A Transcriptional Switch in the Expression of Yeast Tricarboxylic Acid Cycle Genes in Response to a Reduction or Loss of Respiratory Function

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Molecular and Cellular Biology, October 1999, p. 6720-6728, Vol. 19, No. 10
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

A Transcriptional Switch in the Expression of Yeast Tricarboxylic Acid Cycle Genes in Response to a Reduction or Loss of Respiratory Function

Zhengchang Liu and Ronald A. Butow^*

Department of Molecular Biology, University of Texas Southwestern Medical Center, Dallas, Texas 75235-9148

Received 22 April 1999/Returned for modification 11 June 1999/Accepted 2 July 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Hap2,3,4,5p transcription complex is required for expression of many mitochondrial proteins that function in electrontransport and the tricarboxylic acid (TCA) cycle. We show thatas the cells' respiratory function is reduced or eliminated, theexpression of four TCA cycle genes, CIT1, ACO1, IDH1, and IDH2,switches from HAP control to control by three genes, RTG1, RTG2,and RTG3. The expression of four additional TCA cycle genes downstreamof IDH1 and IDH2 is independent of the RTG genes. We have previouslyshown that the RTG genes control the retrograde pathway, definedas a change in the expression of a subset of nuclear genes, e.g.,the glyoxylate cycle CIT2 gene, in response to changes in thefunctional state of mitochondria. We show that the cis-actingsequence controlling RTG-dependent expression of CIT1 includesan R box element, GTCAC, located 70 bp upstream of the Hap2,3,4,5pbinding site in the CIT1 upstream activation sequence. The R boxis a binding site for Rtg1p-Rtg3p, a heterodimeric, basic helix-loop-helix/leucinezipper transcription factor complex. We propose that in cellswith compromised mitochondrial function, the RTG genes take controlof the expression of genes leading to the synthesis of $alpha$ -ketoglutarateto ensure that sufficient glutamate is available for biosyntheticprocesses and that increased flux of the glyoxylate cycle, viaelevated CIT2 expression, provides a supply of metabolites enteringthe TCA cycle sufficient to support anabolic pathways. Glutamateis a potent repressor of RTG-dependent expression of genes encodingboth mitochondrial and nonmitochondrial proteins, suggesting thatit is a specific feedback regulator of the RTGsystem.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Cells reconfigure their pattern of gene expression to accommodate changes in nutrient availability. Often, this is seen asan induction of genes that enable cells to utilize certain nutrientsor as a repression of those genes when such nutrients are no longeravailable. Cells also reconfigure patterns of gene expressionin response to different stress conditions, for instance, heatshock or osmotic stresses, as a mechanism of protection againstthose environmental insults. In cells of the budding yeast Saccharomycescerevisiae, dramatic changes in gene expression are observed whencells switch from fermentative to oxidative metabolism, as inthe diauxic shift, when cells growing on glucose $---$ a repressingcarbon source $---$ begin to deplete the glucose from the medium (8).The expression of many nucleus-encoded mitochondrial proteins,such as components of the electron transport chain and enzymesof the tricarboxylic acid (TCA) cycle, become derepressed duringthe diauxic shift. The derepression of many of these proteinsrequires either Hap1p, an oxygen-sensing transcriptional activator(6, 29), the heteromeric Hap2,3,4,5p transcriptional complex(10, 11, 24, 26, 27, 30, 43), or both of these trans-actingregulators. Thus, the HAP system represents an important mechanismfor global control of expression of key components of respiratorymetabolism.

Yeast cells also modulate the expression of nuclear genes in response to mitochondrial dysfunctions (28). This interorganellesignaling pathway, called retrograde regulation, can be thoughtof as a stress response whose function is to accommodate variouscellular activities to the changes in the mitochondrial state(39). The best-studied example of the retrograde response isthat of the CIT2 gene, whose expression is sensitive to conditionsor mutations that compromise mitochondrial functions, such asinhibition of respiration, loss of TCA cycle activity, or lossof mitochondrial DNA (3, 18, 19). Recently, we found anew cytosolic D-lactate dehydrogenase activity encoded by a previouslyuncharacterized gene, YEL071w, now named DLD3, that shows a similarretrograde response as CIT2, namely, increased expression in cellswith dysfunctional mitochondria (4). CIT2 encodes a peroxisomalisoform of citrate synthase (CS2) that functions in the glyoxylatecycle; CS2 shares 75% sequence similarity with the mitochondrialcitrate synthase (CS1) encoded by the CIT1 gene, suggesting thatCIT1 and CIT2 arose by a duplication of some ancestral citratesynthase gene. In cells with compromised mitochondrial functions,for example, those without mitochondrial DNA ([rho⁰] petites), CIT2 expression is elevated by as much as 30- to 40-fold(19). Physiological studies suggest that this increase in CIT2expression facilitates a more efficient utilization of carbonvia the transfer of metabolites from the glyoxylate cycle to theTCA cycle (40). In contrast to CIT2, the level of CIT1 expressionis unaffected by the loss of mitochondrial DNA (18).

The expression of CIT2 and DLD3 is dependent under all conditions tested on three genes, RTG1, RTG2, and RTG3. RTG1 and RTG3encode basic helix-loop-helix/leucine zipper (bHLH/Zip) transcriptionfactors that bind as a heterodimer to activate transcription toa novel DNA target site, GTCAC, called an R box (14). CIT2 andDLD3 contain two R boxes in their 5' noncoding regions, both ofwhich are required for maximal gene expression. RTG2 encodes anovel cytoplasmic protein that has an amino-terminal ATP bindingdomain similar to the hsp70/actin/sugar kinase superfamily ofATP binding proteins (2). Rtg2p also shares some sequence similaritywith bacterial polyphosphatases and enzymes that hydrolyze guanosinetetra- and pentaphosphate (16). Although the precise functionof Rtg2p is unknown, genetic data suggest that it acts upstreamof Rtg1p and Rtg3p in the control of gene expression (36). TheCIT2-DLD3 retrograde response appears to be controlled by an Rtg2p-dependentredistribution of the Rtg1p-Rtg3p transcriptional complex froma predominantly cytoplasmic location in cells with robust mitochondrialfunction to a nuclear location in cells whose mitochondrial functionshave been compromised, such as in [rho⁰] petites (38).

None of the RTG genes are essential, nor are they required for growth of cells on some nonfermentable carbons sources. Althoughthe RTG genes are required for both basal and retrograde expressionof CIT2 and DLD3, two unexpected phenotypes of the rtg mutantswere observed: an inability of cells to grow on acetate, and agrowth requirement for glutamate and aspartate on minimal glucosemedium (18). These phenotypes are characteristic of cells withblocks in both the TCA and glyoxylate cycles. The inability togrow on acetate is a common phenotype of cells lacking TCA cycleenzymes (23), and cit1 cit2 and aco1 mutants are glutamate auxotrophs(12, 15). These observations suggest a potential defect inthe TCA cycle in rtg mutant cells. Biochemical experiments havesuggested that rtg mutant cells may have multiple and cumulativelesions in the TCA cycle that impair the cells' ability to growon acetate medium (40). Consistent with this conclusion, ithas been shown that RTG2 is required for expression of the ACO1gene in glucose-repressed cells (41).

Here we report that expression of the genes encoding the first three steps of the TCA cycle leading to the synthesis of $alpha$ -ketoglutarate,CIT1, ACO1, IDH1, and IDH2, switches between a dependence on theHAP genes in cells with robust mitochondrial function to the RTGgenes in cells whose mitochondrial respiratory capacity has beenreduced or eliminated. The remaining TCA cycle genes tested $---$ allof which encode enzymes catalyzing steps downstream of isocitratedehydrogenase $---$ have no dependence on the RTG genes for their expressionin either derepressed [rho⁺] (respiratory competent) wild-type cells or [rho⁰] petites. We analyze the control of CIT1 expression in detailand show that it contains a functional R box in the 5' flankingregion of the gene that is required for Rtg1p-Rtg3p-dependentexpression. We propose that the RTG control of genes encodingthe first three enzymes of the TCA cycle leading to the synthesisof $alpha$ -ketoglutarate is to ensure that sufficient glutamate is madefor biosynthetic processes in cells with reduced respiratory capacity.Finally, we show that glutamate is a potent repressor of RTG-dependentgene expression, suggesting an important feedback regulation ofglutamate synthesis. Like the HAP genes, which are responsiblefor a global control of gene expression in derepressed, respiratorycompetent cells, the RTG genes represent a major control pathwayof gene expression in cells with reduced or compromised mitochondrialfunction.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Growth media and growth conditions. Yeast strains were grown at 30°C in YP medium (1% yeast extract, 2% Bacto Peptone) with 2% raffinose (YPR) or 2 or 5% glucose(YPD or YP5%D, respectively); in YNB medium (0.67% yeast nitrogenbase) supplemented with 1% Casamino Acids, leucine (30 mg/liter),lysine (30 mg/liter), and 2 or 5% dextrose (YNBcasD or YNBcas5%D),2% raffinose (YNBcasR), 2% potassium acetate (YNBcasAce, pH adjustedto 5.5), or 2% glycerol (YNBcasGly); or in minimal YNB medium(0.67% yeast nitrogen base without Casamino Acids) supplementedwith leucine (30 mg/liter), lysine (30 mg/liter), uracil (20 mg/liter),and 2 or 5% glucose (YNBD or YNB5%D) or 2% raffinose (YNBR), withor without sodium glutamate (concentrations indicated in the textandfigures).

Strains. Yeast strains used in this study were PSY142 (MAT $alpha$ leu2 lys2 ura3 [rho⁺]) and its derivatives constructed as follows. To construct thertg1 $Delta$ derivative, a 674-bp HindIII-SstI fragment of RTG1 was replacedwith a 1.2-kb XhoI-HindIII fragment of the URA3 gene (18). Ura derivatives were obtained by selection with 5-fluro-orotic acid.An rtg2 $Delta$ derivative was constructed by replacing a SalI-XbaI fragmentof RTG2 with a 2.2-kb fragment of the LEU2 gene, thus deletingcodons 23 to 573 of RTG2 (37). To construct an rtg3 $Delta$ derivative,codons 175 to 340 of RTG3 were replaced with a 1.6-kb fragmentof the LEU2 gene (14). [rho⁰] derivatives of these strains were generated by several passagesof [rho⁺] cells in YPD medium supplemented with 25 µg of ethidium bromideper ml. The hap2 $Delta$ deletion was obtained by replacing bp +44 to+686 of the HAP2 gene with the kanMX4 cassette (42). The hap2 $Delta$ deletion was introduced into the wild-type and $Delta$ rtg1, $Delta$ rtg2, and $Delta$ rtg3 mutant strains. The cit1 $Delta$ and cit2 $Delta$ deletion mutants weredescribed previously (18, 19, 40).

Plasmid constructs. The DNA region from $-$ 806 to +9 of CIT1 was amplified by PCR. The forward primer contained a 5' EcoRI restriction site andreverse primer contained a 5' HindIII restriction site. The CIT1amplified product was inserted into the EcoRI-HindIII site ofYIp356 to produce pCIT1-LacZ. pCIT1-LacZ was linearized by digestionwith KpnI and integrated into the genomic CIT1 locus by standardyeast transformation procedures (32). The pACT1-LacZ plasmidwas constructed similarly by inserting the PCR-amplified DNA regionof ACT1 from $-$ 667 to +9 into the HindIII-EcoRI site of YIp356R.The pACT1-LacZ plasmid was linearized by digestion with NcoI andintegrated into the URA3 locus. The pCIT2-LacZ and pDLD3-LacZreporter gene constructs were described previously (4, 18).To make an R box mutant construct of pCIT1-LacZ, an internal pairof primers, 5'-gtacACGCGTTTTTTTCCGCCGCAG-3' and 5'-gtacACGCGTCGCCTTTTAGCACAAAAATG-3',(lowercase letters indicate plasmid sequence), was used to introducetwo point mutations into the R box, changing GTCAC to GACGC. Toconstruct pCIT1(UAS [upstream activation sequence])-CYC1-LacZand pCIT1(R)(UAS)-CYC1-LacZ, a pair of primers, 5'-gactaagcttTGTATTTACCTTGCATTT-3'and 5'-gactctcgagGGAAAAGCTCCAAAGGG-3', (underlining indicatesrestriction sites), was used to amplify the $-$ 400 to $-$ 260 regionof CIT1 in pCIT1-LacZ and pCIT1(R)-LacZ, respectively. The resultingamplified products were cleaved by HindIII and XhoI and insertedinto the multiple cloning region of pWCJ100, which contains theminimal promoter of CYC1 fused to lacI-lacZ coding sequence. PlasmidpWCJ100 is a centromere-based vector derived from pKM270. pACT1-CIT1was constructed by fusing the ACT1 region from $-$ 457 to $-$ 152 tothe CIT1 region from $-$ 170 to +1990 in plasmid YIp352. pACT1-CIT1was linearized by digestion with ApaI and integrated into theURA3locus.

Electrophoretic mobility shift assay (EMSA). Whole-cell extracts were prepared as described previously (18) except that [rho⁰] cells were used. Cells were grown in YNB5%D medium containingthe necessary nutritional supplements and including 0.01% glutamicacid. A 140-bp DNA sequence from $-$ 400 to $-$ 260 of the CIT1 geneamplified by PCR was used as a probe. The resulting PCR productwas gel purified and end labeled with [ $gamma$ -³²P]ATP by using T4 polynucleotide kinase. The reaction mixturecontained 25 mM Tris-HCl (pH 7.5), 5 mM MgCl, 0.125 mM EDTA, 300mM KCl, 10% glycerol, 0.5 mM dithiothreitol, 0.5 mM phenylmethylsulfonylfluoride, 0.5 µg of aprotinin per ml, 0.5 µg of leupeptin perml, 1 ng of ³²P-labeled probe, 1 µg of salmon sperm DNA, and 40 µg of cell extractin a final volume of 20 µl. After 20 min of incubation at roomtemperature, the reaction mixture was applied to a 4% acrylamidegel (40:1 in 0.5× Tris-borate-EDTA buffer) prerun for 30 min andthen run for 2.3 h at 4°C. The gel was dried and exposed to X-rayfilm.

Yeast transformation and $beta$ -galactosidase assays. Yeast cells were transformed as described by Chen et al. (5). Transformants carrying the desired plasmids were selectedon YNBcasD plates. Liquid precultures were inoculated with a poolof several independent transformants and grown in YNBcasD medium.Cells were collected by centrifugation and diluted into YNBcas5%Dor into YNBcasR medium and grown overnight to an optical densityat 600 nm of ~2.0. Cells were collected by centrifugation, dilutedinto corresponding fresh medium, and collected at an optical densityat 600 nm of ~0.8 after 9 h growth at 30°C. For glutamate repressionanalysis, YNB5%D and YNBR media were used. The preparation ofcell extracts and $beta$ -galactosidase assays were carried out as describedby Rose et al. (33). For each plasmid-strain combination, assayswere conducted in triplicate and independent experiments werecarried out two to threetimes.

RNA isolation and Northern blot analysis. Total yeast RNA was isolated from 50- to 200-ml logarithmic-phase cultures, fractionated on 1.2% agarose gels, transferredto Nytran Plus, and hybridized at 65°C with probes specific fortranscripts of the CIT2 and ACT1 genes as previously described(14). The region from +263 to +1344 of CIT1 was purified bycleaving a plasmid containing that sequence with ClaI and StuIand used as probe for CIT1 transcripts. The remaining probes werePCR amplified from selected coding regions of the genes of interest,using genomic DNA as a template. The PCR products were gel purifiedby using a GenecleanII kit from Bio 101 (Vista, Calif.). The regionsamplified were $-$ 380 to +2855 of ACO1, $-$ 54 to +1237 of IDH1, $-$ 53to +1279 of IDH2, $-$ 59 to +3226 of KGD1, $-$ 126 to +2171 of SDH1,and $-$ 63 to +1660 of FUM1. Hybridization signals were quantifiedwith a Molecular DynamicsPhosphorImager.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Alternative dependence of expression of a CIT1-lacZ reporter gene on HAP2 and RTG1, RTG2, and RTG3. To examine the role of the RTG genes in TCA cycle gene expression, we first investigated the regulation of CIT1 expressionby using a reporter gene construct in which 806 bp of the 5' flankingregion of CIT1 was fused to the Escherichia coli lacZ gene. Thisconstruct was integrated into the CIT1 locus of wild-type PSY142[rho⁺] and [rho⁰] cells and into a hap2 $Delta$ and rtg1 $Delta$ , rtg2 $Delta$ , or rtg3 $Delta$ mutant derivativesof these strains. In agreement with the findings of Rosenkrantzet al. (34), the CIT1-lacZ reporter gene construct fully recapitulatedthe known glucose repression of the native CIT1 gene, with morethan a 15-fold decrease in $beta$ -galactosidase activity in extractsfrom [rho⁺] cells grown on glucose compared with extracts from cells grownon raffinose, a nonrepressing carbon source (Fig. 1A and B). Reportergene activity in [rho⁺] rtg $Delta$ cells was inhibited only modestly (25 to 50%) when thosecells were grown on raffinose but was very strongly inhibitedwhen those cells were grown on glucose. In derepressed [rho⁺] cells, the hap2 $Delta$ mutation nearly abolished CIT1 reporter geneexpression; however, in glucose-repressed [rho⁺] cells, significantly more reporter gene activity remained inthe hap2 $Delta$ background. Finally, in [rho⁺] cells grown on either raffinose or glucose, reporter gene activitywas essentially eliminated in the hap2 $Delta$ rtg $Delta$ double mutants. Theseresults are fully consistent with the known requirement of theHap2,3,4,5p complex for derepressed expression of the CIT1 gene(34).

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FIG. 1. Alternative dependence of CIT1 expression on RTG1, RTG2, RTG3, and HAP2. $beta$ -Galactosidase assays were carried out to determine the activity of a CIT1-lacZ reporter gene in wild-type (WT) PSY142 [rho⁺] and [rho⁰] cells and various mutant derivatives of these strains as indicated. The bp $-$ 806 to +9 region of the CIT1 gene was fused to the coding region of the E. coli lacZ gene, and the resulting construct was integrated at the chromosomal CIT1 locus. For each strain grown on either raffinose (YPR) or glucose (YP5%D) medium, four independent transformants were pooled from mid-log-phase cultures and $beta$ -galactosidase assays on whole-cell extracts were carried out in triplicate as described in Materials and Methods.

In contrast to these results, reporter gene expression was completely dependent on the RTG genes in [rho⁰] petite cells, whether those petites were grown on raffinoseor glucose (Fig. 1C and D). Although expression in [rho⁰] cells still showed some dependence on HAP2 when cells were grownon raffinose, HAP2 was not required for expression in glucose-grownpetite cells. Finally, as in [rho⁺] cells, expression of the CIT1-lacZ reporter gene was eliminatedin the rtg $Delta$ hap2 $Delta$ double mutants. We conclude from these resultsthat the CIT1-lacZ expression is largely dependent on the HAPsystem in cells with robust mitochondrial respiratory functionbut switches to a synergistic dependence on the RTG and HAP systemswhen respiratory function is reduced, as in glucose-repressed[rho⁺] cells, or eliminated, as in [rho⁰] petites. In the most severe case of reduced mitochondrial function $---$ [rho⁰] cells grown on glucose $---$ CIT1 expression is independent of theHAPsystem.

Glutamate auxotrophy. Previous studies showed that rtg mutant [rho⁺] cells grown on minimal glucose medium were glutamate auxotrophs (18). Glutamateauxotrophy could arise from a block in the synthesis of $alpha$ -ketoglutarate,the direct precursor of glutamic acid. The finding that CIT1-lacZexpression was largely independent of the RTG genes in [rho⁺] cells grown on raffinose, but was strongly dependent on thosegenes in cells grown on glucose, raised the possibility that rtgmutant [rho⁺] cells do not require glutamate for growth on minimal raffinosemedium. We therefore compared the glutamate requirements for growthof wild-type [rho⁺] and [rho⁰] cells and their rtg $Delta$ mutant derivatives on minimal raffinoseor glucose medium. Figure 2A and Fig. 2B show that the rtg $Delta$ mutant[rho⁰] cells, in which CIT1-lacZ expression was strongly dependenton the RTG genes, were glutamate auxotrophs when grown on minimalraffinose medium. By contrast, the various rtg $Delta$ [rho⁺] mutant cells, in which CIT1-lacZ expression is largely independentof the RTG genes, were glutamate prototrophs on minimal raffinosemedium. On minimal glucose medium, both the [rho⁰] and [rho⁺] rtg $Delta$ mutant strains were glutamate auxotrophs (Fig. 2C and D),again consistent with the nearly complete dependence of CIT1-lacZexpression in those cells on the RTG genes.

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FIG. 2. Glutamate auxotrophy of rtg mutant cells coincides with RTG-dependent gene expression. Wild-type (WT) PSY142 [rho⁺] and [rho⁰] cells and rtg1 $Delta$ , rtg2 $Delta$ or rtg3 $Delta$ mutant derivatives of those strains were streaked on YNBR or YNBD medium with or without 0.02% glutamate. (A) YNBR plus glutamate; (B) YNBR alone; (C) YNBD plus glutamate; (D) YNBD. Only the [rho⁰] mutant derivatives are glutamate auxotrophs in derepressed cells, whereas both [rho⁺] and [rho⁰] mutant derivatives are glutamate auxotrophs in glucose-repressed cells.

The CIT1 UAS contains a functional R box. A 10-bp DNA segment of CIT1 from $-$ 367 to $-$ 358 has been shown to be important for glucose-repressed expression of the gene(34, 35). Notably, that 10-bp segment starts with GTCAC, anR box binding site for the Rtg1p-Rtg3p heterodimeric complex (14).To determine whether this R box confers the RTG-dependent expressionof CIT1, we first constructed a CIT1-lacZ reporter gene in whicha 140-bp fragment from $-$ 400 to $-$ 260 of the upstream region ofCIT1 containing both the R box site and the Hap2,3,4,5p bindingsite, CCAAT, was fused to a CYC1 transcriptional start site linkedto lacZ (Fig. 3A). The resultant CIT1 UAS-CYC1-lacZ constructin a centromere plasmid was transformed into [rho⁺] and [rho⁰] cells and into rtg3 $Delta$ , hap2 $Delta$ , and rtg3 $Delta$ hap2 $Delta$ double-mutant derivativesof those strains. This reporter gene mimicked the profile of expressionof the $-$ 806 bp CIT1-lacZ reporter gene: it was subject to glucoserepression; expression was dependent on RTG3 in [rho⁺] and [rho⁰] cells grown on glucose medium; and expression was dependentboth on HAP2 and on RTG3 in [rho⁰] cells grown on raffinose medium (Fig. 3B).

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FIG. 3. A functional R box in the CIT1 UAS. (A) Diagram of a CIT1 UAS-CYC1-lacZ construct in which a 140-bp fragment of the upstream region of CIT1 from bp $-$ 400 to $-$ 260 was fused to the transcriptional start site of the CYC1 gene and fused to the reading frame of the E. coli lacZ gene. Positions of the putative Rtg1p-Rtg3p R box binding site, GTCAC, and the Hap2,3,4,5p binding site, ATTGG, are indicated. (B) Wild-type (WT) PSY142 [rho⁺] and [rho⁰] cells and rtg3 $Delta$ , hap2 $Delta$ , and rtg3 $Delta$ hap2 $Delta$ derivatives were transformed with the CIT1 UAS-CYC1-lacZ construct in a centromeric plasmid. Pools of 10 transformants of each were grown to mid-log phase on YNBcasR or YNBcas5%D medium, and $beta$ -galactosidase activity was determined in cell-free extracts. (C) Two mutations were introduced into the R box in the CIT1 UAS-CYC1-lacZ construct as indicated in boldface and described in Materials and Methods. This construct was placed into a centromeric plasmid to yield pCIT1(R)(UAS)-CYC1-LacZ. (D) PSY142 [rho⁺] and [rho⁰] cells were transformed either with pCIT1(UAS)-CYC1-LacZ, containing the wild-type R box, or with pCIT1(R)(UAS)-CYC1-LacZ, containing the mutant R box construct. Ten transformants of each were pooled and grown to mid-log phase in YNBcasR or YNBcas5%D medium, and $beta$ -galactosidase activities were measured in cell-free extracts. Standard errors from triplicate assays are <10%.

To determine whether the R box site is important for RTG1,3-dependent expression, two mutations were introduced into the Rbox of the CIT1 UAS-CYC1-lacZ wild-type reporter construct (Fig.3C), and the effects of those mutations were analyzed in [rho⁺] and [rho⁰] cells grown on raffinose or glucose medium. In [rho⁺] cells grown on raffinose, the R box mutations reduced reportergene expression less than threefold (Fig. 3D), whereas expressionwas reduced more than sixfold in [rho⁰] cells grown on raffinose, and nearly ninefold in [rho⁰] cells grown on glucose. These results suggest that the R boxin the CIT1 UAS is an important cis-acting element for expressionof CIT1, particularly in glucose-repressed [rho⁰] cells in which mitochondrial function is most severely affected.These results are consistent with the differential dependenceof CIT1 expression on RTG3 in [rho⁺] and [rho⁰] cells grown on repressing versus nonrepressing carbonsources.

To determine whether the Rtg1p-Rtg3p complex binds to the CIT1 UAS, the 140-bp DNA fragment containing the R box was usedas a probe in EMSAs with extracts from wild-type [rho⁺] and rtg $Delta$ mutant strains. With extracts from wild-type cells,two bands were detected by EMSA (Fig. 4, lane 2). However, whenextracts from rtg1 $Delta$ or rtg3 $Delta$ strains were used, the fainter, lowerband disappeared (Fig. 4, lanes 3 and 5). The faster-migratingband was still present when an extract from a rtg2 $Delta$ strain wasused (Fig. 4, lane 4). This result is consistent with those ofprevious EMSAs with a CIT2 UAS_r probe showing that Rtg2p is notrequired for the binding of the Rtg1p-Rtg3p complex to R box sites(14, 18) and that Rtg2p is a cytoplasmic protein (38). Collectively,these data strongly suggest that the Rtg1p-Rtg3p complex regulatesCIT1 expression through interaction with the CIT1 R box.

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FIG. 4. The Rtg1p-Rtg3p complex binds to the CIT1 UAS. Whole-cell extracts were prepared from wild-type (wt) [rho⁺] PSY142 cells and from rtg1 $Delta$ , rtg2 $Delta$ , and rtg3 $Delta$ derivatives grown on YNB5%D medium supplemented with 0.01% glutamate. EMSA was carried out with a [ $gamma$ -³²P]ATP-labeled 140-bp DNA probe of the CIT1 UAS as described in Materials and Methods. The control lane 1 is the probe alone. The arrow indicates the gel-retarded band whose presence is dependent on Rtg1p and Rtg3p.

Glutamate represses RTG gene functions. Glutamate is a negative regulator of CIT1 expression in glucose-repressed cells (15, 35). ACO1, whose expression requiresRtg2p in glucose-repressed cells (41), is also subject to glutamaterepression (12). These observations raise the possibility thatglutamate repression of CIT1 expression is correlated with CIT1'sdependence on the RTG genes in glucose-repressed or respiratorydeficient cells. To test this, we examined the effect of additionof glutamate to the growth medium on the expression of the $-$ 806CIT1-lacZ reporter gene in [rho⁺] and [rho⁰] cells grown in medium with raffinose or glucose as the carbonsource. In [rho⁺] cells grown on raffinose, the addition of 0.01 or 0.2% glutamateto the medium resulted in only a partial inhibition of reportergene expression (Fig. 5A), comparable to the inhibitory effectof the rtg $Delta$ mutations in derepressed [rho⁺] cells (Fig. 1). In contrast to these results, glutamate wasa potent inhibitor of reporter gene expression in [rho⁺] and [rho⁰] cells grown on glucose and was slightly less effective as aninhibitor in [rho⁰] cells grown on raffinose. Similar patterns of repression byglutamate were observed when we used a CIT1 reporter gene containingthe 140-bp CIT1 UAS (data not shown). These findings support theconclusion that glutamate is a repressor of RTG-dependent CIT1expression.

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FIG. 5. Glutamate is a repressor of RTG-dependent gene expression. (A) PSY 142 [rho⁺] and [rho⁰] strains with an integrated copy of the $-$ 806 CIT1-lacZ reporter gene and an rtg1 $Delta$ derivative of those strains were grown in YNBR or YNB5%D medium as controls. Parallel cultures contained glutamate in the medium at the indicated concentrations. Whole-cell extracts were prepared, and $beta$ -galactosidase activities were determined. Data are expressed as $beta$ -galactosidase activities normalized to the value for the wild-type (WT) grown in the absence of glutamate. (B) Same as panel A except that wild-type [rho⁺] and [rho⁰] strains lacked the CIT1 reporter gene and instead were transformed with centromere-based plasmids containing a CIT2-lacZ reporter gene (18) or a DLD3 reporter gene in which the bp $-$ 500 region of DLD3 was fused to lacZ (4).

The RTG genes are required for the expression the CIT2 and DLD3 genes in all strains and carbon sources that we have tested.If glutamate is a general negative regulator of RTG-dependentgene expression, then CIT2 and DLD3 expression should also besensitive to glutamate repression independent of carbon sourceand the functional state of mitochondria. To test this, CIT2-LacZand DLD3-lacZ reporter genes were introduced into [rho⁺] and [rho⁰] cells, which were then grown on either raffinose or glucose.Expression of both CIT2-lacZ and DLD3-lacZ was repressed by glutamatein the medium, and the extent of repression was independent ofcarbon source or the functional state of mitochondria (Fig. 5B).As a control, lacZ expression was placed under the control ofthe constitutive ACT1 promoter, but expression of that fusiongene was not repressed by glutamate (data not shown). We concludefrom these experiments that glutamate is a general repressor ofRTG-dependent geneexpression.

Constitutive expression of CIT1 cannot rescue the phenotypes of RTG deletion mutants. Although the RTG genes are essential for CIT2 expression, a cit2 $Delta$ mutant, unlike an rtg $Delta$ mutant, is not a glutamate auxotroph,whereas the cit1 $Delta$ cit2 $Delta$ double mutant requires glutamate for growth(15). Given the finding that CIT1 expression becomes dependenton the RTG genes in glucose-repressed or respiratory activity-deficientcells, we examined whether constitutive expression of CIT1 wouldrescue the glutamate auxotrophy of rtg $Delta$ mutant cells or theirinability to grow on acetate medium. To these ends, we constructeda fusion gene in which CIT1 expression was placed under the controlof the constitutive promoter of the ACT1 gene. The resulting plasmid,pACT1-CIT1, was transformed into a cit1 $Delta$ [rho⁺] strain and into rtg $Delta$ mutant derivatives of the wild-type [rho⁺] strain. Controls included cells transformed with the vectoralone, as well as a cit2 $Delta$ mutant strain. We then determined theability of these strains to grow on YNBcasAce medium and on YNBDmedium with or without glutamate supplementation. The constitutiveexpression of CIT1 from pACT1-CIT1 was not able to restore glutamateauxotrophy to any of the rtg $Delta$ mutant strains (Fig. 6A and B).Although all of these strains are respiratory competent, sincethey were able to grow on medium with glycerol as the sole carbonsource (Fig. 6C), the ACT1-CIT1 fusion gene restored growth tothe cit1 $Delta$ mutant cells only when cells were grown on acetate medium(Fig. 6D). These data suggest that first, CIT1 could be expressedfrom the ACT1-CIT1 fusion gene sufficiently to restore acetategrowth to a cit1 $Delta$ mutant, and second, the reduction in CIT1 andCIT2 expression in rtg $Delta$ mutant cells is not solely responsiblefor their glutamate auxotrophy or inability of those cells togrow on acetate medium. Thus, other defects in the TCA cycle arelikely to exist in these mutants.

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FIG. 6. Constitutive expression of CIT1 fails to rescue the glutamate auxotrophy and acetate phenotypes of rtg mutant cells. Wild-type (WT) PSY142 [rho⁺] cells and cit1 $Delta$ , cit2 $Delta$ , rtg1 $Delta$ , rtg2 $Delta$ , or rtg3 $Delta$ derivatives were transformed with a centromere-based plasmid, pACT1-CIT1, in which CIT1 expression was placed under the control of the constitutive ACT1 promoter. As controls, these strains were also transformed with pRS416 alone. Cells were streaked on YNBD-0.02% glutamate (A), YNBD (B), YNBcasGly (C) or YNBcasAce (D) medium and grown for 2.5 to 3.5 days at 30°.

Expression of CIT1, ACO1, IDH1, and IDH2 requires the RTG genes in cells with dysfunctional mitochondria. To investigate further the relation between the RTG genes and expression of TCA cycle genes, we carried out Northern blotanalysis to examine the relative expression of eight genes encodingproteins that function in the TCA cycle: CIT1, ACO1, IDH1, IDH2,KGD1, SDH1, FUM1, and MDH1. The transcript levels of these genes,normalized to the level of ACT1 mRNA, were compared in [rho⁺] and [rho⁰] wild-type cells and in rtg1 $Delta$ , rtg2 $Delta$ , and rtg3 $Delta$ mutant derivativesof these strains grown in YPR medium. As a control, we also probedfor CIT2 transcripts, whose behavior has previously been wellcharacterized in those strains. Only the CIT2 gene showed a strongdependence on the RTG genes for expression in both [rho⁺] and [rho⁰] cells (Fig. 7). However, four of the TCA cycle genes, CIT1,ACO1, IDH1, and IDH2, which encode proteins catalyzing the firstthree steps of the TCA cycle from oxaloacetate to $alpha$ -ketoglutarate,showed a dramatic dependence on the RTG genes for their expressionin [rho⁰] cells, but not in [rho⁺] cells. In sharp contrast to the elevated expression of CIT2in [rho⁰] cells, the transcript levels of these first four TCA cycle geneswere about the same in [rho⁰] and [rho⁺] cells. Expression of the remaining TCA cycle genes tested, KGD1,SDH1, FUM1, and MDH1, was essentially unaffected by the rtg $Delta$ mutations,and their expression in the wild-type [rho⁰] strain was significantly less than in [rho⁺] cells. Two transcripts that behaved identically were detectedwith the SDH1 probe. The origin of these two transcripts has notbeen investigated further. The HAP genes are known to be requiredfor expression of KGD1, SDH1, FUM1, and MDH1 in derepressed [rho⁺] cells (7, 12, 22, 31). Their reduced expression inderepressed [rho⁰] cells provides the first indication to our knowledge that HAPfunctionality is reduced in derepressed, respiratory activity-deficientcells. From these experiments, we conclude that the expressionof genes encoding proteins that function in the first three stepsof the TCA cycle are under dual HAP-RTG control.

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FIG. 7. Northern blot analysis of TCA cycle gene expression. Total RNA was prepared from PSY142 [rho⁺] and [rho⁰] wild-type (WT) strains and their rtg1 $Delta$ , rtg2 $Delta$ , and rtg3 $Delta$ derivatives grown to mid-log phase on YPR medium. Blots were probed for each of the indicated genes as described in Materials and Methods. RNA loads were normalized to the level of transcripts of the ACT1 gene. CIT2 transcripts were also analyzed as a control.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In an analysis of the cis-acting elements controlling expression of the mitochondrial citrate synthase gene, CIT1, Rosenkrantzet al. (34, 35) concluded that there were distinct upstreamactivation regions required for glucose-repressed and derepressedexpression of the gene. In particular, the region from $-$ 367 to $-$ 348 was necessary for glucose-repressed expression, whereas theregion from $-$ 291 and $-$ 273 was necessary for expression in derepressedcells. The latter is clearly identified as the HAP control region:it contains a consensus Hap2,3,4,5p binding site whose integrityis necessary for CIT1 expression in derepressed cells, consistentwith the known functionality of the Hap complex in cells withrobust respiratoryactivity.

In the present study, we have shown that expression of CIT1 becomes increasingly dependent on the RTG genes as mitochondrialrespiratory function is reduced. The upstream region of CIT1 identifiedby Rosenkrantz et al. (34, 35) as being necessary for glucose-repressedexpression contains a single R box, GTCAC, which we have shownfor the CIT2 and DLD3 genes is a binding site for the Rtg1p-Rtg3p,bHLH/Zip complex (4, 14). CIT2 and DLD3 each contain twoclosely spaced R boxes (in inverted orientation), both of whichare necessary for maximal gene expression. Mutation of the singleR box in the upstream region of CIT1 shows that the R box is mostimportant for CIT1 expression in glucose-repressed cells, consistentwith CIT1's strong dependence on the RTG genes for its expressionunder glucose-repressed conditions. Together with the EMSAs showingthat the Rtg1p-Rtg3p bind to a DNA probe containing the CIT1 Rbox, these findings provide strong support for the conclusionthat the RTG genes play an important role in the regulation ofCIT1 expression under conditions where HAP-dependent expressiondecreases.

We extended this dual HAP-RTG control of gene expression to include ACO1, IDH1, and IDH2. Velot et al. (41) reported thatACO1 expression required RTG2 specifically in glucose-repressedcells. Our studies confirm this finding and extend the controlof ACO1 expression as well as expression of the above-mentionedgenes to include RTG1 and RTG3. It was essential to test whetherexpression required all three of the RTG genes, because we donot yet know whether RTG2 affects gene expression in pathwaysnot involving RTG1 or RTG3. We have inspected the 5' flankingregions of ACO1, IDH1, and IDH2 to see whether they contain Rbox sites. ACO1 has two R boxes at $-$ 772 and $-$ 450. IDH1 containsthree R boxes at $-$ 355, $-$ 476, and $-$ 576, but the only consensusR box for IDH2 evident from the database is one far upstream at $-$ 768. The functionality of these putative Rtg1p-Rtg3p bindingsites and whether potential degenerate R box sites can serve asbinding sites for Rtg1p-Rtg3p will have to be determined on agene-by-gene basis. Finally, we found that expression of all ofthe other TCA cycle genes tested that encode proteins catalyzingsteps of the cycle downstream of IDH1 and IDH2 was independentof the RTG genes in respiratory activity-deficient cells. Collectively,our findings show that the expression of genes encoding the firstthree steps of the TCA cycle from oxaloacetate to $alpha$ -ketoglutaratecome under increasing control of the RTG regulatory pathway asmitochondrial respiratory capacity is reduced. In this way, expressionof those genes can be maintained to compensate for the loss ofHAP genecontrol.

To evaluate the effects of the functional state of mitochondria on TCA cycle gene expression, it is worth emphasizing thatthe combination of strains and growth conditions that we chosehave provided cells with a graded range of mitochondrial functions,from those with robust respiratory activity in derepressed [rho⁺] cells to those with severely debilitated mitochondrial functionin glucose-repressed [rho⁰] cells. The striking observation was that the dependence of CIT1expression on the HAP and RTG genes followed this graded rangeof mitochondrial function: at the extremes, expression was largelyHAP or RTG dependent, whereas in the middle, expression showeda synergistic dependence on the two systems. Although we do notknow the precise details of how the control of expression of theseTCA cycle genes is handed off from largely HAP-dependent expressionin derepressed [rho⁺] cells to RTG-dependent expression in glucose-repressed [rho⁰] petites, it is not likely to be as a result of modulation ofthe level of the RTG gene products, since they are expressed constitutivelyin all cases that we have examined (14, 36, 37). Indeed,the RTG pathway appears to be controlled by an Rtg2p-dependentregulation of the nuclear localization of Rtg1p and Rtg3p (38).There is evidence that some of the components of the HAP complexare induced in cells growing on nonfermentable carbon sources,but how HAP activity is tied to the functional state of mitochondriais lessclear.

The retrograde response versus RTG control of TCA cycle gene expression. Our previous analysis of the CIT2 and DLD3 genes showed that their expression required the RTG genes, independent of the cell'srespiratory state or the carbon source in the growth medium (4,18, 19). A characteristic feature of CIT2 and DLD3 expressionis their retrograde response, namely, a sharply elevated levelof expression in cells with dysfunctional mitochondria. Basedon the present findings, we can define two new patterns of generegulation related to the mitochondrial state that apply to TCAcycle genes. The first is a dual dependence on the HAP and RTGgenes, with an increasing reliance on the RTG genes for expressionin cells whose mitochondrial respiratory function is reduced oreliminated. The overall levels of expression for those genes,CIT1, ACO1, IDH1, and IDH2, in contrast to retrograde responsegenes, are roughly the same in derepressed [rho⁺] and [rho⁰] cells. This combinatorial control between the HAP and RTG genesrepresents a heretofore unrecognized strategy by which cells regulategene expression in response to carbon source and to changes inthe functional state of mitochondria. The second pattern of controlwas evident from our Northern blot data showing that expressionof TCA cycle genes functioning downstream of $alpha$ -ketoglutarate,KGD1, SDH1, FUM1, and MDH1, are all down-regulated in [rho⁰]petites.

We can consider three general pathways used by yeast cells to modulate expression of genes related to mitochondrial oxidativemetabolism. The first is responsive to carbon source and is controlledby the Hap2,3,4,5p complex (10, 11, 24, 26, 27, 30,43). Second are the oxygen-sensing pathways exemplified by controlvia the positive regulator, Hap1p (6, 29), and the negativeregulator, Rox1p, a heme-dependent repressor of hypoxic genes(20, 21, 44). Hap1p is a transcriptional activator that,together with heme, responds to oxygen levels to regulate expressionof an assortment of genes that function in electron transport,oxidative stress, and heme, sterol, and unsaturated fatty acidbiosynthesis (reviewed by Kwast et al. [17]). The RTG genescan now be included as an additional pathway of gene regulationthat monitors the functional state of mitochondria. As mitochondrialrespiratory functions are compromised, the RTG system takes overresponsibility for expression of some, otherwise HAP-dependentgenes as described here and elevates the expression of other genessuch as CIT2 (19) to compensate for the mitochondrialdefects.

A central role for glutamate. A number of previous studies had shown that glutamate is an inhibitor of expression of some TCA cycle genes as well as CIT2(13, 15, 35, 41), but the regulatory targets affectedby glutamate were unknown. It is now clear that glutamate inhibitionoccurs via RTG-dependent gene expression, which we suggest isa reflection of a negative feedback loop that regulates glutamatelevels in cells with compromised mitochondrial function. In yeast,there are three known pathways for glutamate synthesis (1,9, 25): two glutamic dehydrogenase isozymes encoded by GDH1and GDH3 and glutamine synthetase encoded by GLT1. All three pathwaysuse $alpha$ -ketoglutarate as a common precursor of glutamate, whichitself is a precursor for the synthesis of other amino acids andnucleotides. As illustrated in the model shown in Fig. 8, theRTG pathway could be activated to ensure that (i) there is sufficientsynthesis of $alpha$ -ketoglutarate for glutamate synthesis when theHAP system is downregulated, as in respiratory deficient cells,and (ii) anaplerotic pathways and gluconeogenesis are adequatelymaintained as a result of increased supply of intermediates tothe TCA cycle, particularly succinate, from the glyoxylate cycle.The dramatic increase in CIT2 expression in respiratory activity-deficientcells could effectively increase the flux of carbon through theglyoxylate cycle to provide the net carbon needed for anabolicpathways.

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FIG. 8. Model for the role of the RTG genes in the control of expression of TCA and glyoxylate cycle genes. As mitochondrial function decreases (shaded triangle), the expression of CIT1, ACO1, IDH1, and IDH2 becomes increasingly dependent on the RTG genes and less dependent on the HAP genes. Glutamate is shown as a feedback regulator of RTG-dependent pathways of gene expression. $alpha$ -KG, $alpha$ -ketoglutarate.

Glutamate appears to be a key player in the RTG pathways. When supplemented in the growth medium, glutamate is a potent repressorof RTG-dependent gene expression, suggesting that if the RTG pathwayindeed functions to maintain adequate levels of $alpha$ -ketoglutaratefor glutamate biosynthesis, it is subject to a strong glutamatefeedback loop via transcriptional control, where expression ofgenes encoding the first three enzymes of the TCA cycle that leadto the synthesis of $alpha$ -ketoglutarate are repressed by glutamate.Considering the findings to date, we are inclined to speculatethat the intracellular level of glutamate or its direct precursor $alpha$ -ketoglutarate might be a key signal for regulation of the RTG-dependentpathways.

	ACKNOWLEDGMENTS

We thank A. Chelstowska for providing the pACT1-LacZ construct, and we thank C. Epstein for providing primers to generateprobes for TCA cycle genes and for a critical reading of the manuscript.We also thank members of the Butow laboratory for helpfuldiscussions.

This work was supported by grants from the National Institutes of Health (GM22525) and from The Robert A. Welch Foundation(I-0642).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Biology, University of Texas Southwestern Medical Center, 5323Harry Hines Blvd., Dallas, TX 75235-9148. Phone: (214) 648-1465.Fax: (214) 648-1488. E-mail: butow{at}swmed.edu.

This paper is dedicated to our friend and colleague, PaulSrere.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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