Identification and Characterization of MAE1, the Saccharomyces cerevisiae Structural Gene Encoding Mitochondrial Malic Enzyme

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J Bacteriol, June 1998, p. 2875-2882, Vol. 180, No. 11
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Identification and Characterization of MAE1, the Saccharomyces cerevisiae Structural Gene Encoding Mitochondrial Malic Enzyme

Eckhard Boles,¹ Patricia de Jong-Gubbels,² and Jack T. Pronk²^,^*

Institut für Mikrobiologie, Heinrich-Heine-Universität, D-40225 Düsseldorf, Germany,¹ and Kluyver Institute of Biotechnology, Delft University of Technology, 2628 BC Delft, The Netherlands²

Received 23 February 1998/Accepted 27 March 1998

	ABSTRACT

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Pyruvate, a precursor for several amino acids, can be synthesized from phosphoenolpyruvate by pyruvate kinase. Nevertheless,pyk1 pyk2 mutants of Saccharomyces cerevisiae devoid of pyruvatekinase activity grew normally on ethanol in defined media, indicatingthe presence of an alternative route for pyruvate synthesis. Acandidate for this role is malic enzyme, which catalyzes the oxidativedecarboxylation of malate to pyruvate. Disruption of open readingframe YKL029c, which is homologous to malic enzyme genes fromother organisms, abolished malic enzyme activity in extracts ofglucose-grown cells. Conversely, overexpression of YKL029c/MAE1from the MET25 promoter resulted in an up to 33-fold increaseof malic enzyme activity. Growth studies with mutants demonstratedthat presence of either Pyk1p or Mae1p is required for growthon ethanol. Mutants lacking both enzymes could be rescued by additionof alanine or pyruvate to ethanol cultures. Disruption of MAE1alone did not result in a clear phenotype. Regulation of MAE1was studied by determining enzyme activities and MAE1 mRNA levelsin wild-type cultures and by measuring $beta$ -galactosidase activitiesin a strain carrying a MAE1::lacZ fusion. Both in shake flaskcultures and in carbon-limited chemostat cultures, MAE1 was constitutivelyexpressed. A three- to fourfold induction was observed duringanaerobic growth on glucose. Subcellular fractionation experimentsindicated that malic enzyme in S. cerevisiae is a mitochondrialenzyme. Its regulation and localization suggest a role in theprovision of intramitochondrial NADPH or pyruvate under anaerobicgrowth conditions. However, since null mutants could still growanaerobically, this function is apparently not essential.

	INTRODUCTION

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In the yeast Saccharomyces cerevisiae, pyruvate is a key intermediate in sugar dissimilation as well as a precursor for synthesisof the amino acids alanine, leucine, isoleucine, and valine (21,28). During growth on sugars, pyruvate can be provided by pyruvatekinase (EC 2.7.1.40), the enzyme catalyzing the last reactionof the glycolytic pathway (Fig. 1).

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FIG. 1. Possible role of pyruvate kinase and malic enzyme in the formation of pyruvate as a biosynthetic precursor in S. cerevisiae. Abbreviations: PYK, pyruvate kinase; PCK, phosphoenolpyruvate carboxykinase; MAE, malic enzyme; acetyl-CoA, acetyl coenzyme A; TCA, tricarboxylic acid.

In S. cerevisiae, two structural genes (PYK1 and PYK2) that each encode an active pyruvate kinase isoenzyme have been identified(2, 3, 7, 16). PYK1 is essential for growth on sugars,and transcription of PYK1 is induced by them. The Pyk1p enzymeis strongly activated by fructose-1,6-bisphosphate. The secondpyruvate kinase isoenzyme, Pyk2p, is insensitive to fructose-1,6-bisphosphate.Surprisingly, transcription of PYK2 is subject to glucose repressionand is induced on ethanol. Unless it is overproduced, Pyk2p cannotsustain growth of pyk1 null mutants on sugars (3).

When S. cerevisiae is grown on ethanol or acetate, pyruvate kinase has no role in dissimilation. Nevertheless, pyruvate stillhas to be generated for amino acid biosynthesis. In theory, thismay occur via at least two mechanisms (Fig. 1): (i) synthesisof phosphoenolpyruvate from acetyl coenzyme A via the glyoxylatecycle and the gluconeogenic enzyme phosphoenolpyruvate carboxykinase,thus providing the substrate for pyruvate kinase, and (ii) decarboxylationof malate, an intermediate of the glyoxylate cycle, to pyruvateby malic enzyme.

Malic enzyme [(S)-malate:NAD(P)⁺ oxidoreductase (decarboxylating); EC 1.1.1.38-40] catalyzes the oxidative decarboxylationof malate to pyruvate and carbon dioxide, using NAD⁺ or NADP⁺ as the electron acceptor [malate + NAD(P)⁺ $right-arrow$ pyruvate + CO₂ + NAD(P)H]. The enzyme, which can also catalyzethe reductive carboxylation of pyruvate to malate, occurs in awide variety of organisms, including prokaryotes, fungi, plants,and animals. In eukaryotes, malic enzyme may reside in the cytosol,in mitochondria, or, in the case of plants, in the chloroplasts(24, 31).

Malic enzyme has been demonstrated in the yeasts Schizosaccharomyces pombe (27, 31), Rhodotorula glutinis (12), andZygosaccharomyces bailii (15). Its status in S. cerevisiae issomewhat enigmatic. Polakis and Bartley (19) reported that thisyeast did not contain NADP⁺-dependent malate-decarboxylating activity. Furthermore, the inabilityof pyruvate carboxylase-negative S. cerevisiae mutants to growon glucose as the sole carbon source (26) indicates that reductivecarboxylation of pyruvate by malic enzyme cannot replace the anapleroticfunction of pyruvate carboxylase. This notwithstanding, Fuck etal. (13) reported the occurrence of very low activities of malicenzyme in cell extracts of S. cerevisiae. The partially purifiedS. cerevisiae malic enzyme was reported to have a high K_m formalate (ca. 50 mM) and used either NAD⁺ or NADP⁺ as an electron acceptor. Occurrence of malic enzyme in S. cerevisiaeis of applied significance, as conversion of malate to pyruvate(and subsequently to ethanol) can be used to decrease the acidityof wines. With this specific aim, the S. pombe MAE2 gene encodingmalic enzyme has been introduced into S. cerevisiae (32).

So far, it is unknown whether and to what extent pyruvate kinase and malic enzyme contribute to the provision of pyruvatein S. cerevisiae cells growing on ethanol or acetate. Growth onethanol of mutants lacking the two PYK genes has not been investigatedin detail (3), and since no malic enzyme structural gene hasbeen identified in S. cerevisiae, defined mutants lacking theenzyme are not available.

In the course of our work on pyruvate metabolism, evidence was obtained that in addition to the pyruvate kinase reaction,S. cerevisiae contains an alternative pathway for pyruvate synthesis.After systematic sequencing of the yeast genome, a new open readingframe (ORF) of S. cerevisiae which exhibits a high degree of similarityto malic enzyme structural genes from other organisms was identified.In this study, we demonstrate that this ORF indeed encodes anactive malic enzyme. The aim of this work was to investigate therole, regulation, and subcellular localization of the S. cerevisiaemalic enzyme.

	MATERIALS AND METHODS

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Yeast strains and maintenance. All yeast strains used in this work were derived from isogenic strains of the CEN.PK series kindly provided by K.-D. Entianand P. Kötter (Frankfurt, Germany) and are described in Table1. CEN.PK113-7D (MATa MAL2-8^c SUC2) was used as a prototrophic wild-type strain. ChromosomalDNA from strain CEN.PK2-1C (MATa leu2-3, 112 ura3-52 trp1-289his3- $Delta$ 1 MAL2-8^c SUC2) was used to PCR amplify the MAE1 gene. Construction ofstrain EBY121B (MAT $alpha$ leu2-3, 112 ura3-52 trp1-289 his3- $Delta$ 1 MAL2-8^c SUC2 pyk1 $Delta$ ::HIS3 pyk2 $Delta$ ::URA3) was described previously (3).For long-term maintenance, yeast strains were pregrown overnightin shake flasks at 30°C in YPE medium (10 g of Difco yeast extract,20 g of Difco peptone, and 10 g of ethanol liter¹). After addition of glycerol to a concentration of 20% (vol/vol),2 ml aliquots were stored at $-$ 80°C. Working stocks were maintainedon YPE agar slants.

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TABLE 1. S. cerevisiae strains used

Molecular biology techniques. DNA and RNA were prepared and manipulated according to published procedures (22, 23, 25). Transformation of yeast cellswas carried out by the freeze method (10). Escherichia coliJM101, DH5 $alpha$ F', and SURE (Stratagene GmbH) were transformed byelectroporation. p426MET25 (18) served as a vector.

Construction of deletion strains. A mae1 deletion strain was constructed by using a modification of the PCR targeting technique (14, 35). pUG6 (14) wascleaved with SalI and BglII, removing the first of its two loxPsites. In their place, a 3.1-kb SalI/BglII fragment from plasmidpJJH397 (kindly provided by J. J. Heinisch, Düsseldorf, Germany)containing the lacZ gene of E. coli was inserted, resulting inplasmid pUG6lacZ. This plasmid was then used as a template togenerate by PCR a DNA molecule consisting of a lacZ-kanMX markercassette flanked by short homology regions to the MAE1 locus.For this purpose two oligonucleotides were constructed; one (S1-MAE1)[5'-ATGCTTAGAACCAGACTATCCGTTTCCGTTGCTGCTAGATCGCAACTATTCGTACGCTGCAGGTCGAC-3'])contains the sequence from +1 (A of start codon) to +48 of theMAE1 ORF as its short flanking homology region, and the other(S2-MAE1 [5'-ACATCATGTAAAGAGCGGGTGTTGATACCAGCCCATTCCGCATCAGCATAGGCCACTAGTGGATCTG-3'])contains the complementary sequence from +1329 to +1373 of theMAE1 ORF as its short flanking homology region. The corresponding3' ends of the two oligonucleotides bind at the beginning of thelacZ gene and, on the complementary strand, behind the loxP sitein plasmid pUG6lacZ, respectively. PCR with the Expand High FidelityPCR system (Boehringer, Mannheim, Germany), with S1-MAE1 and S2-MAE1as primers and pUG6lacZ (50 ng) as the template (40 s at 95°C,30 s at 50°C, 5 min at 68°C; 25 cycles) yielded a 4.6-kb DNA fragment.This PCR product could be used to replace the DNA sequence encodingamino acids 17 to 443 of Mae1p by the lacZ-kanMX module. Simultaneously,the $beta$ -galactosidase enzyme is fused in frame with the first 16amino acids of Mae1p, allowing to use $beta$ -galactosidase activityas a reporter system for expression of MAE1. Five micrograms ofthe PCR product was transformed into strain CEN.PK113-7D, selectingfor resistance to G418 (200 mg liter¹) on YPD agar plates. Whole yeast cell PCR was used to confirmthe correct replacements in the G418-resistant transformants.One correct transformant strain, EBY.D138A (mae1 $Delta$ ::lacZ-kanMX),was crossed with strain EBY121B (pyk1 $Delta$ pyk2 $Delta$ ), the diploid strainwas sporulated, and tetrads were dissected, resulting in all differentcombinations of MAE1, PYK1, and PYK2 wild-type and deletion alleles,all in an otherwise prototrophic background (Table 1).

Construction of plasmids. The MAE1 gene was cloned by PCR with a pair of primers designed to amplify a DNA fragment enclosing the complete MAE1 ORFwith 90 bp of its 5' regulatory region and 23 bp of its 3' region.Additionally, they added a BamHI and an EcoRI restriction siteat the 5' and 3' ends of the PCR product, respectively. PCR withprimers A12-MAE1 (5'-CGGGATCCAGCTTCGGATATTTGT-3') and A42-MAE1(5'-GGAATTCAGGCGTTGGTTATGCTT-3'), with the Expand High FidelityPCR system and whole yeast cells of strain CEN.PK2-1C as the template(45 s at 95°C, 30 s at 50°C, 3 min at 68°C; 30 cycles), yieldeda 2.1-kb DNA fragment. The fragment was cleaved with BamHI andEcoRI and cloned into the high-copy-number vector p426MET25 (18),resulting in plasmid YEpMET25-MAE1. In this plasmid, the MAE1gene is under control of the methionine-repressible MET25 promoterand the CYC1 terminator.

Shake flask cultivation. Specific growth rates were determined in 500-ml shake flasks containing 100 ml of a mineral medium supplemented with vitamins(30). Glucose (10 g liter¹) or ethanol (10 g liter¹) was added as the carbon source. Where indicated, L-alanine wasadded to a concentration of 10 mmol liter¹. Cultures were incubated at 30°C in a rotary shaker at 150 rpmand inoculated with 1 ml of an exponentially growing shake flaskculture on the same medium. Optical densities at 660 nm were determinedafter dilution of culture samples with water to an optical densityat 660 nm below 0.35. Exponential growth rates were determinedin independent duplicate experiments.

Chemostat cultivation. Aerobic and anaerobic, carbon- and energy-limited chemostat cultivation was performed at 30°C in 2-liter laboratory fermentors(Applikon, Schiedam, The Netherlands). Chemostats were operatedat a dilution rate of (D) 0.10 h¹ and at a stirrer speed of 800 rpm. The culture pH was maintainedat 5.0 by automatic addition of 2.0 M KOH via an Applikon ADI1030 biocontroller. The working volume was kept at 1.0 liter byremoval of effluent from the middle of the culture via an electricallevel controller. This ensured that the biomass concentrationsin the effluent differed by less than 2% from those taken directlyfrom the culture. In aerobic cultures, an airflow of 0.5 litermin¹ was maintained by using a Brooks 5876 gas flow controller (BrooksB.V., Veenendaal, The Netherlands). During anaerobic cultivation,the fermenter and the medium reservoir were flushed with nitrogengas at a flow rate of 0.5 liter min¹. To minimize oxygen diffusion, anaerobic fermentors and mediumreservoirs were fitted with Norprene tubing. The dissolved oxygentension, which was measured with an Ingold polarographic O₂ electrode,remained above 30% of air saturation in aerobic cultures and below0.1% of air saturation in anaerobic cultures. A defined mineralmedium supplemented with vitamins (30) was used. Carbon sources(glucose, ethanol, and acetate) were added at a concentrationof 250 mM carbon liter¹. For anaerobic cultivation, the medium was supplemented withthe anaerobic growth factors Tween 80 (420 mg liter¹) and ergosterol (10 mg liter¹) (29). When asparate replaced ammonium sulfate as the nitrogensource, its concentration in the medium was 50 mmol liter¹.

Preparation of cell extracts. Cells from exponentially growing shake flask cultures or chemostat cultures (ca. 80 mg [dry weight]) were harvested by centrifugationat 1,950 × g for 10 min, washed once, and resuspended in 5 mlof 10 mM potassium phosphate buffer (pH 7.5) containing 2 mM EDTA.After storage at $-$ 37°C, cells were thawed on ice and disruptedby sonication. When cell extracts were prepared for malic enzymeassays, cells were washed once and resuspended in 4 ml of Trisbuffer (50 mM Tris-HCl [pH 7.5] containing 1 mM dithiothreitoland 2 mM MgCl₂). When cell extracts were prepared for $beta$ -galactosidaseassays, cells were washed once and resuspended in 50 mM phosphatebuffer (pH 7.0). After resuspension in the appropriate buffer,cells were disrupted by sonication with 0.7-mm-diameter acid-washedglass beads (Sigma) at 0°C for 3 min (30-s intervals), using anMSE sonicator (150-W output, 8-µm peak-to-peak amplitude). Wholecells and debris were removed by centrifugation at 31,000 × g(20 min, 4°C). The clear supernatant was used as the cell extract.Cell extracts for malic enzyme assays were dialyzed for 4 h at0°C against 50 mM Tris buffer by using 0.5- to 3.0-ml Slide-a-lyzercassettes (10,000-molecular-weight cutoff; Pierce).

Isolation of mitochondria. Mitochondria were isolated from glucose-limited, aerobic chemostat cultures (D = 0.10 h¹). The procedure involved differential centrifugation of cellhomogenates obtained by controlled lysis of spheroplasts essentiallyas described by Bruinenberg et al. (6).

Enzyme assays. Malic enzyme (EC 1.1.1.40) was assayed at 30°C and at 340 nm in a Hitachi model 100-60 spectrophotometer. The assay mixture(1 ml) contained 100 µmol of Tris-HCl (pH 7.5), 10 µmol of MgCl₂,0.4 µmol of NADP⁺, and cell extract. The reaction was initiated by addition of100 µmol of potassium L-malate (pH 7.5). Specific activities werecalculated based on an extinction coefficient of NADPH of 6.3mM¹ cm¹. Latency of malic enzyme in mitochondrial fractions was investigatedby measuring its activity in the presence and absence of 0.65mol of sorbitol liter¹. $beta$ -Galactosidase (EC 3.2.1.23) activity in cell extracts wasmeasured at 30°C with a discontinuous assay measuring the hydrolysisof o-nitrophenylgalactoside (17). Glucose-6-phosphate dehydrogenase(EC 1.1.1.49) was assayed as described by Postma et al. (20);cytochrome c oxidase (EC 1.9.3.1) was assayed by the methoddescribed by Douma et al. (11).

Protein determination. Protein in cell extracts and mitochondrial fractions was assayed by the Lowry method. Bovine serum albumin (fatty acid free;Sigma) was used as a standard.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Growth characteristics of pyruvate kinase-deficient mutants. To investigate whether the presence of either of the pyruvate kinase isoenzymes of S. cerevisiae is required for growth onethanol as the sole carbon source, prototrophic mutants in whicheither PYK1 or PYK2 or both were deleted were constructed. Asreported previously, a functional copy of PYK1 was required forgrowth on glucose as the sole carbon source, whereas deletionof PYK2 had no effect on the specific growth rate on glucose (Table2). However, mutants lacking either one or both PYK genes stillexhibited normal growth rates on a defined medium containing ethanolas the sole carbon source (Table 2). This finding indicated thatduring growth on ethanol, S. cerevisiae is able to synthesizepyruvate via an alternative pathway.

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TABLE 2. Maximum specific growth rates of the prototrophic wild-type strain S. cerevisiae EBY.D149 and of isogenic strains carrying various combinations of null mutations in PYK1, PYK2, and MAE1 (Table 1)^a

YKL029c, a possible structural gene encoding malic enzyme. A possible explanation for the observed growth of pyk mutant strains on ethanol would be the existence of a malic enzyme,catalyzing the oxidative decarboxylation of malate to pyruvate(Fig. 1). Therefore, we compared the complete genome sequenceof S. cerevisiae with the deduced amino acid sequence of the S.pombe malic enzyme, Mae2p (31). We found an ORF designated YKL029cwhich codes for a putative protein with 669 amino acids showing47% amino acid identity to the S. pombe Mae2p. Moreover, aminoacid residues which have been proposed to be involved in substrateor cofactor binding or are conserved between different malic enzymes(summarized in reference 31) are also conserved in S. cerevisiaeMae1p.

YKL029c/MAE1 encodes a functional malic enzyme. To investigate whether YKL029c/MAE1 is indeed a structural gene encoding malic enzyme, malic enzyme activities were determinedin cell extracts of the prototrophic wild-type strain EBY.D149and strain EBY.D152. In the latter strain, most of the MAE1 ORFwas deleted and replaced by a lacZ-kanMX cassette. In glucose-grownshake flask cultures, the wild-type strain exhibited a malic enzymeactivity of 32 nmol min¹ mg of protein¹. Enzyme activities were assayed in dialyzed extracts, since highendogenous rates of NADP⁺ reduction were found in nondialyzed extracts. Malic enzyme activitywas completely abolished in the deletion mutant (Table 3).

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TABLE 3. Specific activities of malic enzyme in dialyzed cell extracts of wild-type S. cerevisiae EBY.D149 and three isogenic mutants^a

To overexpress MAE1, the gene was placed under control of the strong methionine-repressible promoter MET25 in the multicopyvector p426MET25, which carries a URA3 selectable marker. Introductionof this construct into the wild-type strain CEN.PK113-13D in theabsence of methionine resulted in an over 10-fold increase ofthe malic enzyme activity relative to an empty-vector referencestrain and the prototrophic wild-type strain EBY.D149 (Table 2).These results are fully consistent with MAE1 being a structuralgene encoding a protein with malic enzyme activity.

Relationship to malic enzymes from other organisms. To gain some insight into the evolutionary relationships between S. cerevisiae Mae1p and malic enzymes from various organisms,we used the deduced amino acid sequences to calculate a dendrogram.Seven blocks of related malic enzymes from different organismswere found (Fig. 2). The first cluster comprises the malic enzymesof the yeasts S. pombe and S. cerevisiae. In contrast to the malicenzyme from S. pombe and most other organisms, the S. cerevisiaeenzyme has a long amino-terminal extension of about 85 amino acids.The second group of sequences which are closely related to theyeast malic enzymes (about 40% identity) comprises isoenzymesfrom eubacteria, indicating that the yeast enzymes are more relatedto these bacterial isoenzymes than to those of higher eukaryotes,which comprise clusters III to VI. Moreover, there is an additionalgroup of bacterial isoenzymes (cluster VII) which is only verydistantly related to the other malic enzymes.

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FIG. 2. Sequence identity dendrogram of malic enzymes and related proteins from different organisms. The dendrogram was obtained by comparison of the deduced amino acid sequence of S. cerevisiae Mae1p against all nucleotide sequence databases (December 1997) dynamically translated in all reading frames; partial malic enzyme sequences were omitted. The sequences were clustered by the PC/GENE program (IntelliGenetics Inc., release 6.70, 1992) at standard settings. Blocks of homology are boxed and numbered I to VII. For simplicity, not all sequences of cluster VII are shown. If different malic enzyme-related sequences have been identified in an organism, this is indicated by the numbers or names in parentheses. In this case, if known, also the corresponding intracellular localization is indicated: c, cytoplasm; m, mitochondria; ch, chloroplasts.

Role of pyruvate kinase and malic enzyme during growth on ethanol. To investigate whether malic enzyme is responsible for the synthesis of pyruvate in pyruvate kinase-negative mutants of S.cerevisiae, the mae1 deletion mutant EBY.D138A was crossed withstrain EBY121B (pyk1 $Delta$ pyk2 $Delta$ ), and after sporulation of the diploidstrain, spores with all different combinations of the MAE1, PYK1,and PYK2 wild-type and deletion alleles in an otherwise prototrophicbackground were selected (Table 1).

The growth properties of the mae1 deletion strains EBY.D138A and EBY.D152 on yeast extract-peptone medium with glucose orethanol as the carbon source were indistinguishable from the correspondingwild-type strain (data not shown). Deletion of MAE1 did not significantlyaffect the specific growth rate on glucose mineral medium of strainscontaining a wild-type PYK1 allele (Table 2). Deletion of MAE1caused a reduction of the specific growth rate on ethanol. However,upon prolonged incubation, the specific growth rate on ethanolof mae1 null cultures increased to near wild-type levels (Table2). The reason for this phenomenon, which was reproducibly observedin four independent growth experiments with the mae1 null strain,but not with the other strains, was not further investigated.

When both PYK1 and MAE1 were deleted, the cells were no longer able to grow on ethanol. In contrast, cells in which MAE1 andPYK2 were deleted still grew on ethanol, albeit more slowly thancells in which only MAE1 was deleted (Table 2). This findingindicates that during growth of S. cerevisiae on ethanol, pyruvatefor biosynthetic purposes can be efficiently provided either byPyk1p in combination with Pyk2p or by Mae1p. Indeed, growth ofpyk1 mae1 double mutants or pyk1 pyk2 mae1 triple mutants on ethanolcould be completely restored by the addition of low concentrationsof alanine (Table 2) or pyruvate (data not shown). Growth ofthese mutants was also restored after transformation with plasmidYEpMET25-MAE1, demonstrating that the mae1 deletion is indeedthe cause of the observed growth defect.

Regulation of malic enzyme synthesis. Regulation of the MAE1 gene as a function of growth conditions was investigated by measuring malic enzyme activities in cellextracts and by Northern analysis of MAE1 transcription. Furthermore,the mae1 deletion was constructed in such a way that simultaneouslythe first 16 amino acids of the truncated MAE1 ORF were fusedto the E. coli lacZ gene. This enabled us to study regulationof MAE1 by measuring $beta$ -galactosidase activities in cell extractsof the mae1 deletion mutant EBY.D152.

Experiments in shake flask cultures indicated that MAE1 was expressed at low levels during growth on glucose, ethanol, andacetate. Malic enzyme assays in the shake flask cultures suggesteda twofold-higher activity in glucose-grown cultures than in culturesgrowing exponentially on ethanol or acetate (Table 4). However,experiments with the strain carrying the MAE1-lacZ fusion yielded $beta$ -galactosidase activities that were not substantially differentfor the three substrates tested. Also in the Northern experiments,the levels of the MAE1 transcripts did not differ more than twofoldbetween the different conditions in shake flask cultures (Fig.3). Addition of alanine, which could complement the growth defectof mae1 $Delta$ pyk1 $Delta$ double mutants (Table 2), had no effect on MAE1expression (Table 4; Fig. 3).

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TABLE 4. Regulation of MAE1 expression in shake flask cultures and carbon-limited chemostat cultures (D = 0.10 h¹)^a

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FIG. 3. Northern analysis of MAE1 transcription. Cells of the wild-type strain EBY.D149 (lanes 1 to 7) and the mae1 deletion strain EBY.D152 (lane 8) were grown in carbon-limited chemostat cultures (continuous cultures) or in shake flask cultures (batch cultures) with different carbon sources (glucose or ethanol [EtOH]), with different nitrogen sources (ammonia or, in lane 2, aspartate), or supplemented with alanine (lane 7), either aerobically or anaerobically (lane 4). The mae1 $Delta$ strain was grown on YPD medium. Total RNA was prepared from these cultures. The filter was probed with a mixture of a 2.1-kb PCR fragment of the MAE1 coding region and a 3.2-kb DNA fragment containing the complete actin sequence (loading control), both labeled with ³²P, in a 1:1 count ratio. The autoradiogram was exposed to Fuji RX.

In contrast to shake flask cultivation, chemostat cultivation offers the possibility to control specific growth rate via thesupply rate of the growth-limiting nutrient. Thus, gene expressionon different carbon sources or under different cultivation conditionscan be compared at a fixed specific growth rate. Moreover, otherimportant growth parameters such as dissolved oxygen concentrationand culture pH can be kept constant, thus allowing studies onthe impact of a single growth parameter on gene expression.

In aerobic, carbon-limited chemostat cultures of S. cerevisiae grown at a fixed specific growth rate of 0.10 h¹, MAE1 expression did not differ substantially when glucose, ethanol,or acetate was used as the carbon source (Fig. 3; Table 4). Also,provision of aspartate as a nitrogen source, which leads to anincreased production of four-carbon metabolites by the cells,did not lead to a substantial increase of MAE1 expression (Fig.3; Table 4). A clear induction of MAE1 expression was observedonly during anaerobic cultivation on glucose, with a ca. threefoldincrease at the transcriptional level (Fig. 3; Table 4) and aca. fourfold increase of the enzyme activity in cell extracts(Table 4) relative to the aerobic, glucose-limited referencecultures.

Subcellular localization of malic enzyme. The subcellular localization of the S. cerevisiae malic enzyme was investigated by differential centrifugation after controlledlysis of spheroplasts, prepared from aerobic, glucose-limitedchemostat cultures (D = 0.10 h¹). Initial experiments with wild-type cultures revealed enzymeactivity in the particulate fraction. However, enzyme activitiesin the homogenates (in which the protein content was lower thanin the particulate fractions) were below the detection limit,which precluded calculation of malic enzyme recoveries in thevarious fractions (data not shown). Since this result might havebeen due to the low activities of malic enzyme in wild-type cultures(Tables 3 and 4), fractionation experiments were repeated withthe MAE1-overexpressing strain EBY.D160.

Similar to the mitochondrial marker enzyme cytochrome c oxidase, malic enzyme was completely recovered in the particulatefraction (Table 5). Conversely, the cytosolic enzyme glucose-6-phosphatedehydrogenase was recovered in the supernatant obtained afterhigh-speed centrifugation of cell homogenates (Table 5).

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TABLE 5. Subcellular localization of malic enzyme^a

In the enzyme assays performed to calculate recoveries in the various fractions, no precautions were taken to osmoticallystabilize the mitochondria. To investigate whether malic enzymeactivity in the particulate fraction exhibited latency and consequentlywas of intraorganellar origin, are carried out control experimentsin which malic enzyme assays were performed in the presence of0.6 M sorbitol. Under these conditions, only a very low activity(22 nmol min¹ mg of protein¹) was measured in the particulate fraction. Malic enzyme activityincreased to 300 nmol min¹ mg of protein¹ either after sonication (30 s) of the mitochondrial pellet orafter addition of 0.05% Triton X-100 to the sorbitol-containingassay mixture prior to the enzyme assay.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Characteristics and compartmentation of malic enzyme in S. cerevisiae. Our work supports the original report of Fuck et al. (13) that S. cerevisiae contains a genuine malic enzyme activity. Wehave identified and analyzed the corresponding structural geneand determined characteristics of its regulation.

Malic enzymes from different organisms differ in subcellular localization, being found in the cytosol, in mitochondria, orin chloroplasts. Moreover, they differ in cofactor requirement,being able to use either NAD⁺ or NADP⁺ or both as electron acceptors (24, 31). In subcellular fractionationexperiments, malic enzyme activity was recovered in a particulatefraction (Table 5) from which it could be liberated after destructionof the organellar structures. The technique used in this studydoes not discriminate between mitochondria and other organelles.Although present at very low numbers in glucose-limited chemostatcultures, especially peroxisomes might contaminate the particulatefractions. However, as yeast peroxisomes are rather fragile (9,37), the complete recovery and high degree of latency in theparticulate fraction (Table 5) argues against a peroxisomal locationof the S. cerevisiae malic enzyme. A further indication that Mae1pis a mitochondrial protein was obtained from its predicted aminoacid sequence, which shows typical features of mitochondrial targetingsequences. Those targeting signals are N-terminal sequences ofabout 15 to 30 amino acids. They show a preponderance of basicand hydroxyl-carrying residues (Arg, Ser, and Leu) and a correspondingpaucity of acidic residues (1, 34). The function of mitochondrialtargeting sequences is largely determined by the overall balancebetween these basic, hydrophobic, and hydroxylated amino acids(1), and they may form amphiphilic helices (34). The 30 N-terminalamino acids of Mae1p include seven Arg, five Leu, and five Serresidues but no acidic amino acid. This clearly fulfills the demandsof mitochondrial targeting sequences and supports our experimentalresults.

So far, the subcellular localization of malic enzymes in other yeasts has not been investigated. Especially interesting inthis respect is the S. pombe malic enzyme, Mae2p (31), the predictedamino acid sequence of which does not contain a mitochondrialtargeting sequence (our observation). Introduction of the S. pombeMAE2 gene together with a malate permease-encoding gene into S.cerevisiae has been successfully applied to reduce the malic acidcontent of wines (32). The rather inefficient degradation ofmalate by the recombinant strains was attributed to regulatoryconstraints on the S. pombe malic enzyme in S. cerevisiae. Itwill be interesting to see whether overexpression of S. cerevisiaeMAE1 or of a truncated version of this enzyme lacking the mitochondrialtargeting sequence can circumvent some of these difficulties.

In contrast to the S. pombe malic enzyme, which can use only NAD⁺ (27), malic enzyme from S. cerevisiae has been reported touse both NAD⁺ and NADP⁺ as electron acceptors (13). Furthermore, the K_m value of theS. cerevisiae enzyme for malate was found to be over 15-fold higherthan that of the S. pombe malic enzyme (13, 27). Despite thesedifferences in cofactor specificity, substrate affinity, and,probably, localization, the amino acid sequences of the two yeastenzymes show significant similarities to each other (Fig. 2).Interestingly, the yeast enzymes are more closely related to agroup of eubacterial malic enzymes (cluster II) than to thoseof higher eukaryotes, like plants (cluster III, including onefungal enzyme, and cluster V), animals and humans (cluster IV),and human parasites (cluster VI). Cluster VII comprises anothergroup of eubacterial malic enzyme-related proteins which are,however, only very distantly related to the yeast enzymes. Intriguingly,within the individual clusters are found cytosolic as well asmitochondrial or chloroplast isoenzymes, which can be either NAD⁺ or NADP⁺ dependent. This finding indicates that sequence homologies amongmalic enzymes from various organisms are primarily determinedby phylogenetic relationships rather than being the result offunctional constraints related to catalytic properties and intracellularlocalization.

Regulation and physiological function of malic enzyme. The MAE1 gene is expressed at low but constitutive levels during cultivation on the carbon sources glucose, ethanol, and acetate.Moreover, YKL029c/MAE1 was recently found to be constitutivelytranscribed during batch growth in a yeast extract-peptone mediumfrom 2% glucose until glucose exhaustion (8). Although a three-to fourfold induction of MAE1 was observed under anaerobic conditions,a database search (36) with the promoter sequence of the MAE1gene did not reveal any significant transcription factor bindingsites.

The regulatory pattern of malic enzyme suggests a specific function in anaerobic metabolism, e.g., in the provision of intramitochondrialNADPH or pyruvate. However, the growth properties of an mae1 nullmutant indicated that any such function was not essential underthe experimental conditions tested. Growth of the mae1 mutantson glucose under aerobic conditions was not affected, and alsoin anaerobic, glucose-limited chemostat cultures of wild-typeand mae1 null strains (D = 0.10 h¹), yields of biomass and ethanol were the same (data not shown).

A cyclic reaction involving pyruvate carboxylase, NAD⁺-dependent malate dehydrogenase, a mitochondrial dicarboxylate carrier,and (NADP⁺-linked) malic enzyme could act as a transhydrogenase system.Such a system could theoretically convert part of the NADH formedin biosynthesis (33) to NADPH, a cofactor for biosynthetic reactions.However, specific production rates of glycerol, which is the mainredox sink for NADH under anaerobic conditions (33), were thesame in anaerobic chemostat cultures of an mae1 null mutant andthe isogenic wild type (data not shown).

Our results demonstrate that the mitochondrial malic enzyme can meet the biosynthetic requirement of S. cerevisiae for pyruvateduring growth on ethanol or acetate. Alternatively, pyruvate canbe provided by the Pyk1p isoenzyme of cytosolic pyruvate kinase.The recently discovered Pyk2p isoenzyme (3) alone could notsustain growth on ethanol. This is surprising, as its lack ofactivation by fructose-1,6-bisphosphate and relatively high transcriptlevel during growth on ethanol (3) are both compatible witha role of Pyk2p during gluconeogenic growth, when intracellularfructose-1,6-bisphospate concentrations are low. Conversely, thekinetic properties of Pyk1p suggest a low in vivo activity duringgluconeogenic growth, thus questioning its qualification in theprovision of pyruvate (2). The higher growth rate on ethanolif not only Pyk1p but also Pyk2p is expressed (Table 2; compareEBY.D152 and EBY.D155) may reflect an in vivo interaction of theisoenzymes. Such an interaction (e.g., via formation of heteromers)might also explain the slightly different kinetics of pyruvatekinase activity in extracts of wild-type cells and pyk2 null mutants(3).

At least one additional S. cerevisiae enzyme activity described in the literature could also provide pyruvate for biosyntheticpurposes. Serine dehydratase (encoded by the CHA1 gene) [4])converts serine to pyruvate. The requirement for induction byserine (5) or other regulatory constraints may explain whythis enzyme cannot meet the requirement for pyruvate of pyk1 $Delta$ pyk2 $Delta$ mae1 $Delta$ mutants during growth on ethanol media that containammonium salts as the nitrogen source. Suppressor mutants observedupon prolonged incubation of ethanol plates of pyk1 $Delta$ pyk2 $Delta$ mae1 $Delta$ mutants (2a) may represent regulatory mutants expressing serinedehydratase in media lacking serine.

Conclusions and outlook. In this study, a clear phenotype of mae1 null mutants became apparent only when also PYK1 was inactivated. Thus, as in theother eukaryotic organisms investigated in the literature, thephysiological function of malic enzyme in wild-type S. cerevisiaeremains enigmatic. The identification of the MAE1 gene in S. cerevisiaeand the accessibility of this yeast to molecular genetic and physiologicalinvestigations make this organism an interesting model systemfor further studies on this intriguing enzyme. Moreover, the availabilityof an Mae1p-overproducing strain will facilitate enzyme purificationand thus a more detailed enzymological characterization of malicenzyme than was hitherto possible.

	ACKNOWLEDGMENTS

We thank C. P. Hollenberg for his kind support and J. P. van Dijken for critical reading of the manuscript. We are gratefulto K. Freidel for help in performing the Northern analysis andto M. A. H. Luttik for help with the subcellular fractionationexperiments.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Enzymology, Kluyver Institute of Biotechnology, DelftUniversity of Technology, Julianalaan 67, 2628 BC Delft, The Netherlands.Phone: (31) 15 278 3214. Fax: (31) 15 278 2355. E-mail: j.t.pronk{at}stm.tudelft.nl.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Allison, D. S., and G. Schatz. 1986. Artificial mitochondrial presequences. Proc. Natl. Acad. Sci. USA 83:9011-9015[Abstract/Free Full Text].

2. Boles, E. 1997. Pyruvate kinase, p. 171-186. In K.-D. Entian, and F. K. Zimmermann (ed.), Yeast sugar metabolism: biochemistry, genetics, biotechnology and applications. Technomic Publishing Co., Lancaster, Pa.

2a. Boles, E. Unpublished data.

3. Boles, E., F. Schulte, T. Miosga, K. Freidel, E. Schlüter, F. K. Zimmermann, C. P. Hollenberg, and J. J. Heinisch. 1997. Characterization of a glucose-repressed pyruvate kinase (Pyk2p) in Saccharomyces cerevisiae that is catalytically insensitive to fructose-1,6-bisphosphate. J. Bacteriol. 179:2987-2993[Abstract/Free Full Text].

4. Bornaes, C., J. G. Petersen, and S. Holmberg. 1992. Serine and threonine catabolism in Saccharomyces cerevisiae: the CHA1 polypeptide is homologous with other serine and threonine dehydratases. Genetics 131:531-539[Abstract].

5. Bornaes, C., M. W. Ignjatovic, P. Schjerling, M. C. Kielland-Brandt, and S. A. Holmberg. 1993. A regulatory element in the CHA1 promoter which confers inducibility by serine and threonine on Saccharomyces cerevisiae genes. Mol. Cell. Biol. 13:7604-7611[Abstract/Free Full Text].

6. Bruinenberg, P. M., J. P. van Dijken, J. G. Kuenen, and W. A. Scheffers. 1985. Oxidation of NADH and NADPH by mitochondria from the yeast Candida utilis. J. Gen. Microbiol. 131:1043-1051.

7. Burke, R. L., P. Tekamp-Olson, and R. Najarian. 1983. The isolation, characterization, and sequence of the pyruvate kinase gene of Saccharomyces cerevisiae. J. Biol. Chem. 258:2193-2201[Abstract/Free Full Text].

8. DeRisi, J. L., V. R. Iyer, and P. O. Brown. 1997. Exploring the metabolic and genetic control of gene expression on a genomic scale. Science 278:680-686[Abstract/Free Full Text].

9. Distel, B., I. van der Leij, and W. Kos. 1996. Peroxisome isolation, p. 133-138. In I. Evans (ed.), Methods in molecular biology. Humana Press, Totowa, N.J.

10. Dohmen, R. J., A. W. M. Strasser, C. B. Höner, and C. P. Hollenberg. 1991. An efficient transformation procedure enabling long-term storage of competent cells of various yeast genera. Yeast 7:691-692[Medline].

11. Douma, A. C., M. Veenhuis, W. de Koning, M. Evers, and W. Harder. 1985. Dihydroxyacetone synthase is localized in the peroxisomal matrix of methanol-grown Hansenula polymorpha. Arch. Microbiol. 143:237-243.

12. Fernández, M. J., L. Medrano, M. Ruiz-Amil, and M. Losada. 1967. Regulation and function of pyruvate kinase and malate enzyme in yeast. Eur. J. Biochem. 3:11-18[Medline].

13. Fuck, E., G. Stärk, and F. Radler. 1973. Äpfelsäurestoffwechsel bei Saccharomyces. II. Anreicherung und Eigenschaften eines Malatenzyms. Arch. Mikrobiol. 89:223-231[Medline].

14. Güldener, U., S. Heck, T. Fiedler, J. Beinhauer, and J. H. Hegemann. 1996. A new efficient gene disruption cassette for repeated use in budding yeast. Nucleic Acids Res. 24:2519-2524[Abstract/Free Full Text].

15. Kuczynski, J. T., and F. Radler. 1982. The anaerobic metabolism of malate of Saccharomyces bailii and the partial purification of malic enzyme. Arch. Microbiol. 131:266-270[Medline].

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17. Miller, J. H. 1972. In Experiments in molecular genetics. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

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19. Polakis, E. S., and W. Bartley. 1965. Changes in the enzyme activities of Saccharomyces cerevisiae during aerobic growth on different carbon sources. Biochem. J. 97:284-297.

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23. Schmitt, M. E., T. A. Brown, and B. L. Trumpower. 1990. A rapid and simple method for preparation of RNA from Saccharomyces cerevisiae. Nucleic Acids Res. 18:3091-3092[Free Full Text].

24. Schomburg, D., and D. Stephan. 1995. In Enzyme handbook, vol. 9. Class 1.1 oxidoreductases EC 1.1.1.1-EC 1.1.1.149. Springer Verlag, Berlin, Germany.

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26. Stucka, R., S. Dequin, J. M. Salmon, and C. Gancedo. 1991. DNA sequences in chromosomes II and VII code for pyruvate carboxylase isoenzymes in Saccharomyces cerevisiae: analysis of pyruvate carboxylase-deficient strains. Mol. Gen. Genet. 229:307-315[Medline].

27. Temperli, A., U. Künsch, K. Mayer, and I. Busch. 1965. Reinigung und Eigenschaften der Malatdehydrogenase (decarboxylierend) aus Hefe. Biochim. Biophys. Acta 110:630-632[Medline].

28. Umbarger, H. E. 1978. Amino acid biosynthesis and its regulation. Annu. Rev. Biochem. 47:533-606.

29. Verduyn, C., E. Postma, W. A. Scheffers, and J. P. van Dijken. 1990. Physiology of Saccharomyces cerevisiae in anaerobic glucose-limited chemostat cultures. J. Gen. Microbiol. 136:395-403[Abstract/Free Full Text].

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1.	Allison, D. S., and G. Schatz. 1986. Artificial mitochondrial presequences. Proc. Natl. Acad. Sci. USA 83:9011-9015[Abstract/Free Full Text].
2.	Boles, E. 1997. Pyruvate kinase, p. 171-186. In K.-D. Entian, and F. K. Zimmermann (ed.), Yeast sugar metabolism: biochemistry, genetics, biotechnology and applications. Technomic Publishing Co., Lancaster, Pa.
2a.	Boles, E. Unpublished data.
3.	Boles, E., F. Schulte, T. Miosga, K. Freidel, E. Schlüter, F. K. Zimmermann, C. P. Hollenberg, and J. J. Heinisch. 1997. Characterization of a glucose-repressed pyruvate kinase (Pyk2p) in Saccharomyces cerevisiae that is catalytically insensitive to fructose-1,6-bisphosphate. J. Bacteriol. 179:2987-2993[Abstract/Free Full Text].
4.	Bornaes, C., J. G. Petersen, and S. Holmberg. 1992. Serine and threonine catabolism in Saccharomyces cerevisiae: the CHA1 polypeptide is homologous with other serine and threonine dehydratases. Genetics 131:531-539[Abstract].
5.	Bornaes, C., M. W. Ignjatovic, P. Schjerling, M. C. Kielland-Brandt, and S. A. Holmberg. 1993. A regulatory element in the CHA1 promoter which confers inducibility by serine and threonine on Saccharomyces cerevisiae genes. Mol. Cell. Biol. 13:7604-7611[Abstract/Free Full Text].
6.	Bruinenberg, P. M., J. P. van Dijken, J. G. Kuenen, and W. A. Scheffers. 1985. Oxidation of NADH and NADPH by mitochondria from the yeast Candida utilis. J. Gen. Microbiol. 131:1043-1051.
7.	Burke, R. L., P. Tekamp-Olson, and R. Najarian. 1983. The isolation, characterization, and sequence of the pyruvate kinase gene of Saccharomyces cerevisiae. J. Biol. Chem. 258:2193-2201[Abstract/Free Full Text].
8.	DeRisi, J. L., V. R. Iyer, and P. O. Brown. 1997. Exploring the metabolic and genetic control of gene expression on a genomic scale. Science 278:680-686[Abstract/Free Full Text].
9.	Distel, B., I. van der Leij, and W. Kos. 1996. Peroxisome isolation, p. 133-138. In I. Evans (ed.), Methods in molecular biology. Humana Press, Totowa, N.J.
10.	Dohmen, R. J., A. W. M. Strasser, C. B. Höner, and C. P. Hollenberg. 1991. An efficient transformation procedure enabling long-term storage of competent cells of various yeast genera. Yeast 7:691-692[Medline].
11.	Douma, A. C., M. Veenhuis, W. de Koning, M. Evers, and W. Harder. 1985. Dihydroxyacetone synthase is localized in the peroxisomal matrix of methanol-grown Hansenula polymorpha. Arch. Microbiol. 143:237-243.
12.	Fernández, M. J., L. Medrano, M. Ruiz-Amil, and M. Losada. 1967. Regulation and function of pyruvate kinase and malate enzyme in yeast. Eur. J. Biochem. 3:11-18[Medline].
13.	Fuck, E., G. Stärk, and F. Radler. 1973. Äpfelsäurestoffwechsel bei Saccharomyces. II. Anreicherung und Eigenschaften eines Malatenzyms. Arch. Mikrobiol. 89:223-231[Medline].
14.	Güldener, U., S. Heck, T. Fiedler, J. Beinhauer, and J. H. Hegemann. 1996. A new efficient gene disruption cassette for repeated use in budding yeast. Nucleic Acids Res. 24:2519-2524[Abstract/Free Full Text].
15.	Kuczynski, J. T., and F. Radler. 1982. The anaerobic metabolism of malate of Saccharomyces bailii and the partial purification of malic enzyme. Arch. Microbiol. 131:266-270[Medline].
16.	McNally, T., I. J. Purvis, L. A. Fothergill-Gilmore, and A. J. P. Brown. 1989. The yeast pyruvate kinase gene does not contain a string of non-preferred codons: revised nucleotide sequence. FEBS Lett. 247:312-316[Medline].
17.	Miller, J. H. 1972. In Experiments in molecular genetics. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
18.	Mumberg, D., R. Müller, and M. Funk. 1994. Regulatable promoters of Saccharomyces cerevisiae: comparison of transcriptional activity and their use for heterologous expression. Nucleic Acids Res. 22:5767-5788[Free Full Text].
19.	Polakis, E. S., and W. Bartley. 1965. Changes in the enzyme activities of Saccharomyces cerevisiae during aerobic growth on different carbon sources. Biochem. J. 97:284-297.
20.	Postma, E., C. Verduyn, W. A. Scheffers, and J. P. van Dijken. 1989. Enzymic analysis of the Crabtree effect in glucose-limited chemostat cultures of Saccharomyces cerevisiae. Appl. Environ. Microbiol. 53:468-477.
21.	Pronk, J. T., H. Y. Steensma, and J. P. van Dijken. 1996. Pyruvate metabolism in Saccharomyces cerevisiae. Yeast 12:1607-1633[Medline].
22.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. In Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
23.	Schmitt, M. E., T. A. Brown, and B. L. Trumpower. 1990. A rapid and simple method for preparation of RNA from Saccharomyces cerevisiae. Nucleic Acids Res. 18:3091-3092[Free Full Text].
24.	Schomburg, D., and D. Stephan. 1995. In Enzyme handbook, vol. 9. Class 1.1 oxidoreductases EC 1.1.1.1-EC 1.1.1.149. Springer Verlag, Berlin, Germany.
25.	Sherman, F. 1990. Guide to yeast genetics and molecular biology. Getting started with yeast. Methods Enzymol. 194:3-20.
26.	Stucka, R., S. Dequin, J. M. Salmon, and C. Gancedo. 1991. DNA sequences in chromosomes II and VII code for pyruvate carboxylase isoenzymes in Saccharomyces cerevisiae: analysis of pyruvate carboxylase-deficient strains. Mol. Gen. Genet. 229:307-315[Medline].
27.	Temperli, A., U. Künsch, K. Mayer, and I. Busch. 1965. Reinigung und Eigenschaften der Malatdehydrogenase (decarboxylierend) aus Hefe. Biochim. Biophys. Acta 110:630-632[Medline].
28.	Umbarger, H. E. 1978. Amino acid biosynthesis and its regulation. Annu. Rev. Biochem. 47:533-606.
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