(Received for publication, April 22, 1997)
From the Institut de recherches cliniques de Montréal, Montréal, Québec H2W 1R7, Canada
We have isolated a Candida albicans gene that confers resistance to the azole derivative fluconazole (FCZ) when overexpressed in Saccharomyces cerevisiae. This gene encodes a protein highly homologous to S. cerevisiae yAP-1, a bZip transcription factor known to mediate cellular resistance to toxicants such as cycloheximide (CYH), 4-nitroquinoline N-oxide (4-NQO), cadmium, and hydrogen peroxide. The gene was named CAP1, for C. albicans AP-1. Cap1 and yAP-1 are functional homologues, since CAP1 expression in a yap1 mutant strain partially restores the ability of the cells to grow on toxic concentrations of cadmium or hydrogen peroxide. We have found that the expression of YBR008c, an open reading frame identified in the yeast genome sequencing project and predicted to code for a multidrug transporter of the major facilitator superfamily, is dramatically induced in S. cerevisiae cells overexpressing CAP1. Overexpression of either CAP1 or YAP1 in a wild-type strain results in resistance to FCZ, CYH, and 4-NQO, whereas such resistance is completely abrogated (FCZ and CYH) or strongly reduced (4-NQO) in a ybr008c deletion mutant, demonstrating that YBR008c is involved in YAP1- and CAP1-mediated multidrug resistance. YBR008c has been renamed FLR1, for fluconazole resistance 1. The expression of an FLR1-lacZ reporter construct is strongly induced by the overexpression of either CAP1 or YAP1, indicating that the FLR1 gene is transcriptionally regulated by the Cap1 and yAP-1 proteins. Taken collectively, our results demonstrate that FLR1 represents a new YAP1-controlled multidrug resistance molecular determinant in S. cerevisiae. A similar detoxification pathway is also likely to operate in C. albicans.
Cells have evolved elaborate molecular mechanisms to protect themselves from injuries caused by environmental exposure to toxic compounds of different structures and functions. One of these mechanisms, termed multidrug resistance (MDR)1 or pleiotropic drug resistance (PDR), operates in a wide variety of cell types, including bacteria, protozoans, fungi, and mammalian cells (1-4). It involves a network of membrane-associated transporters acting as multidrug efflux pumps and transcription factors regulating the expression of these pumps.
MDR has been extensively studied in the yeast Saccharomyces cerevisiae (3). Yeast transporters involved in MDR belong to two superfamilies: the ATP-binding cassette (ABC) and the major facilitator (MF) superfamilies (3, 5-7). These transporters utilize ATP hydrolysis (ABC) or proton electrochemical gradient (MF) as energy sources for active transport (8, 9). Yeast ABC transporters implicated in MDR include: Pdr5 (also known as Sts1/Ydr1/Lem1) and Snq2, two structurally similar proteins with overlapping but distinct drug specificities (10-14); Ycf1, a vacuolar glutathione-cadmium conjugate pump closely related to the mammalian multidrug resistance-associated and to the cystic fibrosis transmembrane regulator proteins (15-17); and Yor1, a Ycf1 homologue conferring resistance to oligomycin and reveromycin (18, 19). MDR transporters of the MF superfamily in S. cerevisiae include Atr1/Snq1 and Sge1, conferring resistance to aminotriazole and 4-NQO and to crystal violet, respectively (20-22). Several additional open reading frames (ORFs) predicted to code for ABC and MF transporters have been identified with the yeast genome sequencing project, but their role in MDR has yet to be determined (5-7).
Transcription factors such as Pdr1, Pdr3, and yAP-1 are also implicated
in MDR (23-25). Pdr1 and Pdr3, two homologous zinc finger proteins
belonging to the Zn2C6 binuclear zinc cluster family, have been shown to control the expression of the ABC
transporters PDR5, SNQ2, and YOR1 (23,
24, 26-29). yAP-1 (also known as Pdr4/Snq3/Par1) is also associated
with resistance to a variety of toxicants, including CYH, 4-NQO,
sulfometuron methyl, and cadmium, and with tolerance to oxidative
stress induced by compounds such as hydrogen peroxide and diamide
(30-37). yAP-1 belongs to a family of basic domain-leucine zipper
(bZip) transcription factors, which includes S. cerevisiae
Gcn4 and mammalian Fos and Jun (25). It binds to a conserved DNA
sequence termed the yAP-1 response element (YRE) within the promoter of
its targets to activate their transcription (34). yAP-1 targets include
the cadmium resistance ABC transporter gene YCF1 (15, 16),
as well as a number of genes involved in response to oxidative stress
such as GSH1, encoding -glutamylcysteine synthase (38);
TRX2, one of the two genes coding for thioredoxin (36); and
GLR1 encoding glutathione reductase (39). A yAP-1 homologue,
Cad1/yAP-2, has been isolated based on its ability to confer resistance
to cadmium and to 1,10-phenanthroline, but the target genes mediating
this resistance are still unknown (33, 40).
Candida albicans is an opportunistic yeast that causes severe infections in immunocompromised individuals (41). Among the different agents employed in antifungal therapy, the azole derivative FCZ is the most widely used because of its low toxicity and its high efficacy (42). However, the successful treatment of candidosis by FCZ has been impaired by the emergence of drug resistant strains in patients undergoing long term or prophylactic treatment, mostly AIDS patients (42-44). A number of studies investigating the mechanisms of FCZ resistance in C. albicans and other Candida species have shown that resistant strains fail to accumulate FCZ due to an increased drug efflux, suggesting the participation of transporter-mediated drug resistance mechanisms in these strains (45-49). Two C. albicans genes coding for transporters of the ABC superfamily, CDR1 and CDR2, have been recently isolated by complementation of an S. cerevisiae pdr5 null mutant (50, 51). In addition, the C. albicans BENr gene, coding for a multidrug transporter of the MF superfamily, has been cloned through its ability to confer benomyl resistance when overexpressed in S. cerevisiae (52, 53). CDR1, CDR2, and BENr have been shown to be overexpressed in C. albicans clinical and experimental FCZ-resistant isolates (47, 48, 51). However, the molecular mechanisms controlling the transcriptional induction of these transporters in response to drug exposure have not yet been elucidated.
In this report, we describe the identification of a new molecular determinant of C. albicans FCZ resistance by functional overexpression in S. cerevisiae. This gene, named CAP1, codes for a bZip transcription factor structurally and functionally related to S. cerevisiae yAP-1 (25). A search for the transcriptional target(s) of Cap1 mediating FCZ resistance in S. cerevisiae has identified FLR1, predicted to code for a transporter of the MF superfamily highly homologous to C. albicans BENr, as being an MDR effector of both Cap1 and yAP-1 (5, 7). This is the first demonstration that yeast AP-1 proteins can confer MDR by transcriptionally regulating the expression of a transporter of the MF superfamily.
S. cerevisiae diploid
strain W303 (a/ ade2/ade2 his3/his3 leu2/leu2
trp1/trp1 ura3/ura3 can1/can1) was a gift from M. Whiteway
(National Research Council of Canada, Biotechnology Research Institute,
Montreal, Canada). Strains S150-2B (a leu2 ura3 trp1
his3) and DJY125 (a leu2 ura3 trp1 his3
yap1::TRP1) were kindly provided by D. Jamieson (University of Dundee, Dundee, United Kingdom) (35). Cells
were grown in YPD medium or in synthetic dextrose (SD) medium lacking
uracil (SD
ura), leucine (SD
leu), or histidine (SD
his) (54).
Cell transformations were performed by the lithium acetate procedure
(55). Cultures were routinely grown at 30 °C.
Stock solutions of
FCZ (provided by Pfizer Canada Inc., Arnprior, Ontario) and CYH (Sigma,
Mississauga, Ontario) were prepared in water at 10 mg/ml. Stock
solutions of 4-NQO (Sigma) were prepared in dimethyl sulfoxide at 5 mM. Cadmium sulfate (MAT Laboratory, Beauport,
Québec) was dissolved in water at 50 mM. Stocks were aliquoted and kept at 80 °C.
A YEp352-based C. albicans genomic DNA library (a gift from C. Boone, Simon Fraser
University, Burnaby, British Columbia) was introduced in W303 cells
(56). YEp352 is a URA3-based, multicopy vector (57).
Ura+ transformants were selected on SD ura plates,
harvested, and plated on YPD plates containing FCZ at 500 µg/ml.
Plasmids from resistant colonies were recovered, analyzed by
restriction mapping, and found to carry identical genomic DNA inserts.
Plasmid pF1 was chosen for further characterization. Secondary pF1
transformants were found to be resistant to FCZ, thus confirming the
plasmid dependence of the resistance phenotype. A 3-kb
SmaI-PstI fragment from pF1 was subcloned in
plasmid YEp352 cleaved with SmaI and PstI, to
give plasmid pF1a. DNA sequence analysis of pF1a revealed that it
contained a truncated ORF. To obtain a full-length clone, a C. albicans fosmid library was screened with a pF1a subfragment as
probe, yielding five positive fosmids (B. Magee, University of
Minnesota, St. Paul, MN). A 3.2-kb BglII fosmid fragment
hybridizing with the probe was further subcloned into plasmid YEp352 at
the BamHI site, yielding plasmid FosBgl.
Sequencing of the CAP1 gene was performed on both DNA strands of the entire 3.2-kb BglII genomic DNA fragment with custom synthesized oligonucleotides, using the automated sequencing facilities of the Sheldon Biotechnology Center (McGill University, Montreal, Canada). Sequence analyses were performed using the University of Wisconsin Genetics Computer Group programs (58).
CAP1 and YAP1 Expression PlasmidsThe FosBgl and pF1a
plasmids were used throughout this study for expression of the
full-length and truncated versions of the CAP1 gene and were
renamed YEp352/CAP1 and YEp352/CAP1-TR, respectively. A 2.5-kb DNA
fragment overlapping the entire YAP1 gene (positions 349
to +2129 with respect to the initiation codon) (25) was amplified by
polymerase chain reaction (PCR) using S. cerevisiae genomic
DNA as template, the high-fidelity Pfu DNA polymerase (Stratagene), and oligonucleotides 5
-CGGATTCTAGCTGTTTGGTTGAT and
5
-CGGAATTCATACATAGTCTA. The resulting PCR fragment was
gel-purified and cloned blunt into YEp352 cut with SmaI, to
generate plasmid YEp352/YAP1.
For microtiter plate assays, cells
grown for 48 h on selective SD ura were resuspended in a saline
solution (0.85%) to an A600 of 0.1. These cells
were then diluted 100-fold in SD
ura. The diluted cell suspensions
were added to round-bottom 96-well microtiter plates (50 µl/well; in
duplicate) in wells containing equal volumes (50 µl) of medium with
different concentrations of the drug tested or in drug-free medium. The
plates were incubated at 30 °C for 48 h. Cell growth was
evaluated by reading the optical density at 650 nm in a microplate
reader (VmaxTM, Molecular Devices). The relative growth was calculated
as the percentage of growth in drug-containing medium relative to the
control growth in drug-free medium. The chosen concentrations were 50 µg/ml for FCZ, 0.1 µg/ml for CYH, and 1 µM for 4-NQO,
which correspond to the minimal inhibitory concentration of these drugs
for wild-type strain MRY13-1A transformed with control plasmid YEp352.
For the cadmium resistance spot assay, transformants were grown
overnight in SD
ura medium and approximately 104 cells
were spotted onto a YPD plate containing 0 or 10 µM
cadmium. The plates were incubated for 3 days at 30 °C. Resistance
to hydrogen peroxide was tested essentially as described (35). Briefly, transformants were grown to saturation in SD
ura medium and
approximately 106 cells were spread on YPD plates. A filter
paper disc was placed in the center of each plate, 10 µl of hydrogen
peroxide (30% w/v; Aldrich) was added to the disc and the plates were
incubated for 2 days at 30 °C before measuring the diameter of the
zones of growth inhibition.
W303 cells
transformed with plasmids YEp352, YEp352/CAP1, or YEp352/CAP1-TR were
grown in SD ura medium to an A600 of 2.0. Total RNA was extracted using the glass bead extraction method (59).
RNA samples (20 µg) were electrophoresed on a 7.5% formaldehyde, 1%
agarose gel and transferred by capillarity to a Zeta-Probe nylon
membrane (Bio-Rad, Mississauga, Ontario). Detection of specific RNAs
was performed by hybridization at 65 °C in 0.5 M
NaPO4, pH 7.2, 1 mM EDTA, 7% SDS, 1% bovine
serum albumin, and 100 µg/ml salmon sperm DNA with
32P-labeled DNA probes (60). The CAP1 probe was
a 614-bp XbaI-HincII DNA fragment (positions +47
to +661) isolated from clone pF1a. The PDR5 probe was
generated by PCR with primers 5
-CATACAGAAGCTCGAATC and
5
-CCACAGTTGACTGATAGG and overlaps region +111 to +447 of the
PDR5 gene (positions are relative to the translation
initiation codon) (10). The YBR008c probe, which overlaps a
region from
2 to +579 of the YBR008c ORF (GenBank Z35877),
was amplified by PCR with primers 5
-TGGTATACACTTCAACGT and
5
-TGTTATGCACAGTAGCAC. A LEU2 probe, consisting of a 0.6-kb
ClaI-EcoRV fragment isolated from plasmid pJJ282,
was also used as an internal control to monitor RNA loading and
transfer (61). Membranes were washed twice at 65 °C with a solution
containing 40 mM NaPO4, pH 7.2, 5% SDS, 1 mM EDTA, 0.5% bovine serum albumin and twice with a
solution containing 40 mM NaPO4 pH 7.2, 5%
SDS, and 1 mM EDTA) and were exposed for 24 h at
80 °C.
A 3.0-kb fragment overlapping the YBR008c ORF
and its promoter (positions 1146 to +1853; GenBank Z35877) was
amplified by PCR with primers 5
-AGAAAACGGTAACAACAA (forward) and
5
-CGAGCTCTGTGTAGACCTTAGATCT (reverse). The PCR fragment was digested
with SacI (a SacI site was introduced at the 3
end of the reverse primer) and cloned into pGEM-7Zf (Promega, Madison,
WI) cut with SmaI and SacI, to yield plasmid
pGEM7/YBR008. The ybr008c deletion plasmid
(pGEM/ybr008c
::HIS3) was constructed
by replacing a 1.6-kb SpeI-HindIII fragment of YBR008c (corresponding to positions
316 to +1339 relative
to the translation initiation codon) by a 0.9-kb
SmaI-PvuII HIS3 fragment isolated from
plasmid pJJ215 (61). A linear 2.3-kb ybr008c
::HIS3 deletion fragment was
excised with EcoRI and SacI and used to transform
W303 a/
. His+ transformants were selected and
sporulated. Haploid strains MRY13-1A (YBR008c) and
MRY13-1B (ybr008c
::HIS3) were
obtained as meiotic segregants of the heterozygous strain MRY13
(YBR008c/ybr008c
::HIS3). These strains were analyzed by Southern blotting to confirm their genotype at the YBR008c locus.
An FLR1(YBR008c)-lacZ
fusion plasmid was constructed using a PCR fragment overlapping the
promoter region, the translation initiation codon, as well as a short
portion of the coding region of the FLR1 gene (positions
828 to +25). This PCR fragment was generated using oligonucleotides
5
-CGGGATCCGGTAGAAGAGTTACGGAA and 5
-CCAAGCTTTGTCTGTACGTTGAAGTGTA,
which introduce, respectively, a 5
BamHI and a 3
HindIII site for directional cloning into YEp368 cleaved
with BamHI and HindIII (62), generating plasmid YEp368/FLR1. DNA sequencing was performed to confirm that the FLR1 coding region was in frame with the lacZ
gene. MRY13-1A cells carrying plasmid YEp352, YEp352/YAP1,
YEp352/CAP1, or YEp352/CAP1-TR were transformed with YEp368/FLR1.
Cotransformants were grown in SD
ura
leu medium to an
A600 of 1.0. Cells were collected by
centrifugation, rinsed with water, and resuspended in 0.5 ml of Z
buffer (60 mM Na2HPO4, 40 mM NaH2PO4, 10 mM KCl,
1 mM MgSO4, 50 mM
-mercaptoethanol) (63). Cell disruption was achieved by vortexing
the resuspended pellets for 2 min in the presence of glass beads. After
addition of 0.5 ml of Z buffer, the cellular extracts were centrifuged
for 15 min.
-Galactosidase activities were assayed by measuring
o-nitrophenyl-
-D-galactoside hydrolysis in
the supernatants (63) and are expressed as nanomoles of
o-nitrophenol formed/min/mg of protein. Protein
concentrations were determined by the method of Bradford (64), using
bovine serum albumin as standard.
Molecular genetic techniques involving the isolation of
C. albicans genes by functional overexpression in S. cerevisiae provide a powerful approach for the study of drug
resistance mechanisms. We have used this approach to search for
C. albicans genes that mediate resistance to the azole
derivative FCZ when overexpressed in S. cerevisiae. Strain
W303 was transformed with a YEp352-based C. albicans genomic
DNA library (56). Ura+ transformants were pooled and plated
on agar plates containing FCZ (500 µg/ml), a concentration that
corresponds to 10 × the minimal inhibitory concentration for W303
cells transformed with vector YEp352 alone. Plasmids from 12 randomly
chosen resistant colonies were purified and analyzed by restriction
mapping, revealing that all the isolated plasmids carried an identical
6-kb genomic insert. One of these plasmids (pF1) was selected for
further characterization (Fig. 1).
Functional testing of different pF1 subclones indicated that a 3-kb
fragment (pF1a) was sufficient to confer resistance (Fig. 1). DNA
sequence analysis of pF1a revealed the presence of an incomplete ORF
coding for a C-terminal truncated protein. To obtain a full-length
clone for this ORF, a C. albicans fosmid library was
screened with a pF1a subfragment as a probe, yielding five positive
fosmids. A 3.2-kb BglII fosmid fragment hybridizing with the
probe was further subcloned into plasmid YEp352 (57) at the
BamHI site (Fig. 1). The resulting plasmid (FosBgl) was also
functional in conferring FCZ resistance, as determined by agar plate
assay (not shown). DNA sequence analysis of the 3.2-kb BglII
genomic DNA fragment revealed that it contains an ORF of 499 amino
acids (Figs. 1 and 2). This protein is
rather hydrophilic, with an isoelectric point of 5.15 and a predicted
molecular mass of 55 kDa.
A computer search of sequence data bases revealed that the closest homology to the cloned ORF was observed with the S. cerevisiae transcription factor yAP-1 (37% identity, 55% overall homology) (25). The gene was thus named CAP1, for C. albicans AP-1. Other yeast proteins of the AP-1 family found to share a high degree of sequence similarity with the Cap1 protein are S. cerevisiae yAP-2/Cad1 (30% identity, 49% homology) (33, 40) and Schizosaccharomyces pombe pap1, which confers resistance to staurosporine (27% identity, 43% homology) (65). The general structure of these proteins includes an N-terminal basic domain involved in DNA binding to target sequences, followed by a leucine zipper motif implicated in dimerization, and a C-terminal acidic domain with regulatory function (25, 33, 37, 40, 65, 66).
A multiple sequence alignment of Cap1 with its homologues was generated
using the Pileup program (58); the two regions displaying the highest
degree of sequence conservation are presented in Fig. 3. These regions correspond to the
N-terminal basic domain followed by the leucine zipper motif (Fig.
3A) and to the C-terminal acidic domain (Fig.
3B). Within the AP-1 family of transcription factors, Cap1
belongs to a specific subgroup that includes yAP-1, yAP-2, and pap1,
according to three criteria. First, its basic domain is located at the
N terminus, unlike Gcn4, Fos, or Jun in which the basic domain is
located at the C terminus (67). The basic domain contains a short
segment highly conserved among the four proteins, which overlaps two
clusters of basic residues separated by an alanine spacer motif (Fig.
3A). This specific cluster-spacer-cluster organization,
found in all bZip transcription factors, is required for specific DNA
binding activity (67). Second, the third position of the heptad repeat
of the leucine zipper motif, which is a leucine in Gcn4, Fos, and Jun,
differs in all four proteins (an asparagine in both yAP-1 and yAP-2, a
threonine in pap1, and an alanine in Cap1) (Fig. 3A). This
residue appears to be functionally important as replacement of the
asparagine residue with a leucine in yAP-1 (N106L) has been shown to
have a strong negative effect on the DNA binding and transactivating
activities of this protein (66). Third, the C-terminal acidic region,
less conserved than the basic domain, is exclusive to this yAP-1
subfamily of transcription factors. Interestingly, this region contains
three cysteine residues invariably conserved among the four proteins
(Fig. 3B). In yAP-1, these cysteines are part of three
repeated cysteine-serine-glutamate (CSE) sequence motifs recently shown
to be required for normal regulation of yAP-1 in mediating oxidative
stress response (OSR) (37). Given that the truncated Cap1 protein that
lacks the C-terminal region is functional in conferring FCZ resistance
(Fig. 1), this domain appears to be dispensable, at least for this
specific activity of Cap1.
Functional Complementation of yap1 by CAP1
yAP-1 has been
shown to mediate cellular resistance to a large number of toxic
compounds, including cadmium and hydrogen peroxide (33-35). To
determine if the structural homology observed between Cap1 and yAP-1
translates into functional homology, we expressed YAP1 and
CAP1 in DJY125 cells, which carry a yap1
disruption (35), and compared the ability of these cells to grow in the
presence of toxic concentrations of cadmium or hydrogen peroxide. To
this end, DJY125 cells were transformed with plasmid YEp352/YAP1
(carrying the entire YAP1 gene under the control of its
promoter), YEp352/CAP1 (full-length), YEp352/CAP1-TR (truncated), or
YEp352 alone. The S150-2B parental wild-type strain (35) transformed
with YEp352 was also included as a control. These transformants were
then analyzed by a cadmium resistance spot assay (Fig.
4) and by a hydrogen peroxide filter disc
assay (Table I). When compared with
S150-2B (YEp352), DJY125 (YEp352) displayed hypersusceptibility to both
cadmium and hydrogen peroxide, as reported previously for a
yap1 mutant (33, 35). As anticipated, overexpression of
YAP1 in DJY125 was able to restore the ability of the cells to grow in the presence of cadmium (Fig. 4) or hydrogen peroxide (Table
I). Overexpression of CAP1 in DJY125 was also able to restore the ability of the cells to grow in the presence of both compounds, although with a lower efficiency than YAP1 (Fig.
4 and Table I). Finally, DJY125 cells transformed with YEp352/CAP1-TR were as susceptible to the two compounds as DJY125 cells carrying the
vector alone (Fig. 4 and Table I). These results demonstrate that Cap1
and yAP-1 are functionally related and that the C-terminal domain of
Cap1 is required to mediate resistance to cadmium and hydrogen peroxide
in S. cerevisiae DJY125 cells.
|
It has been shown that YAP1 confers resistance to toxic compounds and to oxidative stress by transcriptionally activating a number of downstream target genes encoding effector proteins mediating the resistance (34, 36, 38, 39). It is thus likely that Cap1 mediates FCZ resistance in S. cerevisiae through transcriptional activation of similar effector genes. What could these effectors be? In C. albicans, overexpression of CDR1, CDR2, and BENr has been shown to be associated with FCZ resistance (47). This raised the possibility that homologues of these genes could be the CAP1 target(s) mediating FCZ resistance in S. cerevisiae.
To test this hypothesis, we generated gene-specific probes for
PDR5, the closest S. cerevisiae homologue of
CDR1 and CDR2 (10), and for YBR008c,
the closest BENr homologue in S. cerevisiae identified through a Blast search. As for
BENr, the YBR008c gene product is
predicted to be a member of the MF superfamily (5, 7, 68). Total RNA
was extracted from S. cerevisiae W303 cells transformed with
plasmids YEp352, YEp352/CAP1, or YEp352/CAP1-TR. RNA samples were
analyzed by Northern blotting using a CAP1 (Fig.
5A), a PDR5 (Fig.
5B), or a YBR008c (Fig. 5C) radiolabeled DNA fragment as probe. The membranes were hybridized concurrently with a LEU2 probe as a control (61). RNA
analysis with the CAP1 probe showed that the full-length
CAP1 gene was expressed at high levels in S. cerevisiae, giving rise to two RNA transcripts of 2.2 and 1.9 kb
(Fig. 5A, lane 2), which were absent from the
W303 control cells (Fig. 5A, lane 1). Multiple transcripts were observed in cells expressing the truncated
CAP1 gene (Fig. 5A, lane 3), probably
resulting from read-through transcription within the plasmid due to the
lack of proper transcription termination signals in the truncated gene.
The basal level of PDR5 expression was found to be slightly
induced in cells transformed with CAP1, either full-length
or truncated (Fig. 5B). Finally, YBR008c
expression, undetectable in control cells (Fig. 5C,
lane 1), was dramatically induced in W303 cells
overexpressing either the full-length or the truncated CAP1
gene (Fig. 5C, lanes 2 and 3). The
massive overexpression of YBR008c in these cells is similar
to that observed for BENr in some FCZ resistant
clinical and experimental isolates (47, 48). These results are
consistent with the hypotheses that YBR008c is a target gene
for Cap1 in this heterologous expression system and is potentially the
Cap1 effector mediating FCZ resistance in S. cerevisiae CAP1
transformants.
YBR008c Is Essential for CAP1- and YAP1-mediated FCZ Resistance
To determine whether YBR008c was this
effector, we constructed a yeast strain carrying a chromosomal deletion
of this gene. To this end, a chimeric gene was generated in which a
1.6-kb SpeI-HindIII fragment overlapping the ATG
initiator codon and most of the coding region of YBR008c was
replaced with the HIS3 gene, and was introduced into the
isogenic diploid strain W303. A selected His+ transformant
carrying one wild-type YBR008c and one disrupted ybr008c::HIS3 allele (as confirmed
by Southern blotting analysis; data not shown) was sporulated. Tetrad
dissection gave rise to viable
ybr008c
::HIS3 spores, demonstrating
that YBR008c is not essential for growth. Two sister spores,
MRY13-1A (YBR008c) and MRY13-1B
(ybr008c
::HIS3), were selected for
the following resistance studies.
Strains MRY13-1A and MRY13-1B were transformed with plasmids YEp352,
YEp352/YAP1, YEp352/CAP1, and YEp352/CAP1-TR. These transformants were
tested for their ability to grow in the presence or absence of 50 µg/ml FCZ (the minimal inhibitory concentration for wild-type strain
MRY13-1A transformed with control plasmid YEp352), using a microtiter
plate assay (Fig. 6A). We
found that the three genes (YAP1, CAP1, and
CAP1-TR) were able to confer FCZ resistance when expressed
in the wild-type YBR008c strain, demonstrating that the
ability of CAP1 to mediate FCZ resistance in S. cerevisiae is not restricted to the C. albicans gene
but also extends to its S. cerevisiae homologue. This
finding further expands the spectrum of drugs to which YAP1
has been shown to confer resistance. Interestingly, the full-length
Cap1 protein was approximately 3 times less active than the truncated
Cap1 protein in this assay, indicating that the C-terminal domain of
Cap1 behaves as an inhibitor of Cap1 activity with respect to the
transcriptional regulation of YBR008c in S. cerevisiae (Fig. 6A). Unlike MRY13-1A cells however, MRY13-1B cells transformed with plasmids YEp352/YAP1, YEp352/CAP1, or
YEp352/CAP1-TR were completely unable to grow in FCZ, exhibiting a
relative growth value identical to that of the YEp352 control transformants (Fig. 6A). These results demonstrate that
YBR008c is essential for YAP1- and
CAP1-mediated FCZ resistance. Since MRY13-1B cells
transformed with plasmids YEp352/YAP1, YEp352/CAP1, or YEp352/CAP1-TR
were no more resistant to FCZ than the YEp352 control transformants, we
conclude that no other YAP1 or CAP1 downstream
targets, besides YBR008c, contribute to the FCZ resistance phenotype observed in the corresponding MRY13-1A transformants. In
particular, these results rule out a potential contribution of the
PDR5 gene suggested by the slightly elevated levels of PDR5 RNA transcripts observed in the W303 YEp352/CAP1 and
YEp352/CAP1-TR transformants (Fig. 5B). Finally, MRY13-1B
(YEp352) cells were not more susceptible to FCZ than MRY13-1A (YEp352)
cells, as predicted from the lack of YBR008c constitutive
expression in the absence of CAP1 overexpression (Fig.
5C). Taken together, these data demonstrate that
YBR008c codes for the YAP1 and CAP1
effector protein conferring FCZ resistance in S. cerevisiae.
YBR008c was thus renamed FLR1, for
fluconazole resistance 1.
YAP1- and CAP1-mediated FLR1 Overexpression Confers MDR
Overexpression of YAP1 in S. cerevisiae has been shown to confer resistance to the toxic compounds CYH and 4-NQO, but the target(s) of yAP-1 mediating this resistance has not yet been identified (31, 69). Interestingly, it has been shown that overexpression of the BENr gene in S. cerevisiae confers resistance to both CYH and 4-NQO and that inactivation of BENr in C. albicans results in hypersusceptibility to these two compounds (47, 53, 70). It was thus of interest to investigate if FLR1 was the YAP1 effector mediating CYH and 4-NQO resistance in S. cerevisiae.
To this end, strains MRY13-1A and MRY13-1B transformed with plasmids YEp352, YEp352/YAP1, YEp352/CAP1, and YEp352/CAP1-TR were examined for their ability to grow in the presence of CYH or 4-NQO (Fig. 6, B and C). We found that overexpression of the three genes (YAP1, CAP1, and CAP1-TR) in the wild-type FLR1 strain resulted in resistance to both CYH and 4-NQO (Fig. 6, B and 6C). As observed for FCZ (Fig. 6A), the full-length CAP1 gene was much less active than the truncated CAP1 in conferring resistance to these two compounds (Fig. 6, B and C). MRY13-1B cells transformed with plasmids YEp352/YAP1, YEp352/CAP1, or YEp352/CAP1-TR were as susceptible to CYH as the YEp352 control transformants (Fig. 6B), indicating that FLR1 is the only YAP1 target mediating CYH resistance in S. cerevisiae. In contrast to FCZ and CYH, however, MRY13-1B cells transformed with YEp352/YAP1 retained a significant level of residual resistance to 4-NQO (Fig. 6C), revealing the participation of other YAP1-controlled molecular determinant(s) of 4-NQO resistance in S. cerevisiae besides FLR1. Although almost as active as YAP1 in conferring resistance to 4-NQO in FLR1 wild-type cells, the truncated CAP1 gene was unable to induce the expression of these other 4-NQO resistance determinants, as no residual resistance was observed in MRY13-1B (YEp352/CAP1-TR) as compared with MRY13-1B (YEp352/YAP1) transformants (Fig. 6C). Taken together, these results demonstrate that FLR1 is the only YAP1 target mediating resistance to FCZ and CYH and is one of the YAP1 targets conferring resistance to 4-NQO. Thus, we can conclude that FLR1 represents a new YAP1-controlled multidrug resistance molecular determinant in S. cerevisiae.
FLR1 Is a Transcriptional Target for Proteins of the yAP-1 FamilyTo determine whether FLR1 is under the
transcriptional control of the yAP-1 and Cap1 proteins, we assessed
their ability to activate transcription of a lacZ reporter
gene under the control of the FLR1 promoter. To this end, an
FLR1-lacZ fusion gene was constructed, consisting of 828 bp
of 5 noncoding sequence and 25 bp from the FLR1 gene fused
to E. coli lacZ in plasmid YEp368 (62). This
FLR1-lacZ gene fusion was then introduced into MRY13-1A cells carrying plasmids YEp352/YAP1, YEp352/CAP1, YEp352/CAP1-TR, or
YEp352. The
-galactosidase activities were determined from the
resulting cotransformants to measure the effect of these plasmids on
the expression of the FLR1-lacZ fusion gene (Fig.
7). Presence of the FLR1-lacZ
construct in cells carrying the control plasmid YEp352 gave rise to
0.05 units of
-galactosidase activity, a small but significant value
since use of a control YEp368 vector lacking the FLR1
promoter did not result in any measurable
-galactosidase activity in
the same assay (data not shown). When the FLR1-lacZ plasmid
was introduced in cells transformed with plasmid YEp352/YAP1, a
-galactosidase activity of 5.2 units was obtained, representing an
approximate 100-fold increase as compared with the value measured in
the control YEp352 transformants. This result is consistent with the
proposition that FLR1 is under the transcriptional control of YAP1 in S. cerevisiae. A similar level of
-galactosidase activity was obtained with cells transformed with the
YEp352/CAP1 plasmid (5.7 units), confirming the functional relatedness
between yAP-1 and Cap1. Finally, the
-galactosidase activity
measured in cells transformed with the YEp352/CAP1-TR was approximately
2-fold lower than that measured in cells transformed with YEp352/CAP1
(3.0 units), indicating that the truncated Cap1 protein is less active than the full-length Cap1 protein in this transactivation assay. These
results were unexpected, in light of our data showing that the
truncated Cap1 protein was more active than full-length Cap1 in
conferring FCZ, CYH, and 4-NQO resistance (Fig. 6). Nevertheless, these
data show that both Yap1 and Cap1 are capable of stimulating FLR1 transcription and provide evidence that this control is
mediated through the FLR1 promoter.
These results prompted us to scan the promoter region of the
FLR1 gene for the presence of a DNA sequence motif similar
to previously identified YREs (34). Our analysis revealed that the
FLR1 promoter indeed contains three potential YREs of
sequence 5-TTAGTA/CA, one on the coding strand (position
149 with
respect to the translation initiation codon at +1) and two on the
anticoding strand (positions
161 and
358) (Fig.
8). Functional YREs of similar sequence
have been shown to be present in the promoter of the YAP1
target genes GSH1, YCF1, TRX2, and
GLR1 (Fig. 8) as well as in the SV40 early enhancer element
(34, 36, 38, 39, 71). A detailed functional analysis of the
FLR1 promoter is currently under way to determine whether
the control of FLR1 transcription by yAP-1 is direct or
indirect and whether it is mediated through the YREs present in the
promoter.
Investigation of C. albicans molecular determinants of
FCZ resistance has allowed us to isolate a gene coding for a new member of the yeast AP-1 family that we have named CAP1. A computer
search of protein data bases identified S. cerevisiae yAP-1
as being the closest homologue of the Cap1 protein (25). Other yeast proteins also found to share a high degree of sequence similarity with
Cap1 are S. cerevisiae yAP-2/Cad1 and S. pombe
pap1 (33, 40, 65). These proteins are apparently not only structurally but also functionally related, since their overexpression from a
multicopy plasmid results in a similar phenotype, namely an increased
cellular resistance to different toxicants (31, 33, 40, 65, 69). More
specifically, we show that the sequence homology between the Cap1 and
yAP-1 proteins translates into functional homology, because
(a) CAP1 expression in a yap1 mutant
partially restores the ability of the cells to grow on otherwise toxic
concentrations of cadmium or hydrogen peroxide (Fig. 4 and Table I) and
(b) both yAP-1 and Cap1 can transactivate FLR1 to
confer MDR (Figs. 6 and 8). yAP-1 is the best studied member of this
family of fungal transactivators. In addition to its role in drug
resistance, yAP-1 has been shown to participate in OSR via the
transcriptional activation of a spectrum of targets including
GSH1, encoding -glutamylcysteine synthase (38);
TRX2, one of the two genes coding for thioredoxin (36); and
GLR1, encoding glutathione reductase (39). Therefore, it is
quite possible that Cap1 serves similar functions in C. albicans by transactivating a number of effector genes homologous to those controlled by yAP-1 in S. cerevisiae. The
availability of the cloned CAP1 gene will now allow an
analysis of its role in C. albicans with respect to both MDR
and OSR.
An amino acid sequence comparison of the Cap1, yAP-1, yAP-2, and pap1 proteins indicates that the most conserved regions among these proteins overlap the N-terminal bZip and the C-terminal acidic domains (Fig. 3). A bZip domain is found in a large number of transcription factors of the AP-1 family, including S. cerevisiae Gcn4 and mammalian Jun, Fos, C/EBP, and CREB, and its function in DNA binding and in protein dimerization has been extensively studied (67). However, the role of the C-terminal domain, which is present only in the yeast AP-1 subfamily of transcription factors, is much less understood. A short segment of approximately 60 amino acids located at the extreme C terminus contains a number of highly conserved residues, including three invariably conserved cysteines (33, 40, 65) (Fig. 3B). In yAP-1, these cysteines are part of three repeated cysteine-serine-glutamate (CSE) sequence motifs recently shown to be required for normal regulation by yAP-1 in mediating oxidative stress tolerance (37). It has been shown that truncated yAP-1, yAP-2, and pap1 proteins lacking the C-terminal domain are still functional in conferring resistance to cadmium, to 1,10-phenanthroline, and to staurosporine, respectively, indicating that this domain is dispensable at least for these specific phenotypes (40, 65, 66). During the course of our work, we have isolated a genomic DNA fragment carrying an incomplete version of the CAP1 gene coding for a truncated protein lacking the entire C-terminal domain (Fig. 1). On the one hand, we find that the truncated Cap1 protein is active in conferring FLR1-mediated resistance to FCZ, CYH, and 4-NQO upon overexpression in a wild-type strain (Fig. 6). On the other hand, when tested for its ability to suppress a yap1 mutation, the truncated Cap1 protein is completely inactive in restoring tolerance to cadmium and hydrogen peroxide (Fig. 4 and Table I). A potential explanation for these two different phenotypes is that the truncated Cap1 protein requires the presence of yAP-1 to bring about efficient transcriptional activation. Alternatively, it is possible that the C-terminal domain of Cap1 selectively modulates the protein activity, displaying either an inhibitory or an activating function depending on the transcriptional target. The fact that the truncated Cap1 protein (a) is active in inducing FLR1-dependent 4-NQO resistance but inactive in inducing FLR1-independent 4-NQO resistance (Fig. 6C) and (b) is able to confer FCZ resistance in yap1 DJY125 cells (data not shown) supports the second hypothesis. Finally, we find that the truncated Cap1 protein, which is more active than the full-length protein in conferring MDR, is less active than full-length Cap1 in transactivating an FLR1-lacZ fusion gene (compare Figs. 6 and 7). One possible reason for this discrepancy may be that drugs, present in the drug resistance assay and absent from the transactivation assay, differentially modulate the activity of the two forms of Cap1. As C. albicans genes can behave as mutants when expressed in S. cerevisiae (72), it will be important to study the effect of the Cap1 C-terminal truncation in C. albicans and/or to test the effects of a similar deletion in yAP-1 on its ability to transactivate its different targets in S. cerevisiae to be able to draw definitive conclusions from these observations.
Several ORFs predicted to code for MDR transporters of the MF superfamily (MFS) based on structural considerations have been identified during the yeast genome sequencing project but their role in MDR remains to be determined (5, 7). Based on hydropathy analyses, these ORFs have been grouped into three clusters: members of cluster I (12 ORFs) are predicted to contain 12 TM domains, whereas members of cluster II (10 ORFs) and of cluster III (6 ORFs) are predicted to contain 14 TM domains (5, 7). So far, only two transporters of the MFS in S. cerevisiae have been demonstrated to function as MDR determinants, namely Atr1 (4-NQO and aminotriazole resistance) and Sge1 (crystal violet and ethidium bromide resistance), which both belong to cluster II (reviewed in Ref. 7). Our data, showing that YAP1-mediated FLR1 overexpression in S. cerevisiae results in cellular resistance to FCZ, CYH, and 4-NQO, demonstrates that FLR1 indeed functions as an MDR determinant (Fig. 6). Furthermore, overexpression of FLR1 from the strong constitutive glyceraldehyde-3-phosphate dehydrogenase promoter in S. cerevisiae results in high levels of resistance to these three compounds as well as to benomyl and 1,10-phenanthroline, confirming that FLR1 is an MDR determinant with broad substrate specificity.2 FLR1 (YBR008c) is predicted to code for an integral membrane protein with 12 potential transmembrane segments belonging to cluster I (5, 7). Interestingly, MFS proteins known to function as MDR efflux pumps in other yeasts also belong to cluster I, including C. albicans BENr, Candida maltosa CYHR, and S. pombe CAR1 (7). It will be of interest to determine whether other MFS MDR ORFs, identified based on structural considerations by the systematic analysis of the yeast genome, actually function as MDR determinants and whether some of them are under the transcriptional control of YAP1 as part of a yet unidentified MDR network in S. cerevisiae (see below).
A number of observations indicate that FLR1 expression is under the control of AP-1 proteins. First, the steady state level of FLR1 RNA is drastically increased in CAP1 and CAP1-TR transformants (Fig. 5C). Second, YAP1- and CAP1-mediated multidrug resistance in a wild-type strain is completely abrogated (FCZ and CYH) or strongly reduced (4-NQO) in an flr1 null mutant strain (Fig. 6). Third, the FLR1 promoter contains three DNA sequence elements matching a functional YRE (Fig. 8). Fourth, the FLR1 promoter fused to a reporter gene is strongly transactivated by the overexpression of YAP1 or CAP1 (Fig. 7). Overexpression of YAP1 in S. cerevisiae had been previously shown to confer resistance to different toxic compounds including CYH and 4-NQO, but the target(s) of yAP-1 mediating this resistance had so far remained unidentified (31, 69). The results presented here clearly identify FLR1 as being the YAP1 effector mediating CYH resistance (in addition to FCZ resistance) and one of the YAP1 effectors conferring resistance to 4-NQO. Taken collectively, these results allow us to conclude that FLR1 represents a new YAP1-controlled MDR molecular determinant in S. cerevisiae. This widens the spectrum of already known yAP-1 physiological targets to include an MFS MDR transporter and further substantiates that yAP-1 is a key regulator molecule involved in controlling MDR in addition to OSR. It also raises the possibility that yAP-1 regulates additional unidentified targets involved in MDR. Our results showing residual YAP1-mediated resistance to 4-NQO in an flr1 null mutant strain confirms this hypothesis (Fig. 6C). Such YAP-1 target(s) mediating 4-NQO resistance could well include the ABC transporter SNQ2 and/or the major facilitator ATR1, as both genes have been shown to confer resistance to 4-NQO and to contain YRE motifs in their promoter regions (14, 20, 21, 73). Experiments are currently under way to test this proposition.
C. albicans strains can develop clinical resistance to FCZ
in individuals undergoing long term therapy or prophylactic treatment, mostly AIDS patients (42-44). Two major mechanisms of FCZ resistance have been identified so far in these strains: (a)
alterations in the drug target (14--sterol demethylase, the
product of the ERG16 gene), resulting in an increased
production of the enzyme or in its reduced binding affinity for FCZ
(reviewed in Refs. 74 and 75); and (b) a reduced
intracellular FCZ accumulation, which usually correlates with the
overexpression of the ABC transporter genes CDR1 and
CDR2 and of the MF transporter BENr (47,
51); this latter mechanism appears to be the most important. The
molecular events up-regulating the expression of these transporters in
C. albicans are not known. It has been shown by Northern
blot analyses of C. albicans clinical isolates that
CDR1 is constitutively expressed at low levels in
FCZ-susceptible strains, while CDR2 and
BENr are not expressed in these strains, at least at
levels detectable by this technique (47, 51). However, these genes
become markedly overexpressed in FCZ-resistant isolates, which can
exhibit either CDR1, concomitant CDR1 and
CDR2, or BENr overexpression (47, 48,
51), suggesting the participation of transporter-specific
transactivating factors in the establishment of FCZ resistance in these
isolates. In S. cerevisiae, the expression of
PDR5, a close homologue of CDR1 and
CDR2, is under the transcriptional control of the zinc
finger proteins PDR1 and PDR3 (27); it is thus
possible that PDR1 and PDR3 homologues in
C. albicans also operate to up-regulate CDR1 and
CDR2 expression. On the other hand, our isolation of a
YAP1 homologue from C. albicans together with our
demonstration that both yAP-1 and Cap1 transcriptionally control the
BENr homologue FLR1 in S. cerevisiae suggest that CAP1 could be involved in
controlling BENr expression to cause FCZ resistance
in C. albicans. We have found that overexpressing
CAP1 (the truncated form) in C. albicans CAI4 cells results in BENr overexpression and in FCZ
resistance, confirming that indeed CAP1 participates in the
transcriptional control of BENr in C. albicans.3 What could be
the molecular events leading to BENr transcriptional
activation? FCZ resistance in strains overexpressing BENr is a stable phenotype, suggesting that FCZ
resistance in these strains is due to genetic alterations rather than
to transient cellular adaptations (47, 48). Such permanent alterations potentially include dominant activating mutations in the
BENr promoter or in trans-acting factors controlling
BENr expression, such as CAP1. We are
currently investigating these possibilities in clinical and
experimental FCZ resistant C. albicans isolates
overexpressing BENr.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) U95611.
We thank Dr. Beatrice Magee for providing fosmid clones, Dr. Charles Boone for the C. albicans genomic DNA library, Dr. Derek Jamieson for strain DJY125 and advice, Sandra Weber for technical assistance, and Dr. Tanya Parkinson and Dr. Bernard Turcotte for helpful comments on the manuscript.