ uptake, which may be dissected into four phases (Osmond, 1978),was modulated in response to anaerobic conditions that were imposedfor part or all of the dark period. Inhibiting CO₂ uptake overthe first half of the 13-h dark period by enclosing leaves inan atmosphere of N₂ for 7.5 h resulted in a substantial increasein rates of net CO₂ assimilation when darkened leaves were removedfrom N₂ and transferred to ambient air (half N₂) compared withcontrol plants exposed to ambient air throughout the night. Themalate content of the half-N₂-treated leaves increased rapidlywhen darkened leaves were transferred to ambient air (Fig. 1B).After only 3 h in ambient air, the malate content of half N₂ leaveswas somewhat higher than that in control leaves that had accumulatedmalate over 9 h. At the end of the dark period, the malate contentof the half-N₂ leaves was about 25% higher than that measuredin control leaves.

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Figure 1. Rates of net CO₂ uptake and malate content in leaves exposed to anaerobic conditions for part or all of the dark period. A, Leaves were enclosed in an atmosphere of N₂ for the first half (half N₂) or entire duration (full N₂) of the 13-h dark period before transfer to ambient air. Rates of net CO₂ assimilation were measured. Control leaves were exposed to the ambient atmosphere in the growth chamber. Each gas exchange curve is representative of three replicate runs with SE <10%. B, Malate content was measured in leaves subjected to the above treatments with each point being the mean of three replicates with SE <10%.

, Control leaves; $open circle$ , full-N₂ leaves; $black-square$ , half-N₂ leaves. The solid bar on the x axis represents the period of darkness.

At the start of the 11-h photoperiod, leaves that had been exposed to N₂ for the first half of the dark period (half N₂) showeda small increase in the magnitude and duration of phase II netCO₂ uptake compared with control plants (Fig. 1A). However, inleaves that had been enclosed in an atmosphere of N₂ for the entireduration of the dark period (full N₂), transfer to ambient airat the start of the photoperiod resulted in a substantial increasein the rates of net CO₂ assimilation over both control and half-N₂leaves during phase II. Stomatal closure was delayed by about2 h compared with controls, as judged by the time at which netCO₂ assimilation fell to zero (Fig. 1A). Moreover, after transferto ambient air at the start of the photoperiod, the full-N₂ leavesaccumulated about 60 mmol m² malate over the first 2.5 h of the photoperiod. Thus, in theseleaves PEPc was still active at a period during which net breakdownof malate occurred in control and half-N₂ leaves (Fig. 1B). Despitethis accumulation of malate in full-N₂ leaves during the photoperiod,the malate content attained only about 50% of that measured incontrol leaves, and the majority of decarboxylation was accomplishedwithin 2 h. Consequently, during phase III, stomata remained closedfor only 2 h in full-N₂ leaves compared with 5 h in control leaves(Fig. 1A).

PEPc Kinase Activity, Translatable mRNA, and Manipulation by N₂

Figure 2 shows the changes in PEPc kinase activity and the level of translatable mRNA for the kinase in control and full-N₂leaves throughout the dark period. In control leaves, PEPc kinaseactivity increased over the first part of the dark period, reachinga plateau after 9.5 h in darkness (Fig. 2A). For leaves maintainedin N₂ during the entire dark period (in which malate content remainedlow; Fig. 1B), PEPc kinase activity increased steadily over thecourse of the dark period and was substantially higher than thatmeasured in control leaves at comparable stages throughout thenight. However, Figure 2B indicates that the levels of translatablePEPc kinase mRNA in control and full-N₂ leaves were similar forthe first 9.5 h of the dark period. Subsequently, levels of translatablemRNA in leaves enclosed in N₂ were higher than those measuredin control leaves.

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Figure 2. PEPc kinase activity and levels of translatable PEPc kinase mRNA under ambient and anaerobic conditions at night. Leaves were enclosed in an atmosphere of N₂ overnight to prevent malate accumulation or maintained in ambient air. Samples for PEPc kinase assays (A) and RNA isolation and measurement of PEPc kinase translatable mRNA (B) were taken simultaneously from the same leaves at intervals over the 13-h dark period. Shown are autoradiographs of the ³²P-labeled PEPc bands following SDS-PAGE. The doublet of PEPc bands is caused by the presence in a ratio of about 10:1 of two related subunits in K. fedtschenkoi PEPc, both of which are phosphorylated by PEPc kinase (Carter et al., 1991

). The relative intensity of the PEPc bands, shown below each track, was determined by phosphor imaging. The total incorporation of [³⁵S]Met into in vitro translation products using RNA isolated from control and N₂-treated leaves was similar (data not shown). The results are from duplicate experiments

The time course of changes in PEPc kinase activity and translatable mRNA (Fig. 2), together with changes in the apparent K_iof PEPc for malate for control and full-N₂ leaves, are illustratedin Figure 3. Changes in the apparent K_i for malate reflect thephosphorylation state of PEPc (Carter et al., 1991). In K. daigremontiana,the apparent K_i in control leaves increased from 0.5 to 5.0 mMduring the night, compared with the range of 0.3 to 3.0 mM seenwith K. fedtschenkoi in earlier work (Nimmo et al., 1984). However,the apparent K_i in full-N₂ leaves reached 8 mM, implying thatthe enzyme was not fully phosphorylated in control leaves. Thechanges in apparent K_i closely followed changes in PEPc kinaseactivity. The increase in the apparent K_i measured in leaves enclosedin N₂ compared with controls was reflected by an increased PEPckinase activity in the full-N₂ leaves. In control leaves, thelevels of kinase-translatable mRNA reached a plateau at 2 AM,whereas kinase activity and apparent K_i achieved maximum values2 h later. In full-N₂ leaves, a peak in kinase mRNA levels occurredat 6 AM. The levels of mRNA were substantially higher than thosemeasured in control leaves at this time. In both control and fullN₂ leaves, levels of translatable mRNA declined over the lastpart of the dark period.

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Figure 3. Apparent K_i of PEPc for L-malate, PEPc kinase activity, and translatable kinase mRNA under ambient and anaerobic conditions at night. Control leaves (

) were kept in ambient air throughout. Full-N₂ leaves ( $open circle$ ) were enclosed in an atmosphere of N₂ overnight to prevent malate accumulation. Half-N₂ leaves ( $black-square$ ) were enclosed in an atmosphere of N₂ to prevent malate accumulation for the first half of the dark period before transfer to ambient air. Samples for PEPc and PEPc kinase assays and RNA isolation were taken simultaneously from the same leaves at intervals over the dark period. Kinase activity and translatable mRNA values are expressed as percentages of the maximum reached during the 13-h dark period. The results are from duplicate experiments.

Figure 3 also illustrates changes in apparent K_i for malate, PEPc kinase activity, and levels of translatable mRNA that occurredwhen leaves exposed to N₂ for the first half of the dark periodwere subsequently transferred to ambient air for the remainderof the night. In these leaves, following transfer to ambient air,the apparent K_i for malate and PEPc kinase activity were appreciablyhigher than in the controls. In the 2 h following transfer ofthe half-N₂ leaves to ambient air, rates of net CO₂ uptake reacheda maximum (Fig. 1A). Over this period, the level of kinase mRNAin the half-N₂ leaves rose significantly. By 6 AM, when malatecontent peaked (Fig. 1B), kinase mRNA had dropped to a level comparableto that measured in control leaves. The peak in kinase mRNA at4 AM preceded the time when maximum PEPc kinase activity was reachedin half-N₂ leaves at 6 AM. There was little change in apparentK_i over thisperiod.

Figure 4 compares the changes that occurred at the start of the photoperiod in control leaves with those in leaves maintainedin N₂ throughout the dark period (full N₂) but transferred toambient air at the start of the photoperiod. In control leaves,the rapid down-regulation of PEPc activity was shown by a decreasein the apparent K_i of PEPc for L-malate and by the low level ofPEPc kinase activity over the 1st h of the photoperiod as ratesof net CO₂ assimilation fell to zero and malate was broken down(Fig. 1). In the same leaves, the low levels of kinase mRNA detectedat the start of the photoperiod declined to essentially zero after100 min in the light. In contrast, the apparent K_i for malate,PEPc kinase activity, and kinase mRNA at the start of the photoperiodwere substantially higher in leaves previously exposed to N₂ overnightthan in control leaves, and remained high well into the photoperiodas net CO₂ uptake continued and malate was accumulated (Fig. 1).

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Figure 4. Changes in the apparent K_i for L-malate, PEPc kinase activity, and translatable kinase mRNA at the start of the photoperiod after a night in ambient or anaerobic conditions. Leaves that had been maintained in an atmosphere of N₂ overnight to prevent malate accumulation were transferred to ambient air at the start of the photoperiod ( $open circle$ ). Control leaves were maintained in ambient air (

). Samples for PEPc and PEPc kinase assays and RNA isolation were taken simultaneously from the same leaves at intervals over the light period. Kinase activity and translatable mRNA values are expressed as percentages of the maximum reached during the photoperiod. The results are from duplicate experiments.

Physiological Aspects of Temperature Manipulations

It has been suggested that the disruption of the circadian oscillations of CO₂ exchange in CAM plants by high temperaturemay be a consequence of increased efflux of malate from the vacuoleto the cytosol, the site of PEPc activity (Wilkins, 1983; Gramset al., 1997). Figure 5 illustrates the physiological consequencesof exposing either control leaves or leaves prevented from accumulatingmalate over the first half of the dark period (half N₂) to an8°C increase in temperature in the middle of the night (from 2:30-3AM). In control leaves there was a rapid decline in the rate ofnet CO₂ assimilation as the temperature was increased from 19°Cto 27°C (Fig. 5A). The sharp increase in malate content over the30-min rise in temperature (Fig. 5B) may be attributed to an increasein refixation of respiratory CO₂ by PEPc. Overall, the maximumnet assimilation rate at 27°C was <50% of that measured at 19°Cin control leaves. Despite the continued net uptake of CO₂, themalate content of the control leaves dropped slightly over thefirst few hours of exposure to the higher temperature, suggestingconsumption of malate through increased rates of mitochondrialrespiration. However, marked breakdown of malate was observedover the last hour of the dark period, when net CO₂ assimilationhad virtually ceased. Rates of net CO₂ assimilation in leavesremoved from N₂ immediately after the temperature had been increasedto 27°C were approximately 5-fold higher than those measured incontrol leaves. However, net assimilation rates dropped sharplyduring the first 1.5 h at the higher temperature in N₂-treatedleaves, reached a plateau for 3 h, and then decreased over thelast hour of the dark period. Malate content in the N₂-treatedleaves showed a marked increase over the first 2 h at the highertemperature and a more gradual increase over the remaining 3.5h. In contrast to control leaves, the net breakdown of malatein N₂-treated leaves did not commence until the start of the photoperiod(data not shown).

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Figure 5. Modulation of net CO₂ assimilation rates and malate accumulation by a temperature increase at night. Control leaves (

) were exposed to ambient air. Half-N₂ leaves ( $open circle$ ) were enclosed in an atmosphere of N₂ for the first half of the dark period to prevent malate accumulation. Leaves were subjected to an 8°C rise in temperature from 2:30 to 3 AM. The half-N₂ leaves were subsequently exposed to ambient air at 27°C for the duration of the dark period. A, Rates of net CO₂ uptake by leaves under the two treatments with each gas exchange curve representative of three replicate runs with SE <10%. B, Malate content was measured in leaves subjected to the above treatments, with each point the mean of three replicates with SE <10%. The solid bar on the x axis represents the period of darkness.

Modulation of PEPc Kinase Activity and Translatable mRNA by Temperature

Figure 6 indicates that an 8°C rise in temperature over 30 min resulted in a decrease in PEPc kinase activity and kinase-translatablemRNA and a slight decrease in apparent K_i in control leaves. Theseparameters continued to fall over the following 70 min at 27°C.In contrast, in leaves prevented from accumulating malate overthe first half of the dark period, an 8°C rise in temperatureover 30 min resulted in an increase in apparent K_i, PEPc kinaseactivity, and kinase-translatable mRNA. However, transfer of theN₂-treated leaves to ambient air after the temperature rise resultedin a marked decrease in translatable PEPc kinase mRNA, kinaseactivity, and the apparent K_i for L-malate over 70 min at thehigher temperature as malate accumulated, presumably in the cytosol.Additional experiments in which the levels of PEPc kinase mRNAwere measured at more frequent intervals after the temperatureincrease confirmed a steady decline in the levels of mRNA from3 until 4:10 AM (data not shown). From 4:10 until 7 AM, the levelsof kinase mRNA in half-N₂ leaves were maintained at 20% of maximum.This was mirrored by a maintenance of PEPc kinase activity andby the plateau in net CO₂ assimilation in half-N₂ leaves (Fig.5A). For the latter part of the dark period, the apparent K_i forL-malate and the levels of kinase activity and mRNA were somewhathigher in N₂-treated leaves, in which the malate content was lowbut rising compared with controls, in which the malate contentwas high but declining (Fig. 5B).

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Figure 6. Modulation of the apparent K_i for L-malate, PEPc kinase activity, and translatable kinase mRNA by an increase in temperature at night. Control leaves (

) were exposed to ambient air. Half-N₂ leaves ( $open circle$ ) were enclosed in an atmosphere of N₂ for the first half of the dark period to prevent malate accumulation. All leaves were subjected to an 8°C rise in temperature from 2:30 to 3 AM. The half-N₂ leaves were subsequently exposed to ambient air at 27°C for the duration of the dark period. Samples for PEPc and PEPc kinase assays and RNA isolation were taken simultaneously from the same leaves at intervals over the dark period. Kinase activity and translatable mRNA values are expressed as percentages of the maximum reached in leaves during a normal dark period at 19°C. The results are from duplicate experiments.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

In this work we have manipulated intact plants to affect the magnitude of dark CO₂ uptake and malate accumulation, and monitoredthe effects of these manipulations on the levels of PEPc kinasemRNA and activity. The results allow a number of conclusions aboutthe control of PEPc kinase to be drawn. First, the data clearlydemonstrate the physiological significance of PEPc phosphorylation,as shown by the close correlation between the activity in vitroof PEPc kinase, net CO₂ uptake by PEPc, and malate accumulationin vivo under ambient air and after transfer from anaerobic conditionsto ambient air. For example, leaves prevented from accumulatingmalate overnight in an atmosphere of N₂ exhibited an extendedperiod of CO₂ uptake by PEPc for 2 to 3 h at the start of thephotoperiod under ambient air (Fig. 1) (Borland and Griffiths,1997). Under these conditions, kinase activity remained detectableand PEPc remained phosphorylated (as judged by its malate sensitivity)for several hours into the photoperiod (Fig. 4). In leaves movedfrom N₂ to ambient air midway through the dark period, malateaccumulated significantly faster, PEPc kinase activity was higher,and PEPc was more highly phosphorylated than in control leaves.(Figs. 1 and 3). The data presented here support and extend thoseof Hartwell et al. (1996) on B. (K.) fedtschenkoi in showing thatthese physiologically significant changes in PEPc kinase activityreflect changes in the translatable mRNA for this protein. Moreover,recent work using northern analysis with a PEPc kinase cDNA hasshown that there are very similar changes in the level of PEPckinase transcripts (J. Hartwell, A.M. Borland, G.I. Jenkins, andH.G. Nimmo, unpublisheddata).

Previous work has demonstrated clearly that PEPc kinase mRNA and activity and the phosphorylation state of PEPc are undercircadian control (Nimmo et al., 1987; Carter et al., 1991; Hartwellet al., 1996). These effects contribute to the well-establishedcircadian control of CO₂ fixation in CAM plants (e.g. Wilkins,1992). The influence of a circadian oscillator, rather than light/darkcontrol, is illustrated by the fact that in K. fedtschenkoi inan 8-h photoperiod, both the increase and decrease in PEPc kinasemRNA and activity occur during the dark period (Hartwell et al.,1996). In the present work using K. daigremontiana in an 11-hphotoperiod, the increase in PEPc kinase mRNA and activity alsooccured during the dark period (Figs. 2 and 3). The decline inPEPc kinase mRNA commences during the dark period, but the declinein kinase activity occurs only at the start of the lightperiod.

The data in this paper allow a further conclusion to be drawn about the control of PEPc kinase. The circadian control of kinasemRNA and activity can be influenced by metabolic status, specificallyby treatments that affect the content or compartmentation of malate.For example, in leaves that cannot accumulate malate, PEPc kinaseactivity is significantly higher than in control leaves, eventhough PEPc kinase mRNA levels are similar (Figs. 2 and 3). Althoughsubjecting leaves to an anaerobic environment under N₂ could initself affect mRNA abundance, the data shown here present a numberof testable hypotheses. Thus, in leaves with a high malate content,translation of PEPc kinase mRNA is reduced, the rate of inactivation(possibly by turnover) of PEPc kinase is increased, or both. Themechanisms(s) responsible could involve sensing of malate itselfor of another metabolite the level of which correlates with thetotal leaf malatecontent.

Another effect of the prevention of malate accumulation was observed in experiments in which the temperature was increasedfrom 19°C to 27°C in the middle of the dark period. In controlleaves, this increase in temperature was accompanied by a reductionin the level of PEPc kinase mRNA. In contrast, in leaves in whichmalate accumulation had been prevented, there was a marked increasein kinase mRNA as temperature increased (Fig. 6). Experimentsconducted with K. fedschenkoi have indicated that low temperature(i.e. 4°C) stabilizes the levels of kinase mRNA and postponesde-phosphorylation (Hartwell et al., 1996).

The effect of increased temperature on circadian rhythms of CO₂ fixation has been ascribed to increased permeability of thetonoplast to malate and efflux of malate to the cytoplasm (Wilkins,1983, 1992). There is direct experimental support for this hypothesis(Friemert et al., 1988). One possible explanation of our datais that PEPc-kinase-translatable mRNA is negatively regulatedby cytosolic malate. However, it must be emphasized that no directmeasurements of cytosolic malate have been made in CAM plants,and we have not been able to ascertain whether the temperatureincrease reduced PEPc-kinase-translatable mRNA through an increasein total malate (Fig. 5B), an increase in cytosolic malate, alowering of cytosolic pH, or a change in another metabolite. Eithertranscription of the PEPc kinase gene or the stability of thekinase mRNA could be affected. Presumably, the relevant metabolitelevel in control leaves was insufficient to reduce the accumulationof PEPc kinase mRNA observed during the first 10 h of darkness(Fig. 3). PEPc kinase mRNA started to decline later in controlleaves than in half-N₂ leaves (6 and 4 AM, respectively) (Fig.3). Because the total leaf malate contents were actually similarat these times in the two treatments (Fig. 1B), there may be athreshold level of total malate in the dark (at about 120 mmolm²) above which malate is sufficient to reduce PEPc kinase mRNA.However, PEPc kinase mRNA starts to decline after 6 AM, even inleaves treated with full N₂ and unable to accumulate malate (Fig.3), so at least part of the decline at this time may reflect circadiancontrol.

Overall, the control of flux through PEPc is multilayered. Fine control is achieved by changes in cytosolic levels of pH andopposing metabolic effectors such as malate (negative) and Glc6-P (positive), whereas the phosphorylation of PEPc representsa means for coarse control of flux through this enzyme. The timingof phosphorylation is set by a circadian oscillator. The datain this paper show that circadian control can be overridden bymetabolite control, probably in various ways. Our data are consistentwith the view that metabolites can affect PEPc kinase gene expressionor mRNA stability, and perhaps the stability of the kinase itself.Such metabolite effects may influence entrainment of the circadianrhythm to environmental conditions that support photosyntheticplasticity and survival through temporarily optimizing CO₂ uptake.Identification of the factors responsible will require measurementof the amount and distribution of a number of key metabolites,includingmalate.

	ACKNOWLEDGMENT

A.M.B. is grateful to Professor H. Griffiths (Department of Agricultural and Environmental Sciences, University of Newcastle)for his continued interest in thiswork.

	FOOTNOTES

Received April 19, 1999; accepted August 2, 1999.

¹ Financial support was provided by the Natural Environment Research Council and the Biological and Biotechnological ScienceResearch Council, UnitedKingdom.

^* Corresponding author; e-mail a.m.borland{at}ncl.ac.uk; fax 191-222-5228.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

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Metabolite Control Overrides Circadian Regulation of Phosphoenolpyruvate Carboxylase Kinase and CO2 Fixation in Crassulacean Acid Metabolism1

Metabolite Control Overrides Circadian Regulation of Phosphoenolpyruvate Carboxylase Kinase and CO₂ Fixation in Crassulacean Acid Metabolism¹