Molecular Cloning and Functional Expression of Alternative Oxidase from Candida albicans

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Journal of Bacteriology, July 1999, p. 4098-4102, Vol. 181, No. 13
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Molecular Cloning and Functional Expression of Alternative Oxidase from Candida albicans

Won-Ki Huh and Sa-Ouk Kang^*

Laboratory of Biophysics, Department of Microbiology, College of Natural Sciences, and Research Center for Molecular Microbiology, Seoul National University, Seoul 151-742, Republic of Korea

Received 29 December 1998/Accepted 18 April 1999

	ABSTRACT

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The AOX1 gene, which encodes an alternative oxidase, was isolated from the genomic DNA library of Candida albicans. The geneencodes a polypeptide consisting of 379 amino acids with a calculatedmolecular mass of 43,975 Da. The aox1/aox1 mutant strain did notshow cyanide-resistant respiration under normal conditions butcould still induce cyanide-resistant respiration when treatedwith antimycin A. The measurement of respiratory activity andWestern blot analysis suggested the presence of another AOX. WhenC. albicans AOX1 was expressed in alternative oxidase-deficientSaccharomyces cerevisiae, it could confer cyanide-resistant respirationon S. cerevisiae.

	TEXT

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In addition to the cytochrome-involved respiratory pathway, higher plants (11), protists (6), and fungi (17, 22)are known to possess an alternative, cyanide-resistant respiratorypathway, which is specifically inhibited by hydroxamic acids (27).Cyanide-resistant respiration appears to be mediated by alternativeoxidase (AOX), which is believed to accept electrons from theubiquinone pool of the main cytochrome pathway and to reduce oxygento water (2). The detailed nature and the physiological rolesof the alternative respiratory pathway mediated by AOX are stillpoorly understood. Cyanide-resistant respiration has been shownto be involved in thermogenic inflorescence (21), climactericand ripening of fruits (15), and cell-type proportioning duringDictyostelium development (19). Some reports show that reactiveoxygen species, such as superoxide radical anion or hydrogen peroxide,induce the expression of AOX (23, 32). These observationssuggest that cyanide-resistant respiration is related to defensesystems against oxidativestress.

In the dimorphic fungus Candida albicans, the existence of cyanide-resistant respiration has been previously reported (1,28). However, the process by which the alternative respiratorypathway appears in this fungus is still controversial. As a firststep to investigate the nature and the physiological roles ofcyanide-resistant respiration in C. albicans, we isolated theAOX1 gene, which encodes an AOX, and report here the effects ofdisruption and overexpression of the AOX1 gene in C. albicans.We also report the functional expression of the C. albicans AOX1gene in Saccharomyces cerevisiae.

Yeast strains and media. The C. albicans and S. cerevisiae strains used in this study are listed in Table 1. For routine growth of cells, YPD medium(1% yeast extract, 2% peptone, 2% glucose) was used. The cellscontaining plasmids or disrupted genes were cultured in syntheticdextrose (SD) minimal medium with the appropriate supplement (29).Ura auxotrophs were selected on SD minimal medium supplemented with625 mg of 5-fluoroorotic acid and 30 mg of uridine per liter (FOAmedium).

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TABLE 1. C. albicans and S. cerevisiae strains used in this study

Isolation and characterization of the AOX1 gene from C. albicans. A genomic library of C. albicans was generated by partially digesting chromosomal DNA with Sau3AI, followed by ligation into $lambda$ EMBL3 vector (Stratagene) and packaging with Gigapack II packagingextracts (Stratagene). From the predicted amino acid sequencesof AOXs from Sauromatum guttatum (24), Arabidopsis thaliana(14), Glycine max (33), Nicotiana tabacum (31), Mangiferaindica (7), Trypanosoma brucei (4), Hansenula anomala (25),and Neurospora crassa (18), two highly conserved regions wereidentified, and the degenerate oligonucleotide primers correspondingto residues 145 to 151 (AGVPGMV) and 229 to 235 (GYLEEEA) of H.anomala AOX (25) $---$ 5'-GCTGGTGT(C/T)CC(A/T)GGTATGGT-3' and 5'-GCTTCTTC(C/T)TCCAA(A/G)TAACC-3',respectively $---$ were synthesized. PCR using the oligonucleotide primerpair could amplify a DNA fragment of about 0.3 kbp from the chromosomalDNA of C. albicans ATCC 10231. When cloned and sequenced, thefragment showed a high degree of amino acid sequence similarityto H. anomala AOX upon BLAST searches of the GenBank database.The cloned PCR product was used as a probe to screen the $lambda$ EMBL3genomic library. From positive clones, the common 3.2-kbp EcoRVfragment was subcloned in pGEM-5Zf(+) (Promega) andsequenced.

The cloned insert contained a continuous open reading frame (ORF) of 1,140 bp that encodes a polypeptide consisting of 379amino acids with a calculated molecular mass of 43,975 Da. C.albicans AOX1 did not contain the CUG codon, which encodes serinein C. albicans but encodes leucine in S. cerevisiae and elsewhere(26). The nucleotide sequence of AOX1 did not have the consensussequence for splicing. The fact that the gene does not containan intron was confirmed by reverse transcription-PCR (data notshown). The predicted amino acid sequence of C. albicans AOX showed54, 35, and 24% identity to that of H. anomala AOX (25), N.crassa AOX (18), and S. guttatum AOX (24), respectively. Thehydropathy plot of AOX obtained according to the method proposedby Kyte and Doolittle (16) predicted that the enzyme would bean integral membrane protein with two transmembrane segments correspondingto amino acid residues 176 to 194 and 239 to 257. This predictionagreed well with the previous reports (20) in which AOX wassupposed to be an inner mitochondrial membrane protein with twomembrane-spanning helices. According to the method proposed byGavel and von Heijne (10), the cleavage site for the mitochondrialpresequence was predicted to be between Ser residues at positions42 and 43. The molecular mass of the presumed mature form of C.albicans AOX, which consists of 337 amino acids, was calculatedto be 39,331Da.

On genomic Southern analysis with the genomic DNA from C. albicans ATCC 10231, four bands were detected when the genomic DNAwas digested with ClaI, EcoRI, or HindIII, and two bands weredetected when the genomic DNA was digested with XbaI (data notshown). Since the nucleotide sequence of AOX1 ORF contains oneClaI site, one EcoRI site, two HindIII sites, and no XbaI site,this hybridization pattern strongly suggested that AOX is encodedby a gene family with two members in C. albicans. In order toestimate the mRNA size and study the possible transcriptionalregulation of AOX1, Northern blot analysis was carried out. However,it was impossible to obtain the signal for AOX1, presumably becauseof the very low level of AOX1mRNA.

Disruption and overexpression of AOX1 in C. albicans. Disruption of AOX1 in C. albicans was carried out as described by Fonzi and Irwin (9). An in vitro construct was preparedby replacing a portion of the coding region of AOX1 with the hisG-URA3-hisGsequence (Fig. 1A), and used to transform CAI4. The resultingUra⁺ transformants were screened by Southern blot analysis, and thespontaneous Ura pop-out revertants from them were selected on FOA medium. A homozygousdisruption of AOX1 was generated by repeating the above procedure,and confirmed by PCR and Southern blot analysis (Fig. 1B). Inorder to overexpress AOX1 in C. albicans, we constructed the plasmidpWK302 by inserting the entire AOX1 gene and its flanking sequencesinto the plasmid pRC2312 (3). C. albicans cells were transformedwith the parent plasmid pRC2312 or pWK302, and transformants containingeither plasmid were selected by plating on uracil-deficient medium.

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FIG. 1. Sequential disruption of C. albicans AOX1. (A) Restriction map of the AOX1 locus and insertion of the hisG-URA3-hisG cassette at the BglII/HindIII sites in the AOX1 coding sequence. The endonuclease restriction sites are abbreviated as follows: B, BglII; C, ClaI; E, EcoRI; E5, EcoRV; H, HindIII; P, PstI; S, SpeI; X, XbaI. (B) Southern blot analysis with the bracketed sequence (as indicated in A) used as a probe. The DNA digested with BglII was from the following strains: lane 1, CAI4, AOX1/AOX1; lane 2, WH301, $Delta$ aox1::hisG-URA3-hisG/AOX1; lane 3, WH302, $Delta$ aox1::hisG/AOX1; lane 4, WH303, $Delta$ aox1::hisG/ $Delta$ aox1::hisG-URA3-hisG; lane 5, WH304, $Delta$ aox1::hisG/ $Delta$ aox1::hisG.

Respiration of cells was measured polarographically at 25°C by using a YSI 5300 Biological Oxygen Monitor Micro System (YellowSprings Instrument) as described by Minagawa and Yoshimoto (22).The total respiration rate of fresh CAI4 was approximately 108nmol of O₂ · h¹ · (mg of wet cell)¹ (Fig. 2A). When 1 mM KCN was added to the cells, the respirationrate was reduced to 14 nmol of O₂ · h¹ · (mg of wet cell)¹, which corresponds to the rate of cyanide-resistant respiration.The total respiration rate of fresh WH304 was about 9% lower thanthat of CAI4, and its cyanide-resistant respiration was scarcelyobserved on the addition of KCN. The respiratory behavior of WH305carrying the empty vector pRC2312 was somewhat similar to thatof CAI4. In the case of WH306 transformed with pWK302 plasmidcontaining AOX1, the total respiration rate was about 22% higherthan that of WH305 as a reference, and the rate did not changeon the addition of KCN. These results indicated that the clonedAOX1 gene encodes a functional AOX enzyme.

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FIG. 2. Respiratory characteristics of C. albicans and S. cerevisiae strains. Shown are respiratory activities of fresh cells of C. albicans (A), antimycin A-treated cells of C. albicans (B), fresh cells of S. cerevisiae (C), and antimycin A-treated cells of S. cerevisiae (D). Oxygen uptake in the absence (open bars) or the presence (solid bars) of 1 mM KCN was measured with an oxygen monitor. Data shown represent the means + standard errors (error bars) of three independent experiments. The absence of an error bar indicates that the error was too small to allow display of the error in the columns.

It has been reported that the expression of AOX protein is induced and cyanide-resistant respiration increases when the cytochromepathway is blocked by the respiratory inhibitors (25, 30).To investigate the effects of respiratory inhibitor on cyanide-resistantrespiration of C. albicans, cells were incubated in the presenceof 10 µM antimycin A for 1 h as described by Sakajo et al. (25).Incubation of CAI4 in the presence of 10 µM antimycin A greatlyenhanced cyanide-resistant respiration, the rate of which wasalmost identical to the total respiration rate (Fig. 2B). Unexpectedly,WH304 treated with antimycin A also showed cyanide-resistant respiration,the rate of which was about 91% of that of CAI4. Considering thatWH304 is the aox1/aox1 null mutant strain, this observation stronglysuggested that C. albicans may have another AOX, which can beinduced by antimycin A. The respiratory activity of antimycinA-treated WH305 was similar to that of CAI4, and the cyanide-resistantrespiration rate of antimycin A-treated WH306 was about 58% higherthan that of WH305 as areference.

For Western blot analysis, C. albicans mitochondria were isolated as described previously (12); added to 125 mM Tris-HCl,pH 6.8, containing 8% sodium dodecyl sulfate (SDS), 20% glycerol,and 0.004% bromophenol blue; and boiled for 2 min. Polyacrylamidegel (8%) was used for separating the mitochondrial proteins. Theresolved proteins were transferred onto a nitrocellulose membrane(Schleicher & Schuell) and probed with the antibody raised againstthe AOX protein from S. guttatum (8) at dilutions of 1:1,000.Western blot analysis with fresh cells showed that AOX was littleexpressed in WH304 and the expression of AOX remarkably increasedin WH306 compared with WH305 (Fig. 3A). These results were consistentwith the measurement of respiration (Fig. 2A). In Western blots,AOX from C. albicans appeared to occur as a monomeric form withan apparent molecular mass of 39 kDa. The apparent molecular massof C. albicans AOX coincided well with the predicted molecularmass of the mature enzyme (39,331 Da). When WH304 was treatedwith antimycin A, we could observe the induction of another AOXprotein, which occurred at the same position in SDS-polyacrylamidegel as that of the cloned one (Fig. 3B). These observations demonstratedthe presence of another AOX, which is also supported by the resultof genomic Southern blot analysis, which indicated that AOX isencoded by a gene family with two members in C. albicans.

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FIG. 3. Western blot analysis of AOX. (A) Western blot analysis of AOX from fresh cells of CAI4 (lane 1), WH304 (lane 2), WH305 (lane 3), and WH306 (lane 4). (B) Western blot analysis of AOX from antimycin A-treated cells of CAI4 (lane 1) and WH304 (lane 2). (C) Western blot analysis of AOX from WH117 (lane 1) and WH119 (lane 2). Mitochondrial proteins (30 µg) were separated by SDS-polyacrylamide gel electrophoresis, transferred to nitrocellulose, and probed with a monoclonal antibody to AOX. Numbers on the left side of the immunoblots are molecular masses of the standards. The arrow on the right side of each immunoblot indicates AOX.

Functional expression of C. albicans AOX1 in S. cerevisiae. It has been reported that S. cerevisiae does not have cyanide-resistant respiration mediated by AOX (22). We introducedC. albicans AOX1 into S. cerevisiae to see whether it can confercyanide-resistant respiration on S. cerevisiae. In order to expressC. albicans AOX1 in S. cerevisiae, we constructed the plasmidpWK303 by inserting the entire AOX1 gene and its flanking sequencesinto the plasmid pRS424 (5). Then, S. cerevisiae cells weretransformed with the parent plasmid pRS424 or pWK303, and Trp⁺ transformants were selected. As expected, the respiration ofWH117 carrying the empty vector was completely inhibited by theaddition of KCN (Fig. 2C). In the case of WH119 transformed witha multicopy plasmid containing C. albicans AOX1, the total respirationrate was about 80% higher than that of WH117 as a reference andthe addition of KCN did not affect the respiration rate. The totalrespiration rate of WH117 incubated in the presence of 10 µM antimycinA decreased dramatically (Fig. 2D). The respiratory activity ofantimycin A-treated cells of WH119 was similar to that of freshcells of WH119. In accordance with the measurement of respiration,Western blot analysis demonstrated that AOX was highly expressedin WH119 (Fig. 3C). These results indicated that C. albicans AOXcan be functionally expressed in AOX-deficient S. cerevisiae andconfirmed that the presence of AOX is enough to carry out cyanide-resistantrespiration.

According to Kumar and Söll (14), Arabidopsis AOX could confer cyanide-resistance on E. coli; E. coli cells transformedwith a plasmid carrying the Arabidopsis AOX gene grew well inthe presence of 0.5 mM KCN, which suppressed growth of the cellstransformed with the empty vector. In order to examine if C. albicansAOX could enhance cyanide-resistant growth of S. cerevisiae, WH117and WH119 were grown in the medium containing 0.5 mM KCN and cellgrowth was monitored. The presence of KCN significantly retardedthe cell growth in both strains. However, there was no differencein cell growth pattern between WH117 and WH119 (data not shown).Presumably, an unknown cyanide-resistant respiratory pathway inherentin S. cerevisiae, which is not mediated by AOX, may be sufficientto cause cyanide-resistant growth in S. cerevisiae.

Since seed germination, wound healing, flowering, and exposure to cold shock or oxidants were shown to be associated withincreased AOX activity, AOX seems to be closely related to celldifferentiation or stress response. However, the precise regulationmechanism and physiological roles of AOX have not been fully understoodyet. C. albicans, one of the dimorphic fungi, is a good modelsystem for studying cell differentiation and understanding thebiology of eukaryotic organisms. Therefore, the investigationof AOX in C. albicans is believed to contribute greatly to elucidatingthe nature of cyanide-resistant respiration. At present, we areattempting to clone another AOX from C. albicans, which is inducedby respiratoryinhibitors.

Nucleotide sequence accession number. The nucleotide sequence data reported in this paper have been submitted to GenBank under accession no. AF031229.

	ACKNOWLEDGMENTS

We thank William A. Fonzi for providing strain CAI4 and the p5921 plasmid and Richard D. Cannon for providing the pRC2312plasmid. We also thank Thomas E. Elthon for the generous giftof the monoclonal antibody againstAOX.

This work was supported by a research grant for the SRC (Research Center for Molecular Microbiology, Seoul National University)from the Korea Science and Engineering Foundation(KOSEF).

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratory of Biophysics, Department of Microbiology, College of Natural Sciences,and Research Center for Molecular Microbiology, Seoul NationalUniversity, Seoul 151-742, Republic of Korea. Phone: (82) (2)880 6703. Fax: (82) (2) 888 4911. E-mail: kangsaou{at}plaza.snu.ac.kr.

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1.	Aoki, S., and S. Ito-Kuwa. 1982. Respiration of Candida albicans in relation to morphogenesis. Plant Cell Physiol. 23:721-726[Abstract/Free Full Text].
2.	Berthold, D. A., and J. N. Siedow. 1993. Partial purification of the cyanide-resistant alternative oxidase of skunk cabbage (Symplocarpus foetidus) mitochondria. Plant Physiol. 101:113-119[Abstract].
3.	Cannon, R. D., H. F. Jenkinson, and M. G. Shepherd. 1992. Cloning and expression of Candida albicans ADE2 and proteinase genes on a replicative plasmid in C. albicans and in Saccharomyces cerevisiae. Mol. Gen. Genet. 235:453-457[Medline].
4.	Chaudhuri, M., and G. C. Hill. 1996. Cloning, sequencing, and functional activity of the Trypanosoma brucei brucei alternative oxidase. Mol. Biochem. Parasitol. 83:125-129[Medline].
5.	Christianson, T. W., R. S. Sikorski, M. Dante, J. H. Shero, and P. Hieter. 1992. Multifunctional yeast high-copy-number shuttle vectors. Gene 110:119-122[Medline].
6.	Clarkson, A. B., Jr., E. J. Bienen, G. Pollakis, and R. W. Grady. 1989. Respiration of bloodstream forms of the parasite Trypanosoma brucei brucei is dependent on a plant-like alternative oxidase. J. Biol. Chem. 264:17770-17776[Abstract/Free Full Text].
7.	Cruz-Hernandez, A., and M. A. Gomez-Lim. 1995. Alternative oxidase from mango (Mangifera indica, L.) is differentially regulated during fruit ripening. Planta 197:569-576[Medline].
8.	Elthon, T. E., R. L. Nickels, and L. McIntosh. 1989. Monoclonal antibodies to the alternative oxidase of higher plant mitochondria. Plant Physiol. 89:1311-1317[Abstract/Free Full Text].
9.	Fonzi, W. A., and M. Y. Irwin. 1993. Isogenic strain construction and gene mapping in Candida albicans. Genetics 134:717-728[Abstract].
10.	Gavel, Y., and G. von Heijne. 1990. Cleavage-site motifs in mitochondrial targeting peptides. Protein Eng. 4:33-37[Abstract/Free Full Text].
11.	Henry, M. F., and E. J. Nyns. 1975. Cyanide-insensitive respiration: an alternative mitochondrial pathway. Subcell. Biochem. 4:1-65[Medline].
12.	Huh, W.-K., S.-T. Kim, K.-S. Yang, Y.-J. Seok, Y. C. Hah, and S.-O. Kang. 1994. Characterization of D-arabinono-1,4-lactone oxidase from Candida albicans ATCC 10231. Eur. J. Biochem. 225:1073-1079[Medline].
13.	Huh, W.-K., B.-H. Lee, S.-T. Kim, Y.-R. Kim, G.-E. Rhie, Y.-W. Baek, C.-S. Hwang, J.-S. Lee, and S.-O. Kang. 1998. D-Erythroascorbic acid is an important antioxidant molecule in Saccharomyces cerevisiae. Mol. Microbiol. 30:895-903[Medline].
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