Ascorbate Biosynthesis in Mitochondria Is Linked to the Electron Transport Chain between Complexes III and IV

doi:10.1104/pp.123.1.335

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Ascorbate Biosynthesis in Mitochondria Is Linked to the Electron Transport Chain between Complexes III and IV¹

Carlos G. Bartoli, Gabriela M. Pastori,^* and Christine H. Foyer

Instituto de Fisiología Vegetal, Facultad de Ciencias Agropecuarias, Universidad Nacional de La Plata, Casilla de Correos 327, (1900) La Plata, Argentina (C.G.B.); and Biochemistry and Physiology Department, IACR-Rothamsted Experimental Station, Harpenden, Herts AL5 2JQ, United Kingdom (G.M.P., C.H.F.)

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

Ascorbic acid is synthesized from galactono- $gamma$ -lactone (GL) in plant tissues. An improved extraction procedure involving ammoniumsulfate precipitation of membrane proteins from crude leaf homogenatesyielded a simple, quick method for determining tissue activitiesof galactono- $gamma$ -lactone dehydrogenase (GLDH). Total foliar ascorbateand GLDH activity decreased with leaf age. Subcellular fractionationexperiments using marker enzymes demonstrated that 80% of thetotal GLDH activity was located on the inner mitochondrial membrane,and 20% in the microsomal fraction. Specific antibody raised againstpotato (Solanum tuberosum L.) tuber GLDH recognized a 56-kD polypeptidein extracts from the mitochondrial membranes but failed to detectthe equivalent polypeptide in microsomes. We demonstrate thatisolated intact mitochondria synthesize ascorbate in the presenceof GL. GL stimulated mitochondrial electron transport rates. Therespiration inhibitor antimycin A stimulated ascorbate biosynthesis,while cyanide inhibited both respiration and ascorbate production.GL-dependent oxygen uptake was observed in isolated intact mitochondria.This evidence suggests that GLDH delivers electrons to the mitochondrialelectron transport chain between complexes III andIV.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Ascorbic acid is an abundant antioxidant in plant tissues that is found in millimolar concentrations in leaves and storageorgans (for review, see Smirnoff 1996; Noctor and Foyer, 1998).It reacts directly with O₂^·, ·OH, and ¹O₂ (Buettner and Jurkiewicz, 1996), recycles the lipid-soluble $alpha$ -tocopherol by reduction of its oxidized form (Sharma and Buettner,1993), and is essential for the protection of enzymes with prosthetictransition metal ions (Padh, 1990). It is involved in the regulationof the fundamental cellular processes of photoprotection and regulationof photosynthesis (Foyer and Harbinson, 1994), root elongation,cell vacuolarization, and cell expansion (for review, see Smirnoff,1996). Ascorbic acid is also involved in the cell cycle (Kerkand Feldman, 1995) and in other important enzyme reactions inplant tissues (i.e. ethylenebiosynthesis).

The pathway of ascorbate biosynthesis in plants is different from that in animals. It has remained unresolved until recently,when convincing evidence in support of a novel putative pathwaywas presented (Wheeler et al., 1998). Although many steps remainto be completely elucidated, the last step in the pathway involvesthe conversion of L-galactono- $gamma$ -lactone (GL) to ascorbic acid,a reaction catalyzed by the membrane-bound enzyme L-galactono- $gamma$ -lactonedehydrogenase (GLDH) (Ostergaard et al., 1997). GLDH, with a molecularmass of 56 kD, is highly specific for GL and requires cytochromec (Cyt c) as a second substrate that is reduced as GL is convertedto ascorbic acid (Ôba et al., 1995; Ostergaard et al., 1997;Imai et al., 1998). GL is synthesized from L-Gal by a novel enzyme,L-Gal dehydrogenase (Wheeler et al., 1998), and is rapidly convertedto ascorbic acid when applied to different plant tissues (Conklinet al., 1996; Arrigoni et al., 1997). The ascorbate pool in leavesrepresents over 10% of the soluble carbohydrates (Noctor and Foyer,1998), and concentrations of 20 to 50 mM have been found in spinachchloroplasts and cytosol (Foyer et al., 1983). Even when ascorbicacid is present at high concentrations, there are no data on theconcentration of GL in plant tissues, and the integration of ascorbatesynthesis, regeneration, and degradation is still not completelyresolved.

The requirement of mitochondria for the biosynthesis of ascorbic acid from GL was reported in early studies (Mapson and Breslow,1958). By Suc-density gradient fractionation, GLDH activity waslocalized in mitochondria of white potato (Solanum tuberosum L.)tubers and spinach leaves (Ôba et al., 1994; Mut-suda et al.,1995). Mitochondria from fava bean embryos and maize seedlingswere used as a source of GLDH for studies on the in vivo conversionof GL into ascorbic acid (Arrigoni et al., 1997; De Gara et al.,1997). Very recently, the presence of GLDH on the mitochondrialinner membrane from kidney bean hypocotyls has been reported (Siendoneset al., 1999). Although GLDH activity was also found in microsomesfrom potato tubers (Ôba et al., 1994), no fur-ther studies havebeen carried out to establish unequivocally the localization ofthis enzyme in other subcellularcompartments.

An accurate assay of GLDH activity in crude homogenates has not been reported until now because of the specificity of thisenzyme for Cyt c as an electron acceptor and the high interferenceof competing reactions. The use of mitochondrial preparationsis therefore a prerequisite for the measurement of GLDH activity,precluding experiments that require a rapid extraction of planttissues. The present study describes a new method for the quick,reproducible measurement of GLDH activity in crude leaf homogenates.We demonstrate that isolated intact mitochondria synthesize ascorbatein the presence of the precursor GL. The localization of GLDHon the inner mitochondrial membrane and its specificity for Cytc as an electron acceptor are confirmed. The localization of GLDHactivity in potato leaf microsomes and the involvement of GLDHin mitochondrial electron transport are alsodiscussed.

	RESULTS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

At the outset of this study it was clear that an improved extraction method for the assay of GLDH activity in leaf homogenateswas needed. By precipitation of crude leaf homogenates with 20%(w/v) (NH₄)₂SO₄, two fractions, designated as membrane-bound andsoluble proteins, were obtained (Table I). GLDH activity wasfound to be associated mostly with the membrane-enriched fractionand had a distribution similar to that of NADPH-Cyt c reductase,which is used as a membrane-bound protein marker. This simple,rapid step allows full recovery of GLDH activity and allows easyanalysis of GLDH activity in plant tissues.

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Table I. GLDH and NADPH-CCR activities in potato leaf extracts after precipitation of protein membranes with 20% (NH₄)₂SO₄
Values in parentheses are the percentage of enzyme activities. Values are means of three different experiments ± SD.

The relationship between GLDH and ascorbate content was studied in young, mature, and senescent potato leaves (Table II).Total foliar ascorbate concentration decreased dramatically withleaf age, being lowest in senescent leaves. The ascorbate/dehydroascorbateratio also decreased significantly in senescent leaves. GLDH activitywas highest in young leaves and decreased with age, being lowestin senescent leaves. Furthermore, when potato leaves from eachleaf age were incubated in saturating (50 mM) GL for 3 h, GLDHactivity was lower in mature and senescent leaves than in youngleaves.

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Table II. Biosynthesis of ascorbate in potato leaves at different stages of development
Indirect GLDH activity is measured as the difference in ascorbate content in whole leaves after incubation in 50 mM GL for 3 h. Values in parentheses indicate the percentage of DHA. Values represent the mean of three different experiments ± SD.

Subcellular fractionation of potato leaves yielded intact chloroplasts, microsomal and cytosolic fractions, as well as a fractionenriched in intact mitochondria and peroxisomes. These were characterizedby the distribution of enzyme marker activities and chlorophyllcontents (Table III). GLDH activity was mainly associated withthe mitochondrial- and peroxisomal-enriched fraction, althoughover 20% of the enzyme activity was found in microsomes. The purityof the microsomal fraction was estimated by measuring NADPH-Cytc reductase and Cyt c oxidase activities as microsomal and mitochondrialmarkers, respectively. Although there was a low contaminationof microsomes by mitochondria, the rest of the GLDH activity wasassociated with the microsomal fraction. The GLDH activity foundin chloroplasts and in cytosol was of the same order as the levelof contamination. Therefore, GLDH was not present in these fractions(Table III).

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Table III. Distribution of GLDH activity in subcellular fractions of potato leaves
Values between parentheses indicate a percentage of enzyme activities. Values are means of three different experiments ± SD.

Mitochondria and peroxisomes were separated in Percoll-density gradients, and the purity of each fraction was determined bymeasuring Cyt c oxidase and hydroxypyruvate reductase activitiesas marker enzymes of mitochondria and peroxisomes, respectively(Table IV). GLDH activity was found in mitochondria; the activityin peroxisomes was attributed to mitochondrial contamination.

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Table IV. Distribution of GLDH activity in intact mitochondria and peroxisomes from potato leaves
Values are means of three different experiments ± SD. nd, Non-detected.

The localization of GLDH was further studied by comparing the latency of the enzyme together with the enzyme markers Cyt coxidase and malate dehydrogenase (Table V). In intact mitochondria,GLDH and Cyt c oxidase activities were barely detectable and theirlatencies were over 85%, reflecting the high yield of intact organellesisolated by Percoll-density gradient. After disruption of theintact mitochondria with 0.15% (w/v) Triton X-100, GLDH and Cytc oxidase latencies decreased to a similar extent, while malatedehydrogenase activity remained high, suggesting that GLDH localizationis similar to Cyt c oxidase (Table V).

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Table V. Latency of GLDH, CCO, and MDH in mitochondria from potato leaves
Enzyme latencies are expressed as a percentage and calculated as described in "Materials and Methods." HT, Mitochondria after swelling in hypotonic medium. Values are means of three different experiments ± SD.

Inner- and outer-membrane enriched fractions were prepared from intact leaf mitochondria, and Cyt c oxidase and antimycinA-resistant Cyt c reductase activities were used as inner andouter mitochondrial membrane markers, respectively (Table VI).By measuring GLDH/Cyt c oxidase and GLDH/antimycin A-resistantCyt c reductase activity ratios, GLDH was found to be largelyassociated with the inner-membrane-enriched fraction.

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Table VI. GLDH activity in mitochondrial inner- and outer-membrane enriched fractions from potato leaves
Cyt c oxidase (CCO) and antimycin A-resistant Cyt c reductase (A-CCR) were used as inner and outer membrane markers, respectively. Values are means of three different experiments ± SD.

The localization of the GLDH protein was also determined by western-blot analysis using a specific antibody against GLDH frompotato (Fig. 1). A polypeptide of 56 kD was detected only in themitochondrial fraction with this antibody (Fig. 1A). AlthoughGLDH activity was detected in microsomes, the antibody did notrecognize polypeptides in this fraction. Similarly, the antibodydid not detect polypeptides in chloroplasts, peroxisomes, or cytosol.Western analysis of mitochondrial inner- and outer-membrane-enrichedfractions revealed that GLDH is localized in the mitochondrialinner membrane (Fig. 1B). The antibody detected proteins withmolecular masses of 56, 30, 28, and 26 kD.

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Figure 1. Western blot of GLDH in potato leaf subcellular fractions (A) and mitochondrial inner- and outer-membrane-enriched fractions (B). Fifty micrograms of protein was loaded onto 12% (w/v) denaturing acrylamide gels, transferred to nitrocellulose membranes, and blotted against a specific antibody against GLDH from potato. Px, Peroxisomes; Mit, mitochondria; Mic, microsomes; Cyt, cytosol; Chl, chloroplasts; OM, mitochondrial outer-membrane-enriched fraction; IM, mitochondrial inner-membrane-enriched fraction.

The predicted GLDH transmembrane regions and orientation in the inner mitochondrial membrane are shown in Figure 2. The analysispredicted three spanning membrane regions and a FAD-binding domainon the outside of the inside membrane. This suggests that thecatalytic site of GLDH faces the outside of the inner mitochondrialmembrane. Analysis of absorption spectra suggested the presenceof a flavin prosthetic group associated with purified sweet potatoGLDH (Imai et al., 1998). The amino acid sequence of polypeptidesgenerated after partial digestion with V8-protease predicts asimilar binding domain.

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Figure 2. Predicted inner mitochondrial membrane-spanning region of GLDH. GLDH transmembrane regions and orientation were predicted using the Tmpred program. A, GLDH protein sequence from sweet potato (Imai et al., 1998

). Areas included in boxes are membrane-spanning regions, while those underlined are peptides generated after digestion with a V8 protease. The Leu at position 137 indicates the normal position for the FAD-binding domain, and is located on the outside of the inner mitochondrial membrane. B, Predicted inner mitochondrial membrane-spanning region of GLDH.

The localization of GLDH in the mitochondrial inner membrane and its specificity for Cyt c suggested the possible involvementof GLDH in the mitochondrial respiratory electron transport chain.To explore this possibility, respiration rates and ascorbate productionwere estimated in intact mitochondria isolated from potato tubers(Table VII). Potato tubers were selected for these assays becausethey could be isolated in large numbers, are free of chlorophylls,and contain a similar pattern of localization of GLDH to potatoleaves (data not shown). Respiration rates in the presence ofADP and NADH were high, but they were increased over 20% when5 mM GL was present in the respiration medium. While the productionof ascorbate by intact mitochondria was undetectable in controlconditions, the presence of GL in the medium provoked a markedincrease in ascorbate production, indicating that isolated mitochondriaare able to synthesize ascorbate at a high rate through GLDH activity(Table VII).

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Table VII. Effect of GL and mitochondrial respiratory chain inhibitors on respiration rate and ascorbate production in isolated mitochondria from white potato tubers
Respiration was measured after incubation of intact mitochondria in buffer containing 5 mM GL and 5 µg/mL antimycin A or 1 mM KCN for 90 min. Values represent the mean of three different experiments ± SD. nd, Non-detected.

The respiratory inhibitors antimycin A and KCN provoked a decrease of respiration in the absence or presence of GL. However,ascorbate production was stimulated by antimycin A, an inhibitorof Cyt c reductase at the level of complex III. Rotenone, an inhibitorof complex I, did not decrease ascorbate production, althoughthe presence of other NADH dehydrogenases resistant to rotenoneresulted in only a partial inhibition of mitochondrial respiration(data not shown). In contrast, KCN, a potent inhibitor of Cytc oxidase in complex IV, provoked complete inhibition of ascorbatesynthesis. The inhibition of ascorbate production by KCN was notdue to a decrease of GLDH activity, since KCN did not inhibitthis enzyme in the in vitro assay (data notshown).

To confirm that GL is an electron donor to the mitochondrial respiration, oxygen uptake was measured in intact mitochondriaincubated with 5 mM GL without ADP and NADH (Table VIII). In theabsence of ADP and NADH, GL provoked an approximately 35% increasein the respiration rate in all experiments.

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Table VIII. Mitochondrial respiration in the presence of GL as the only source of electrons in isolated mitochondria from white potato tubers
Respiration was measured in intact mitochondria in the presence of 5 mM GL. Respiratory control = 2.15. Values represent the mean of three different experiments.

	DISCUSSION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

The mitochondrial inner membrane is one of the most complex biological membranes. It is a highly specialized system for oxidativephosphorylation and energy-linked ion translocation (Douce, 1985).Energy capture, transduction, and utilization are achieved ina number of reactions that are energetically interlinked and involveat least several hundred polypeptides. In the present study weanalyzed the function of GLDH, a protein bound to the inner mitochondrialmembrane, and its interaction with the respiratory electron transportchain. We also demonstrated that isolated intact mitochondriaproduce ascorbate, as suggested by the early studies on crudemitochondria preparations (Mapson and Breslow, 1958).

Foliar ascorbate and GLDH activity decrease with leaf age, with the lowest levels found in senescent leaves. The turnoverof ascorbate in leaves is clearly regulated by developmental triggers.The loss of GLDH activity with leaf age implies that ascorbatesynthesis is decreased as leaves mature and senesce. Similarly,the increase in the amount of oxidized ascorbate with age impliesdecreased capacity for reduction. Whether the loss of GLDH isdue to decreased transcription/translation or increased proteinturnover is unknown; however, age-dependent losses in GLDH andascorbate will render the leaf less able to combat oxidation.Therefore, senescent leaves are more susceptible to oxidativestress.

GLDH activity was found in mitochondria and microsomes isolated from potato leaves and tubers. Our results on the localizationof GLDH in mitochondria are in agreement with previous studies,such as the pioneering work of Mapson and Breslow (1958), whoreported the requirement of these organelles for the biosynthesisof ascorbate, and with Ôba et al. (1994), Mutsuda et al. (1995),and Arrigoni et al. (1997), who demonstrated the presence of GLDHin mitochondria from potato tubers, spinach leaves, bean embryos,and maize seedlings, respectively. GLDH was found to be associatedwith the mitochondrial inner membrane of kidney bean hypocotyls(Siendones et al., 1999).

The data presented in this manuscript confirm the localization of GLDH activity on the inner mitochondrial membrane and providecorroborative evidence by detection of the protein on westernblots. Bands of low M_r detected by the antibody could be productsof GLDH degradation, as reported by Imai et al. (1998). Sincethe antibody did not recognize polypeptides in the microsomes,even though 20% of the total foliar activity was localized withthis fraction, it would appear that an epitopically distinct GLDHform resides in the microsomes. The antibody did not detect polypeptidesin membranes of other subcellular compartments, confirming thatGLDH is absent from other sites in the plant cell. The naturalelectron acceptor for the microsomal GLDH form is unknown, butthe involvement of other cytochromes present in microsomal fractionssuggests that electron donation may not be limited to Cyt c. MicrosomalGLDH may use L-gulono- $gamma$ -lactone as a substrate. This would explainwhy purified GLDH is specific for GL and does not catalyze theoxidation of L-gulono- $gamma$ -lactone (Ôba et al., 1995), while intacttissues can oxidize GL and L-gulono- $gamma$ -lactone. This was demonstratedin Arabidopsis cell suspension cultures incubated with a rangeof potential biosynthetic precursors of ascorbic acid (Davey etal., 1999). It is interesting that cytosolic expression of ratliver L-gulono- $gamma$ -lactone oxidase in potato (T. Imai, A. Kingston-Smith,and C.H. Foyer, unpublished results), lettuce, and tobacco plantsresults in increased ascorbate biosynthesis (Jain and Nessler,2000). This enzyme must have access to an alternative electronacceptor, since there has been no attempt to target this enzymeto the inner mitochondrial membrane in thesestudies.

GL may diffuse through the outer mitochondrial membrane, which is highly permeable to solutes such as Suc, nucleotides, andNAD⁺, while a specific ascorbate transporter may be required for transportacross the inner membrane, which is impermeable to Suc but selectivelypermeable to a limited number of anions, depending on the orientationof GLDH. While the transport of dehydroascorbate is mediated byGlc transporters in animals, ascorbate is transported across cellularmembranes by a different mechanism, as demonstrated in Xenopuslaevis oocytes (Rumsey et al., 1997). While analogous systemshave yet to be characterized in plants, several transport systemshave been described (Horemans et al., 1999). According to thepredicted localization, GLDH spans the inner mitochondrial membrane,but no transporters would be required, since the catalytic siteof GLDH faces the intermembranespace.

Plant mitochondria are considerably more complex than animal mitochondria. Apart from producing ATP through an electron transportchain, plant mitochondria interact with chloroplasts to producea wealth of primary and secondary metabolites (some specificallyin response to stress), and participate in photorespiration (forreview, see Douce, 1985; Mackenzie and McIntosh, 1999). Respirationinvolves the transfer of electrons from organic molecules to oxygenthrough four respiratory complexes located in the inner mitochondrialmembrane (Fig. 3). Unlike animals, respiratory oxygen consumptionin plants is not completely inhibited by cyanide because of thepresence of a cyanide-resistant, alternative respiratory pathwaythat drives electrons from ubiquinone to oxygen in the inner mitochondrialmembrane, by-passing the cytochromes in complexes III and IV.Respiration via the alternative pathway only proceeds in the presenceof high concentrations of respiratory substrates (Lambers, 1982),and is up-regulated by many types of stress, including exposureto cold, pathogen attack, drought, and wounding (Mackenzie andMcIntosh, 1999). A principal function may be prevention of excessiveproduction of superoxide and hydrogen peroxide (Wagner and Moore,1997).

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Figure 3. Hypothetical model of the interaction between GLDH and the mitochondrial electron transport chain. GLDH feeds electrons into Cyt c between complexes III and IV, while GL is converted into ascorbate. The inhibition of Cyt c oxidase by KCN in complex IV blocks ascorbate production, possibly by the accumulation of electrons in Cyt c. AOX, Alternative oxidase; DH, dehydrogenase; UQ, ubiquinone.

The presence of GLDH in the inner mitochondrial membrane and its capacity to donate electrons to the mitochondrial electrontransport chain during ascorbate biosynthesis contribute to thecomplexity of plant mitochondrial respiration (Fig. 3). GL isable to function as an alternative electron donor, allowing GLDHto reduce Cyt c between complexes III and IV. GLDH is not inhibitedby KCN, but ascorbate synthesis is completely blocked when thisinhibitor is added to mitochondria. This suggests that the inhibitionof Cyt c oxidase activity by KCN inhibits ascorbate synthesisin situ due to a lack of an available electron acceptor. Therefore,intact mitochondria cannot synthesize ascorbate when the electronacceptor Cyt c is fullyreduced.

A pivotal question concerns the relative rates of flux of electron transport driven by ascorbate synthesis and that drivenby the activity of the tricarboxylic acid cycle. Since GLDH maynot be the rate-limiting step of ascorbate synthesis, the supplyof GL may frequently be limiting. However, in situations of elicitrapid ascorbate turnover, GLDH activity may be high enough toimpact on the rate ofrespiration.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Plant Material

Potato (Solanum tuberosum L. cv Solara) plants were grown for 4 weeks in a growth chamber at 20°C with a 16-h photoperiod(photosynthetic photon flux density of 300 µmol m² s¹). Plants were placed in 5-L pots containing a soil mixture. Leaveswere selected at three developmental stages: young (50% expansion);mature (full expansion); and senescent (yellowish expanded). Whitepotato tubers, obtained from a local store, were used for mitochondrialrespirationstudies.

Subcellular Fractionation

The following procedures were carried out at 4°C. Mature potato leaves were homogenized in extraction medium (30 mM 3-[N-morpholino]-propanesulfonicacid [MOPS], pH 7.5, 0.2% [w/v] bovine serum albumin [BSA], 4mM Cys, 0.35 M mannitol, 1% [w/v] PVP-40, 25 mM Na₄P₂O₇, and 2mM EDTA) at a ratio of 1 g of tissue per 5 mL of extraction medium,in a homogenizer. The homogenate was filtered through four layersof cotton cloth and centrifuged at 2,200g for 5 min to obtainthe chloroplast fraction. Chloroplasts were resuspended in 10mL of washing medium (20 mM MOPS, pH 7.2, 0.2% BSA [w/v], 0.3M mannitol, and 1 mM EDTA), and centrifuged at the same speedonce more. The first 2,200g supernatant was centrifuged at 14,000gfor 15 min to yield a fraction enriched in mitochondria and peroxisomes.This pellet was resuspended in washing medium, and centrifugedagain at 14,000g before being loaded onto a gradient consistingof a bottom layer of 15 mL of 28% (w/v) Percoll in 10 mM MOPS,pH 7.2, 0.3 M Suc, and 0.1% (w/v) BSA, and a top layer of 21 mLof the same solution with mannitol instead of Suc (Jiménez etal., 1997). After centrifugation at 41,400g for 35 min, intactmitochondria and peroxisomes were washed twice by a 10-times dilutionin washing medium and centrifugation at 17,400g for 15 min. Mitochondriafrom white potato tubers were isolated using the same method asfor leafmitochondria.

For isolation of microsomal and cytosolic fractions, the first 14,000g supernatant was centrifuged at 100,000g for 1h.

Isolation of Mitochondrial Outer and Inner Membranes

Outer- and inner-membrane-enriched fractions from potato leaf mitochondria were isolated as described by Mannella (1987).In this method, intact mitochondria are exposed to successivelygreater hypotonic shocks, which increases succinate-Cyt c oxidoreductaseand malate dehydrogenase activities as the outer and inner membranesare being disrupted, respectively. Intact mitochondria isolatedfrom potato leaves were swollen in 12 mM mannitol for 30 min,a concentration suitable to separate the outer membrane withoutdisrupting the inner membrane, and then loaded in a 0.6 to 0.9M Suc-step gradient, which was then centrifuged in a swingingbucket rotor at 40,000g for 60 min. Outer membranes were recoveredfrom the supernatant fraction between the bottom and the Suc interphase.Inner membranes and remaining intact mitochondria were collectedfrom the bottom of the tube. Both fractions were diluted at leastthree times in a 20 mM MOPS, pH 7.2, and 0.3 M mannitol, and centrifugedat 60,000g for 1.5 h. Pellets consisting of mitochondrial outer-and inner-membrane enriched fractions were resuspended in smallvolumes of the samemedium.

Ascorbate Determination

Ascorbate was measured as described by Foyer et al. (1983). Fifty milligrams of leaf tissues were homogenized in 0.5 mL of1 M HClO₄ with mortar and pestle in an ice bath and centrifugedat 13,000g for 5 min at 4°C. 0.1 M 4-(2-hydroxyethyl)-1-piperazineethanesulfonicacid (HEPES)/KOH buffer, pH 7.0, was added to the supernatantsat a ratio of 1:5 (buffer:extract), neutralized with 1 M K₂CO₃to pH 5.6, and centrifuged again as above. Ascorbate was measuredas the difference of A₂₆₅ before and after the addition of ascorbateoxidase.

Enzyme Assays

GLDH (EC 1.3.2.3) activity was assayed by the reduction of Cyt c at 550 nm ( $epsilon$ = 21 mM¹ cm¹) in a medium consisting of 50 mM Tris-HCl, pH 8.0, 60 µM Cytc, 0.15% (w/v) Triton X-100, and 25 to 50 µg of sample protein(Ostergaard et al., 1997). GLDH activity was also estimated indirectlyby incubating two leaf discs in 50 mM GL or in water as a controlfor 3 h. Indirect GLDH activity was calculated as the differencein ascorbate content between GL-treated and control leafdiscs.

Cyt c oxidase (EC 1.9.3.1) activity was measured by incubating 5 to 10 µg of protein of each sample in 30 mM MOPS, 0.3 Mmannitol, and 50 µM reduced Cyt c, and following the oxidationof Cyt c (Tolbert et al., 1968).

NADPH-Cyt c reductase (EC 1.6.2.4) activity was determined by the reduction of Cyt c in a reaction mixture containing 0.3M potassium phosphate buffer, pH 7.6, 20 µM Cyt c, 0.1 mM NADPH,and 10 to 50 µg of sample protein (Simontachi et al., 1992).

Antimycin A-resistant Cyt c reductase (EC 1.6.99.3) activity was estimated by the reduction of Cyt c in a reaction mixturecontaining 20 mM MOPS, pH 7.0, 1 mM KCN, 1 mM NADH, 1 µg/mL antimycinA, 50 µM Cyt c, and 10 to 25 µg of sample protein (Mannella, 1987).

Malate dehydrogenase (EC 1.1.1.82) activity was measured as the oxidation of NADH at 340 nm ( $epsilon$ = 6.22 mM¹ cm¹) in a medium consisting of 20 mM MOPS, pH 7.2, 1 mM oxalacetate,1 mM KCN, 0.2 mM NADH, and 10 to 50 µg of sample protein (Molleret al., 1987).

Hydroxypyruvate reductase (EC 1.1.1.29) activity was determined by the oxidation of NADH in a reaction mixture containing69 mM potassium phosphate buffer, pH 6.2, 0.2 mM NADH, 1 mM KCN,2.0 mM hydroxypyruvate, and 10 to 50 µg of sample protein (Schwitzguébeland Siegenthaler, 1984).

Enzyme Latency Determination

The enzyme latency was determined in intact mitochondria in a reaction mixture containing 0.3 M mannitol by assaying the enzymeactivities before and after the addition of 0.025% (v/v) TritonX-100. The latency was calculated with the following formula (Burgesset al., 1985):

<UP>Latency</UP>=[(<UP>Activity</UP>+<UP>Triton</UP>)<UP>−</UP>(<UP>Activity</UP>−<UP>Triton</UP>)]<UP>/</UP>(<UP>Activity</UP>+<UP>Triton</UP>)×100

Improved Extraction and Assay for GLDH Activity

An improved method for the assay of GLDH activity in potato leaf crude homogenates was devised: 10 g of potato leaves wereground in 50 mL of extraction buffer, filtered through four layersof cheesecloth, and centrifuged at 2,200g for 5 min. Twenty percent(w/v) (NH₄)₂SO₄ was added to the 2,200g supernatants, incubatedat 4°C for 30 min under continuous stirring, and centrifuged at10,000g for 20 min. The pellet containing membrane-bound proteinswas resuspended in 1 mL of washing medium without BSA. GLDH activitywas measured in the resuspended pellet after a semi-purificationstep through Sephadex G-25.

SDS-PAGE and Western Blotting

Fifty-milligram protein samples of each subcellular fraction were incubated at 95°C for 4 min in sample buffer containing62.5 mM Tris-HCl, pH 6.8, 10% (v/v) glycerol, 2% (w/v) SDS, 5%(v/v) 2- $beta$ -mercaptoethanol, and 0.0025% (w/v) bromophenol blue.Samples were loaded on a 12% (w/v) denaturing polyacrylamide geland electrophoresed at 25 mA/gel for 1.5 h. For western blotting,proteins were electrotransferred to a nitrocellulose membraneat 70 V for 1 h. Blots were blocked in 5% (w/v) non-fat dry milkdissolved in PBS (10 mM phosphate buffer, pH 7.4, 2.7 mM KCl,and 137 mM NaCl) for 2 h, and probed with a polyclonal antibodyagainst GLDH from potato tubers for 1 h. After washing the membranethree times for 10 min each with PBS-T (PBS plus 0.05% [w/v] Tween20) blots were incubated with a secondary antibody against goatanti-rabbit IgG conjugated to alkaline phosphatase for 1 h, washedwith PBS-T, and developed with a colorimetric assay consistingof 0.15 mg/mL 5-bromo-4-chloro-3-indolyl phosphate, 0.3 mg/mLnitroblue tetrazolium, 100 mM Tris-HCl buffer, pH 9.5, and 5 mMMgCl₂ (Sigma, Dorset,UK).

Ascorbate Production by Whole Leaves and Intact Mitochondria

Whole leaves were incubated in 50 mM GL for 3 h using water as a control. Intact mitochondria were incubated in the mediumused for respiration studies consisting of 20 mM MOPS, pH 8.0,0.3 M mannitol, 1 mM MgCl₂, 5 mM K₂HPO₄, 10 mM KCl, plus 2 mMGL for 15 to 90 min at room temperature. The reaction was stoppedby the addition of HClO₄, and the ascorbate content was assayedimmediately.

Measurements of Mitochondrial Respiration Rate

Respiration experiments were carried out in intact mitochondria isolated from white potato tubers for an accurate assay ofrespiratory rates without the interference of chlorophylls. Oxygenuptake was recorded with an oxygen electrode (Hansatech, King'sLynn, UK). Mitochondrial respiration was measured at pH 8.0, sincelower pHs inhibit GLDH activity. Oxygen uptake was estimated ina medium containing 20 mM MOPS, pH 8.0, 0.3 M mannitol, 1 mM MgCl₂,5 mM K₂HPO₄, and 10 mM KCl, followed by the addition of 2 mM NADHand 0.1 mM ADP. Rates of respiration in mitochondria from potatotubers were similar to those reported in the literature. The possibleinteraction of GLDH with the mitochondrial respiratory electrontransport chain was studied using 5 µg/mL antimycin A and 1 mMKCN as inhibitors of complexes III and IV,respectively.

Chlorophyll and Protein Determinations

Chlorophylls and proteins were measured according to the methods of Arnon (1949) and Bradford (1976),respectively.

Analysis of GLDH Structure

GLDH transmembrane regions and orientation were predicted with the program TMpred (Hofmann and Stoffel, 1993), which predictsprotein membrane-spanning regions and their orientation. The algorithmis based on the statistical analysis of TMbase, a database ofnaturally occurring transmembrane proteins. The prediction ismade using a combination of several weight matrices for scoring.The prediction of GLDH was based in the protein sequence deducedfrom GLDH cDNA from sweet potato (Imai et al., 1998; accessionno. AB017357).

	ACKNOWLEDGMENTS

The authors wish to thank Drs. M. Nishikimi and T. Imai for the antibody against GLDH. The authors are indebted to Guy Kiddle,Prof. Verrier, and the BioInformatics Department at IACR-Rothamstedfor invaluable assistance in the computer analysis of GLDH orientationwithin the inner mitochondrialmembrane.

	FOOTNOTES

Received September 29, 1999; accepted February 2, 2000.

¹ C.B. acknowledges financial support from the British Council, Consejo Nacional de Investigaciones Científicas y Técnicas,and Fundacion Antorchas at IACR-Rothamsted.

^* Corresponding author; e-mail gabriela.pastori{at}bbsrc.ac.uk; fax 44-1582-763010.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
RESULTS
DISCUSSION
MATERIALS AND METHODS
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Ascorbate Biosynthesis in Mitochondria Is Linked to the Electron Transport Chain between Complexes III and IV¹