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Antimicrobial Agents and Chemotherapy, July 2006, p. 2300-2308, Vol. 50, No. 7
0066-4804/06/$08.00+0     doi:10.1128/AAC.00196-06
Copyright © 2006, American Society for Microbiology. All Rights Reserved.

Multiple cis-Acting Sequences Mediate Upregulation of the MDR1 Efflux Pump in a Fluconazole-Resistant Clinical Candida albicans Isolate

Davina Hiller, Stephanie Stahl, and Joachim Morschhäuser^*

Institut für Molekulare Infektionsbiologie, Universität Würzburg, Röntgenring 11, D-97070 Würzburg, Germany

Received 14 February 2006/ Returned for modification 4 April 2006/ Accepted 11 April 2006

Top Abstract Introduction Materials and Methods Results Discussion References

 
Overexpression of the MDR1 gene, which encodes a multidrug efflux pump of the major facilitator superfamily, is a frequent cause of resistance to the antimycotic agent fluconazole and other metabolic inhibitors in clinical Candida albicans strains. Constitutive MDR1 overexpression in such strains is caused by mutations in as yet unknown trans-regulatory factors. In order to identify the cis-acting sequences in the MDR1 regulatory region that mediate constitutive MDR1 upregulation, we performed a promoter deletion analysis in the genetic background of an MDR1-overexpressing clinical C. albicans isolate. We found that several different regions in the MDR1 promoter can mediate MDR1 overexpression in this isolate. In contrast, deletion of one of these regions abolished benomyl-induced MDR1 expression in a C. albicans laboratory strain. These results suggest that multiple transcription factors control expression of the MDR1 efflux pump in C. albicans and that the mutation(s) that causes constitutive MDR1 overexpression and drug resistance in clinical C. albicans isolates affects the activities of several of these transcription factors.

Top Abstract Introduction Materials and Methods Results Discussion References

 
The yeast Candida albicans is a member of the microflora on mucosal surfaces of the gastrointestinal and urogenitary tracts in many healthy people, but it can also cause superficial as well as life-threatening systemic infections, especially in immunocompromised patients (21). Oropharyngeal candidiasis, which frequently affects patients infected with the human immunodeficiency virus and AIDS patients, is commonly treated with the antimycotic agent fluconazole, which inhibits the biosynthesis of ergosterol, the major sterol in the fungal cell membrane. C. albicans can develop resistance to fluconazole, especially during long-term treatment of oropharyngeal candidiasis (30). Fluconazole resistance is caused by different molecular mechanisms, including alterations in the sterol biosynthetic pathway; overexpression of the ERG11 gene, which encodes the target enzyme of fluconazole, sterol 14-demethylase (Erg11p); mutations in the ERG11 gene that result in a reduced affinity of Erg11p to fluconazole; and overexpression of genes encoding membrane transport proteins which actively transport fluconazole out of the cell. In clinical C. albicans strains, several of these mechanisms are often combined to result in the stepwise development of clinically relevant fluconazole resistance (for a review, see reference 18).

Two types of efflux pumps that mediate resistance to fluconazole and structurally unrelated toxic compounds have been identified in C. albicans (6, 23-25). While CDR1 and CDR2 belong to the ATP-binding cassette (ABC) transporters, MDR1 is a member of the major facilitator superfamily which uses the proton gradient across the cytoplasmic membrane as an energy source for transport. In drug-susceptible C. albicans strains, MDR1 is expressed only at low levels in standard laboratory media, but its expression can be induced by some toxic compounds, like benomyl (10, 13, 27). In contrast, many fluconazole-resistant clinical C. albicans isolates constitutively overexpress MDR1 (8, 9, 16, 22, 26, 29). Comparison of the MDR1 promoter sequences in matched pairs of fluconazole-susceptible and MDR1-overexpressing, fluconazole-resistant C. albicans isolates from the same patient demonstrated that the constitutive MDR1 upregulation in the resistant isolates was not caused by promoter mutations but was caused by alterations in a trans-regulatory factor(s) (31). However, in contrast to the ABC transporters CDR1 and CDR2, whose expression has recently been shown to be controlled by the transcription factor Tac1p, which is mutated in CDR1/CDR2-overexpressing C. albicans strains (3, 4), the regulatory factors controlling MDR1 expression and the mutations that are responsible for its constitutive activation in drug-resistant clinical isolates have not yet been identified.

It is likely that transcription factors that normally activate MDR1 only under inducing conditions are constitutively active in MDR1-overexpressing, drug-resistant C. albicans isolates. Alternatively, MDR1 upregulation may also result from relief of repression by a negative regulatory factor. To control MDR1 expression, such transcription factors must bind to their target sequences within the MDR1 promoter. Therefore, to gain more insight into the mechanisms that lead to MDR1 upregulation, we set out to identify the cis-regulatory sequences in the MDR1 promoter which mediate its constitutive overexpression in drug-resistant clinical C. albicans isolates. To this end, we generated a series of MDR1 promoter deletion derivatives and determined their activities in the genetic background of such a clinical isolate.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Strains and growth conditions. The C. albicans strains used in this study are listed in Table 1. All strains were stored as frozen stocks with 15% glycerol at –80°C. The strains were propagated on synthetic defined medium (SD) agar plates containing 6.7 g of yeast nitrogen base without amino acids (YNB; Bio 101, Vista, Calif.), 20 g of glucose, 0.77 g of complete supplement medium without uracil (CSM-URA; Bio 101), and 15 g of agar per liter. For routine growth of the strains, YPD liquid medium (20 g of peptone, 10 g of yeast extract, 20 g of glucose, 15 g of agar per liter) was used. To support the growth of ura3 strains, 100 µg ml^–1 uridine was added to the medium.

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TABLE 1. C. albicans strains used in this study

Plasmid constructions. To generate the P_MDR1-GFP fusion, a 1.1-kb MDR1 promoter fragment was amplified by PCR from plasmid pGFP50 (31) with primers MDR1p7 and MDR1p9 (see Table 2 for the primer sequences), and the PCR product was digested at the XhoI and BamHI sites introduced at positions –1101 and –9, respectively, with respect to the position of the MDR1 start codon. The GFP gene from pGFP31 (19) was amplified with primers GFP13 and GFP4, and the PCR product was digested at the BamHI site introduced before the start codon (boldface in Table 2) and at an internal NcoI site. Sequences from the ACT1-coding region (positions +862 to +1547) were amplified from pGFP31 with primers ACT23 and ACT22. The PCR product was digested at the KpnI and XhoI sites that were introduced and was cloned together with the P_MDR1 fragment and the N-terminal GFP fragment into KpnI/NcoI-digested pGFP31 to result in pMPG1. ACT1 upstream sequences (positions –762 to +48) were then amplified with primers ACT24 and ACT25. The PCR product was digested at the SacII and PstI sites that were introduced and was cloned into SacII/PstI-digested pMPG1 to produce pMPG2, in which the GFP reporter gene is placed under control of the MDR1 promoter (see Fig. 1).

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TABLE 2. Primers used in this study

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FIG. 1. MDR1 promoter analysis. The structure of the insert of plasmid pMPG2 containing the PMDR1-GFP reporter fusion is shown on top. The MDR1 promoter is symbolized by the bent arrow; the GFP gene, which is fused to the transcription termination sequence of the ACT1 gene (TACT1; filled circle), is symbolized by the gray arrow; and the URA3 selection marker is symbolized by the hatched arrow. The ACT1 flanking sequences (position numbers are with respect to the position of the ACT1 start codon) used for ectopic integration of the PMDR1-GFP fusion into the ACT1 locus are represented by the white arrows, which also indicate the orientation of the ACT1 gene at the integration site. The relevant restriction sites used for the plasmid constructions are shown. Enlarged representations of the MDR1 regulatory region and deletion derivatives are shown below, and the names of the corresponding plasmids are indicated to the left. The extent of the MDR1 promoter sequences contained in the various plasmids is given. The transcriptional start site mapped at position –65 by Harry et al. (12) is indicated by the small bent arrow, and activating regions 1 to 3 identified in the present study are indicated by the black bars in pMPG2. The YRE is indicated by the small gray box. The fluorescence micrographs to the right of each construct show cells of strain F5U4 carrying the corresponding reporter fusion for illustration, and the mean fluorescence of the cells measured by flow cytometry is given. The inducibilities of the various MDR1 promoter derivatives by benomyl were also determined by measuring the fluorescence of transformants of strain CAI4 carrying the same reporter fusions in the presence of benomyl. All values are the means of results obtained for two independently constructed reporter strains.

Sequential truncations of the MDR1 promoter starting from position –913, –588, –495, –397, –300, or –286 were generated by amplification of MDR1 promoter fragments with primer MDR1p9 and one of the following primers: MDR1p16, MDR1p17, MDR1p19, MDR1p20, MDR1p18, or MDR1p21. The PCR products were digested at the XhoI and BamHI sites that were introduced and were substituted for the full-length MDR1 promoter in pMPG2 to generate pMPG7, pMPG8, pMPG9, pMPG10, pMPG12, and pMPG13, respectively.

Internal deletions within the MDR1 promoter region (see Fig. 2) were made as follows. Digestion of pMPG2 at two XbaI sites located at positions –916 and –592 within the MDR1 promoter and religation resulted in pMPG3. To construct pMPG4, a distal MDR1 promoter fragment (positions –1097 to –600) was amplified with primer pair MDR1p7/MDR1p10, and a proximal MDR1 promoter fragment (positions –496 to –10) was amplified with primer pair MDR1p9/MDR1p11. The PCR products were digested with XhoI/EcoRI and EcoRI/BamHI, respectively, and cloned together into XhoI/BamHI-digested pMPG2. Additional deletion constructs were made in an analogous fashion: for pMPG5, distal (positions –1097 to –500) and proximal (positions –287 to –10) MDR1 promoter fragments were amplified with the primer pairs MDR1p7/MDR1p12 and MDR1p9/MDR1p13 and substituted for the MDR1 promoter fragment in pMPG2. For pMPG6, the primer pairs MDR1p7/MDR1p14 and MDR1p9/MDR1p15 were used in the same way to delete the region from positions –272 to –101. To construct pMPG11, the distal and proximal MDR1 promoter fragments from pMPG4 and pMPG5, respectively, were fused and substituted for the MDR1 promoter in pMPG2. For pMPG14, pMPG15, pMPG16, and pMPG17, which contain deletions from positions –312 to –270, positions –355 to –309, positions –275 to –240, and positions –242 to –209, respectively, distal and proximal MDR1 promoter fragments were amplified with the primer pairs MDR1p7/MDR1p23 and MDR1p9/MDR1p22, MDR1p7/MDR1p25 and MDR1p9/MDR1p24, MDR1p7/MDR1p14 and MDR1p9/MDR1p26, and MDR1p7/MDR1p27 and MDR1p9/MDR1p28, respectively, and substituted for the MDR1 promoter fragment in pMPG2. To obtain pMPG19 containing a deletion from positions –205 to –101, a distal MDR1 promoter fragment was amplified with the primers MDR1p7/MDR1p29 and substituted for the corresponding fragment in pMPG6.

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FIG. 2. Structures of MDR1 promoter derivatives carrying internal deletions (indicated by the dashed lines). The extent of the MDR1 promoter sequences in each derivative is indicated, and the names of the plasmids containing the corresponding PMDR1-GFP reporter fusions are given to the left. The constitutive and benomyl-inducible activities of the MDR1 promoter derivatives in strains F5U4 and CAI4, respectively, were determined as explained in the legend to Fig. 1. The results obtained with strains carrying the PMDR1-GFP fusion contained in pMPG2 are taken from Fig. 1 and are included for comparison.

Truncated MDR1 promoter regions containing additional internal deletions (see Fig. 3 and 4) were obtained as described below and substituted for the full-length MDR1 promoter in pMPG2. For pMPG20, part of the MDR1 promoter from pMPG5 was amplified with primers MDR1p20 and MDR1p9. To produce pMPG21, the distal MDR1 promoter fragment from pMPG20 was fused with the proximal MDR1 promoter fragment from pMPG17. For pMPG22, part of the MDR1 promoter from pMPG14 was amplified with primers MDR1p21 and MDR1p9. For pMPG23, part of the MDR1 promoter from pMPG20 was amplified with primers MDR1p31 and MDR1p9. To create pMPG24, the distal MDR1 promoter fragment from pMPG22 was fused with the proximal MDR1 promoter fragment from pMPG11. For pMPG26, part of the MDR1 promoter from pMPG16 was amplified with primers MDR1p21 and MDR1p9. pMPG27 was obtained by amplifying the distal MDR1 promoter fragment and flanking ACT1 sequences from pMPG20 with primers ACT23 and MDR1p32 and fusing it with the proximal MDR1 promoter fragment from pMPG20.

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FIG. 3. Structures and activities of truncated MDR1 promoter derivatives with internal deletions. For explanations, see the legend to Fig. 1. The results obtained with strains carrying the PMDR1-GFP fusions contained in pMPG2 and pMPG5 are taken from Fig. 2 and are included for comparison.

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FIG. 4. Structures and activities of truncated MDR1 promoter derivatives with internal deletions in the region between positions –313 and –239. For explanations, see the legend to Fig. 1. The results obtained with strains carrying the PMDR1-GFP fusions contained in pMPG2 and pMPG13 are taken from Fig. 1 and are included for comparison.

C. albicans transformation. C. albicans strains were transformed by electroporation (14) with the following gel-purified, linear DNA fragments: the SacI-SphI fragment from pSFIU4 (28) to inactivate the URA3 gene in strain F5 and the KpnI-SacII fragments from pMPG2 and its derivatives to integrate the P_MDR1-GFP fusions into one of the ACT1 alleles of strains F5U4 or CAI4 with the help of the URA3 marker. Uridine-prototrophic transformants were selected on SD agar plates and mycophenolic acid (MPA)-resistant transformants were selected on SD agar plates containing 10 µg ml^–1 MPA (Sigma, Deisenhofen, Germany), as described previously (20). Single-copy integration of all constructs was confirmed by Southern hybridization.

Isolation of genomic DNA and Southern hybridization. Genomic DNA from C. albicans strains was isolated as described previously (17). DNA (10 µg) was digested with the appropriate restriction enzymes, separated in 1% (wt/vol) agarose gels, and after ethidium bromide staining, transferred by vacuum blotting onto nylon membranes and fixed by UV cross-linking. Southern hybridization with enhanced chemiluminescence (ECL)-labeled probes was performed with the ECL labeling and detection kit from Amersham (Braunschweig, Germany), according to the instructions of the manufacturer.

Fluorescence microscopy and flow cytometry. To detect and quantify GFP expression in the reporter strains, cells grown overnight in YPD medium were pelleted, suspended in phosphate-buffered saline to a density of 2 x 10⁵ cells per ml, and kept on ice. To induce the MDR1 promoter in transformants of strain CAI4, the overnight cultures were mixed with an equal volume of fresh YPD medium containing 50 µg ml^–1 benomyl and incubated for 3 h before harvesting of the cells. Fluorescence microscopy was performed with a Zeiss LSM 510 inverted confocal laser scanning microscope equipped with a Zeiss Axiovert 100 microscope. Imaging scans were acquired with an argon laser with a wavelength of 488 nm and corresponding filter settings for green fluorescent protein (GFP) and parallel transmission images. The cells were observed with a x63 immersion oil objective. Fluorescence-activated cell sorter (FACS) analysis was performed with a FACSCalibur cytometry system equipped with an argon laser emitting at 488 nm (Becton Dickinson, Heidelberg, Germany). Fluorescence was measured on the FL1 fluorescence channel equipped with a 530-nm band-pass filter. Ten thousand cells were analyzed per sample and were counted at low flow rate. Fluorescence and forward scatter data were collected by using logarithmic amplifiers. Data analysis was performed on fluorescence intensities that excluded cell autofluorescence and cell debris. The mean fluorescence values were determined with CellQuest Pro (Becton Dickinson) software.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Generation of a ura3 derivative of MDR1-overexpressing, clinical C. albicans isolate F5. In previous work we had ectopically integrated the GFP reporter gene under the control of the MDR1 promoter (P_MDR1) into the CDR4 locus in matched pairs of fluconazole-resistant and fluconazole-susceptible clinical C. albicans isolates with the help of the dominant MPA^R selection marker to demonstrate that the constitutive MDR1 overexpression observed in the resistant isolates was caused by alterations in a trans-regulatory factor and not by mutation of the MDR1 promoter (31). As the MPA^R marker seems to integrate preferentially into the IMH3 gene from which it is derived, many MPA-resistant transformants had to be screened to identify those that contained the P_MDR1-GFP fusion (31). Therefore, to facilitate integration of a larger number of reporter constructs containing GFP under the control of MDR1 promoter deletion derivatives, we decided to generate a ura3 mutant of fluconazole-resistant isolate F5, which would allow introduction of the reporter fusions with the help of the URA3 marker. For this purpose, we transformed strain F5 with a URA3 deletion construct in which the MPA^R flipper cassette (32) was inserted between URA3 flanking sequences. This construct had previously been used to create ura mutants of the C. albicans model strain WO-1 (28). Two rounds of integration of the MPA^R flipper cassette and subsequent FLP-mediated excision of the cassette resulted in strain F5U4, in which both URA3 alleles were specifically deleted from the genome (Table 1). ura mutant F5U4 retained the drug-resistant phenotype of its parental strain, strain F5 (data not shown), and the constitutive activation of the MDR1 promoter (see below), demonstrating that it could be used to identify the sequences in the MDR1 promoter that mediated its upregulation by the unknown regulatory factor(s).

Analysis of MDR1 promoter activity in strain F5U4. To verify the constitutive activation of the MDR1 promoter in strain F5U4, we placed the GFP reporter gene under the control of the same 1.1-kb MDR1 promoter fragment used in our previous studies (31), but in a cassette containing the URA3 selection marker instead of the MPA^R marker. In addition, we used flanking sequences from the ACT1 gene instead of the inconveniently long CDR4 flanking sequences, such that the P_MDR1-GFP fusions would be integrated into the ACT1 locus in an orientation opposite that of the ACT1 gene, and introduced unique restriction sites upstream and downstream of the MDR1 promoter fragment to facilitate the generation of deletion derivatives (see Materials and Methods) (Fig. 1).

Integration of the P_MDR1-GFP fusion from plasmid pMPG2 into strain F5U4 resulted in fluorescence of the cells, whereas no fluorescence was observed when the same reporter fusion was integrated in an identical fashion into fluconazole-sensitive laboratory strain CAI4, which does not detectably express the MDR1 gene (Fig. 1 and data not shown). This result confirmed that the 1.1-kb MDR1 promoter fragment (for the purpose of this study referred to as the full-length MDR1 promoter) integrated at the ACT1 locus was constitutively active in the genetic background of clinical C. albicans isolate F5 and did not exhibit detectable activity in a laboratory strain.

Multiple cis-acting sequences mediate constitutive MDR1 upregulation in clinical C. albicans isolate F5. We then constructed a series of reporter fusions with shorter MDR1 promoter regions, which were integrated in an analogous fashion in strain F5U4, to identify the sequences in the MDR1 promoter that mediated its constitutive activation in clinical isolate F5. As can be seen in Fig. 1, deletion of MDR1 promoter sequences distal to position –495 (plasmids pMPG7, pMPG9, and pMPG10) had no effect on its activity, and a further deletion to position –397 (pMPG13) affected only the level of expression but not the constitutive activity of the promoter. However, removal of the next 100 bp to position –300 (pMPG12) or –286 (pMPG8) abolished the activity of the MDR1 promoter, suggesting that sequences located between positions –397 and –301 (hereafter termed activating region 1) are required for constitutive MDR1 expression in isolate F5.

We also constructed a set of internal deletions within the full-length MDR1 promoter (Fig. 2). As expected from the results described above, deletion of sequences from positions –916 to –593 (pMPG3) or from positions –599 to –497 (pMPG4) did not affect the activity of the MDR1 promoter, whereas a deletion comprising the region from positions –599 to –288 (pMPG11) abolished MDR1 promoter activity. Surprisingly, however, deletion of the region from positions –499 to –288 (pMPG5) had only a minor effect on MDR1 promoter activity; i.e., activating region 1 was dispensable for constitutive MDR1 expression when the sequences upstream of position –499 were present. Small deletions ranging from positions –355 to –309, –312 to –272, –275 to –240, or –242 to –209 (plasmids pMPG14 to pMPG17, respectively) had only a minor effect or no effect on MDR1 promoter activity in strain F5U4, whereas deletion of sequences from positions –272 to –101 (pMPG6) or from positions –205 to –101 (pMPG19) abolished MDR1 expression. The MDR1 transcriptional start site has been mapped to position –65 (12); therefore, it is likely that the latter deletions affected the MDR1 core promoter.

To delimit the region that could mediate MDR1 upregulation in the absence of activating region 1, additional MDR1 promoter truncation-deletion constructs were tested (Fig. 3). A fragment ranging from positions –588 to –500 (hereafter termed activating region 2) was sufficient to mediate MDR1 expression in strain F5U4 when MDR1 promoter sequences starting from position –287 were also present (pMPG20). Neither of two overlapping fragments within activating region 2, either that from positions –588 to –547 (plasmid pMPG27) or that from positions –552 to –500 (plasmid pMPG23), was sufficient to mediate MDR1 expression in this context. The latter fragment contained a Yap1p response element (YRE), located between positions –532 and –526, indicating that YRE alone was not sufficient to mediate the constitutive MDR1 activation conferred by the whole activating region 2. Activating region 2 was unable to mediate MDR1 expression when the remaining MDR1 promoter sequences were shortened to position –208 (pMPG21), indicating that the region located between positions –287 and –209 contains an additional activating region, activating region 3.

In an attempt to define essential sequences in the proximal MDR1 promoter region, we generated another series of MDR1 promoter truncation-deletion derivatives (Fig. 4). Small deletions were introduced into the MDR1 promoter fragment starting from position –397 (pMPG13). All these overlapping deletions, comprising the sequences from positions –312 to –288 (pMPG24), positions –312 to –272 (pMPG22), or positions –275 to –240 (pMPG26), abolished MDR1 expression in strain F5U4. Interestingly, the same deletions, which presumably affected activating region 1 (pMPG24 and pMPG22) or activating region 3 (pMPG26), had almost no effect when they were introduced into the full-length promoter (compare pMPG22 and pMPG26 in Fig. 4 with pMPG14 and pMPG16 in Fig. 2).

Altogether, these results demonstrate that multiple cis-acting sequences within the MDR1 promoter mediate its constitutive activation in clinical C. albicans isolate F5. These cis-acting sequences include activating region 1, located between positions –397 and –301 (and possibly beyond), and activating region 2, located between positions –588 and –500. Together with proximal MDR1 promoter sequences starting from position –300, either of these regions is sufficient to mediate constitutive MDR1 upregulation. Sequences between positions –287 and –209 contain a third activating region that is required for the activity of activating region 2 (compare pMPG20 and pMPG21 in Fig. 3) as well as activating region 1 (compare pMPG13 and pMPG26 in Fig. 4) but that is dispensable in the full-length MDR1 promoter (compare pMPG2 with pMPG16 and pMPG17 in Fig. 2). Other sequences, e.g., the region between positions –495 and –397 (compare pMPG9 and pMPG13 in Fig. 1), are not required for constitutive MDR1 expression in isolate F5 but influence MDR1 expression levels.

Activating region 2 mediates benomyl-induced MDR1 expression in drug-susceptible C. albicans laboratory strain CAI4. In drug-susceptible C. albicans isolates, MDR1 is expressed only at low, basal levels (usually below the detection limit in Northern hybridization experiments), but MDR1 expression can be induced in these strains by certain chemicals, like benomyl (10, 13, 27). To investigate whether the same sequences that are required for constitutive MDR1 upregulation in clinical isolate F5 are also involved in inducible MDR1 expression in a drug-susceptible strain, we introduced all our reporter constructs into laboratory strain CAI4. None of the promoter deletion derivatives exhibited detectable activity in the absence of an inducing substance, suggesting that MDR1 expression is not under negative control, which might have been relieved after deletion of a binding site for a repressor. Benomyl efficiently induced the wild-type MDR1 promoter in strain CAI4 (Fig. 1, pMPG2); however, in contrast to the constitutive MDR1 expression in strain F5U4, benomyl-induced MDR1 expression depended on the presence of activating region 2. Whereas the truncated MDR1 promoter fragment starting at position –495 retained full activity in strain F5U4, the same promoter fragment was inactive and could not be induced by benomyl in strain CAI4 (Fig. 1, pMPG9). Furthermore, while deletion of sequences from positions –599 to –495, which contain activating region 2, from the full-length MDR1 promoter did not affect its activity in strain F5U4, the same deletion abolished benomyl-induced MDR1 expression in strain CAI4 (Fig. 2, pMPG4). Of note, activating region 2 was not sufficient for benomyl induction when the region from positions –499 to –287 was deleted (Fig. 3, pMPG20). These results indicate that the constitutive activation of the MDR1 promoter observed in clinical isolate F5 involves mechanisms different from those used to induce the promoter in the presence of benomyl.

Top Abstract Introduction Materials and Methods Results Discussion References

 
In this work we tried to define the cis-acting sequences in the MDR1 promoter that mediate the constitutive overexpression of this efflux pump in fluconazole-resistant, clinical C. albicans isolates. In a simple model, such drug-resistant isolates may contain a mutation in a transcription factor regulating MDR1 expression which rendered the transcription factor constitutively active. Deletion of the binding site for this transcription factor from the MDR1 promoter should therefore abolish its constitutive upregulation in a drug-resistant C. albicans strain. Such a situation has recently been described for the overexpression of the ABC transporter CDR2, whose expression is controlled by the transcription factor Tac1p. Gain-of-function mutations in TAC1 result in CDR2 (and CDR1) upregulation in drug-resistant C. albicans strains, and this upregulation depends on a single Tac1p binding site in the CDR2 promoter (3-5). The results of our promoter analysis indicate that the constitutive upregulation of MDR1 is more complex. We identified multiple cis-activating regions in the MDR1 promoter which in different combinations could mediate its activation in a drug-resistant C. albicans isolate. None of these regions was essential for constitutive MDR1 expression in drug-resistant isolate F5 since each of them could be deleted in the full-length MDR1 promoter without a loss of its activity, but the presence of at least two of them was required. A comparison of the three activating regions identified did not reveal sequences with striking similarity, suggesting that different transcription factors bind to these regions and activate the MDR1 promoter. Therefore, the constitutive MDR1 upregulation in clinical isolate F5 can be explained by different models. One possibility is that a gain-of-function mutation has occurred in a regulatory protein that controls the activities of several transcription factors that bind to the different activating regions in the MDR1 promoter. Such a mutation would result in the simultaneous activation of these transcription factors, which, in turn, can act together in different combinations to mediate MDR1 expression. Alternatively, several transcription factors might bind to each of the activating regions, including one that is common to all activating complexes and may be recruited by different factors to their binding sites. A mutation in such a transcription factor would also result in the simultaneous activation of several different activating regions. It is indeed likely that more than one transcription factor binds to the activating regions identified in the MDR1 promoter. For example, sequences from positions –552 to –500 containing the Yap1p response element could not substitute for the complete activating region 2 located between positions –588 and –500. Therefore, the C. albicans homologue of Yap1p, Cap1p, which has been shown to induce expression of the MDR1 homologue FLR1 in Saccharomyces cerevisiae and which is also involved in the regulation of MDR1 expression in C. albicans (1, 2), may bind to activating region 2 and mediate MDR1 upregulation, but only in combination with a second transcription factor binding within this region. MDR1 upregulation in other drug-resistant C. albicans strains may be caused by a similar mechanism, since strikingly similar alterations in the protein expression pattern were recently found in isolate F5 and an unrelated MDR1-overexpressing clinical C. albicans isolate compared with the patterns in their matched drug-susceptible isolates (15). In contrast, the inducible MDR1 expression that is also seen in drug-susceptible C. albicans strains exposed to certain chemicals seems to occur by a different mechanism. We found that activating region 2 was essential for benomyl-induced MDR1 expression in laboratory strain CAI4, whereas this region was dispensable for constitutive MDR1 upregulation in clinical isolate F5 when activating regions 1 and 3 were present. Therefore, MDR1 induction by benomyl may involve one but not all of the regulatory factors that mediate MDR1 overexpression in the clinical isolate. Karababa et al. recently compared the alterations in the gene expression profile of an MDR1-overexpressing, clinical C. albicans isolate and those seen upon induction of MDR1 expression by benomyl in a laboratory strain and found that the drug-induced gene expression only partially mimicked the alterations observed in the clinical isolate in which MDR1 was constitutively overexpressed (13). These findings also indicate that the mechanisms resulting in constitutive MDR1 overexpression in drug-resistant isolates are different from those leading to benomyl-induced MDR1 expression and involve additional regulatory factors.

Harry et al. recently also performed an MDR1 promoter deletion analysis with a C. albicans laboratory strain (11). Interestingly, they also identified two activating regions in the MDR1 promoter that mediate its induction by various chemicals, and these regions correspond to activating regions 1 and 2 identified in our study. Those authors did not identify activating region 3 described by us because they used only truncated MDR1 promoter constructs and no derivatives containing internal deletions, which were necessary to detect this third activating region. Similar to our results, activating region 2 (positions –600 to –500) was found in the study performed by Harry et al. (11) to mediate MDR1 induction in response to the presence of different toxic chemicals. In striking contrast, however, in the study by Harry et al. (11) induction by benomyl did not require activating region 2 but depended on activating region 1 (positions –400 to –300). While it is possible that the contrasting results with respect to the MDR1 promoter region involved in benomyl induction were caused by the differences in the origin of the MDR1 promoter or the integration site of the reporter fusions in the two studies, we favor a different explanation. It is not known how toxic compounds like benomyl induce gene expression, which may be a secondary response of the cells to stress conditions caused by the presence of the chemical and may not involve direct binding of benomyl to a transcription factor. Differences in the protocols used to expose the cells to benomyl in the two studies may have affected the cells in different ways, resulting in the use of alternative pathways to induce MDR1 expression.

The regulatory factors controlling expression of the MDR1 multidrug efflux pump in C. albicans and the mutations that cause constitutive MDR1 overexpression in drug-resistant clinical isolates still remain unknown. Our results demonstrating the involvement of several cis-activating regions in constitutive MDR1 upregulation and the existence of different mechanisms of MDR1 induction will help to explain how these regulatory factors control MDR1 expression once they have been identified.

 
We thank Calin Apetrei for help with the FACS analysis and Bill Fonzi and Fritz Mühlschlegel for the gift of strain CAI4.

This study was supported by the Deutsche Forschungsgemeinschaft (DFG grant MO846/3 and SFB630) and the European Community (EC project QLK2-CT-2001-02377). Sequence data for Candida albicans were obtained from the Stanford Genome Technology Center website at http://www-sequence.stanford.edu/group/candida. Sequencing of Candida albicans was accomplished with the support of the NIDR and the Burroughs Wellcome Fund.

 
* Corresponding author. Mailing address: Institut für Molekulare Infektionsbiologie, Universität Würzburg, Röntgenring 11, D-97070 Würzburg, Germany. Phone: 49-931-31 21 52. Fax: 49-931-31 25 78. E-mail: joachim.morschhaeuser{at}mail.uni-wuerzburg.de.

Top Abstract Introduction Materials and Methods Results Discussion References

 

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Antimicrobial Agents and Chemotherapy, July 2006, p. 2300-2308, Vol. 50, No. 7
0066-4804/06/$08.00+0     doi:10.1128/AAC.00196-06
Copyright © 2006, American Society for Microbiology. All Rights Reserved.

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