Transcriptional profile of Paracoccidioides spp. in response to itraconazole

Background Itraconazole is currently used to treat paracoccidioidomycosis. The mechanism of action of azoles has been elucidated in some fungi, although little is known regarding its mechanism of action in Paracoccidioides spp. The present work focused on identification of regulated transcripts using representational difference analysis of Paracoccidioides spp. yeast cells treated with itraconazole for 1 and 2 h. Results Paracoccidioides Pb01 genes up-regulated by itraconazole included genes involved in cellular transport, metabolism/energy, transcription, cell rescue, defense and virulence. ERG11, ERG6, ERG3, ERG5 and ERG25 were up-regulated at multiple time points. In vivo infection experiments in mice corroborated the in vitro results. Ergosterol levels and distribution were evaluated in Paracoccidioides Pb18 yeast cells, and the results demonstrate that both factors were changed in the fungus treated with itraconazole. Conclusion To our knowledge, this is the first transcriptional analysis of Paracoccidioides spp. exposed to a triazole drug. Here acetyl seems to be intensively produced from different metabolic pathways to produce ergosterol by the action of ergosterol synthesis related enzymes, which were also affected in other fungi. Among the genes affected, we identified genes in common with other fungi, as well as genes unique to Paracoccidioides Pb01. Those genes could be considered target to new drugs. Voltage-gated Ca2+ alpha subunit (CAV), Tetracycline resistance protein (TETA) and Hemolisyn-iii channel protein (HLYiii) were found only here and a probably involvement with resistence to itraconazole could be investigated in the future. However our findings do not permit inference to current clinical practice.


Background
Paracoccidioides spp., a complex of several phylogenetic species, is the agent of paracoccidioidomycosis (PCM). Paracoccidioides spp. is a thermodimorphic fungus, which grows in the soil as saprobic mycelium, resulting in the formation of propagules, which initiate infection in humans when inhaled into the respiratory tract. Subsequently, in the lung, the mycelia propagules develop into yeast cells [1]. PCM is endemic in Latin America [2], with 80% of cases reported in Brazil, where it is the eighth-leading cause of mortality among infectious and parasitic diseases, establishing it as a serious public health problem [3,4].
Itraconazole is suggested to be the best alternative for first-line therapy of PCM and should be administered over a long period [5]. Itraconazole is a triazole antifungal drug, which are multi-ringed synthetic compounds containing three nitrogen atoms in the azole ring. Mechanistically, the triazole drugs inhibit the synthesis of ergosterol, an essential component of fungal cell membranes, and cause abnormalities in the membrane permeability and consequently cell death [6]. Itraconazole and related azole derivatives act by blocking the ergosterol biosynthesis pathway through the inhibition of the fungal cytochrome P450 enzyme lanosterol demethylase (Erg11) [7].
The global response to azoles, including itraconazole, of fungi such as Saccharomyces cerevisiae [8], Trichophyton rubrum [9], Aspergillus fumigatus [10] and Candida albicans [11,12] has been studied using transcriptional and proteomic approaches. In general, the findings revealed both specific and nonspecific antifungal-induced changes in gene and protein regulation. There was an increase in expression of the genes involved in lipid, fatty acid and sterol metabolism, as well as genes involved in drug adaptation, including cell stress response, drug efflux and small molecule transport.
Despite of the importance of Paracoccidioides spp., nothing is known about the mechanism of itraconazole inhibition in this pathogen. Here, cDNA libraries were constructed to obtain expressed sequence tags (ESTs) of Paracoccidioides spp. The representational difference analysis (RDA) technique was used to identify changes in the transcriptional profile of Paracoccidioides spp. in response to itraconazole, with the aim of identifying the adaptative response of the fungus to the compound. Transcript levels were also measured during the infection process. In addition, the transcript levels of ERG genes, ergosterol levels and ergosterol localization were evaluated.

Libraries characteristics
A total of 861 ESTs were successfully sequenced. From these, 224 up-and 208 down-regulated ESTs were obtained from yeast cells after incubation with itraconazole for 1 h, containing 55 singlets and 26 contigs for up-regulated transcripts and three singlets and 20 contigs for downregulated ones. In addition, 230 up-and 199 downregulated ESTs were obtained from yeast cells after incubation with itraconazole for 2 h, containing three singlets and 10 contigs for up-regulated and seven singlets and 12 contigs for down-regulated. The ESTs obtained were submitted to the National Center for Biotechnology Information (NCBI) database under accession numbers: LIBEST_028165 Paracoccidioides Pb01 itraconazole 1 h up Library, LIBEST_028164 Paracoccidioides Pb01 itraconazole 1 h down Library, LIBEST_028167 Paracoccidioides Pb01 itraconazole 2 h up Library and LIBEST_028166 Paracoccidioides Pb01 itraconazole 2 h down Library.
The ESTs were processed using the Blast2GO program, which allowed us to annotate and identify the different functional groups. The functional classification was based on the homology of each EST, considering e-values ≤10 −5 significant, using BLASTx against the GenBank non-redundant database and the MIPS functional annotation scheme ( Table 1). The analyses indicated the presence of transcripts from different functional categories: metabolism/energy, transcription, cell rescue, defense and virulence, protein synthesis and biogenesis, protein fate, cellular transport, biogenesis of cellular components and cellular communication.
In addition, genes precursors to the components of membrane and cell walls were found, such as phospholipids and carbohydrates, as well as genes related to detoxification. These components are diacylglycerol o-acyltransferase (DGAT), chitin synthase regulator 2 (CHSr), hemolysiniii channel protein (HLYiii), tetracycline resistance protein (TETA), voltage-gated Ca 2+ alpha subunit (CAV) and the MFS transporter.
using specific oligonucleotides in qRT-PCR. The results showed that all transcripts were increased at all time points ( Figure 2B).

Paracoccidioides Pb18 transcripts identified in mice treated with itraconazole
We investigated whether the regulated transcripts identified by RDA experiments using Pb01 also occurred in another cryptic species, Pb18, in vivo. Balb/c mice infected with Paracoccidioides Pb18 were treated with itraconazole, and spleens were removed. The treatment with itraconazole reduced the fungal burden 42% in the spleens. RNAs extracted from recovered fungus were analyzed in qRT-PCR experiments using MFS, GST and CHSr genes. In agreement with the RDA data, all the evaluated genes were up-regulated in spleen fungal samples after treatment with itraconazole ( Figure 2C).

GST-specific activity correlates with transcriptional data
Because GST transcripts were up-regulated in our study and are described in the literature as important for the detoxification of many different xenobiotics [14], we evaluated the GST-specific activity in protein extracts of fungus grown in the presence of itraconazole. GST-specific activity in the presence of itraconazole (0.26 μmol/mg/ min) was 6.5 times higher than in the absence of itraconazole (0.04 μmol/mg/min) ( Figure 2D).

Analysis of the ergosterol level
Because transcript levels of ergosterol pathway components were changed in the presence of itraconazole, we evaluated if itraconazole could disturb the total intracellular level of ergosterol. The method for quantification of ergosterol used here takes advantage of the unique four-peak spectral absorption pattern produced by extracted sterols between 240 and 300 nm. Comparing the scans obtained from control (1.0 g of ergosterol/g yeast cells to Pb01; 1.2 g of ergosterol/g yeast cells to Pb18) and the corresponding itraconazole-exposed cultures (0.80 g of ergosterol/g yeast cells to Pb01; 0.62 g of ergosterol/g yeast cells to Pb18), a decrease of 39% and 48.6% was identified in the ergosterol content of Paracoccidioides Pb01 and Pb18 yeast cells, respectively grown in the presence of itraconazole.
Effect of itraconazole on ergosterol localization in Paracoccidioides Pb01 and Pb18 yeast cells Because itraconazole induces changes in transcript levels in the ergosterol pathway and disturbs the total intracellular ergosterol content [15], the localization of ergosterol molecules was assessed in Paracoccidioides Pb01 and Pb18 yeast cells. Ergosterol was detected by its ability to bind to the dye filipin. This characteristic has been used to detect ergosterol in dimorphic fungi [16], yeasts, filamentous fungi [17,18] and mammalian cells [19]. The distribution of ergosterol on the surface of Paracoccidioides Pb01 and Pb18 yeast cells treated with itraconazole was strikingly different from that observed in the control untreated cells. Control cells showed a homogeneous fluorescence distribution ( Figure 3A and C). In contrast, the cells treated with itraconazole displayed dark regions without filipin fluorescence ( Figure 3B and D).

Discussion
Among the Paracoccidioides Pb01 genes regulated by itraconazole were those involved in cellular transport, metabolism/energy, transcription, cell rescue, defense and virulence. Similar and different groups were also observed in other fungi in response to different azoles [8,9,11,12,15] (Figure 5). Among the genes affected, we identified genes in common with other fungi, as well as genes unique to Paracoccidioides. In fact few Paracoccidioides spp. genes were shared with genes from other fungi. This could be due to different techniques and classes of azoles used in the works. The comparison with ither fungi show that cell processes related to stress response, xenobiotic efflux are trigered upon itraconazol in different fungi. The genes exclusively regulated in Paracoccidioides spp. reveal that fungi response to drugs can partially involve specific processes that may be related to different sensibility of differetn fungi to itraconazol treatment. This could be due to different techniques and classes of azoles used in the works.
Although ERG genes were not identified in the RDA experiments, qRT-PCR results showed that ERG11, ERG3, ERG6, ERG5 and ERG25 genes were temporally regulated, particularly after longer contact with the drug (6 h). Acetyl is a carbon donator in the cell production of ergosterol [8]. Acetyl CoA seems to be intensively produced due to up-regulation of transcripts from different metabolic pathways, including lipid degradation by hormone-sensitive lipase (LIPE) and ACAD and amino acid metabolism by IVD. Acetyl CoA pool increasing in the cell is optimized with reduction of aconitase trasncripts (ACO), once this enzymes participates of the acetyl-CoA oxidation in TCA. In addition, the induction of BADH and CYSD could lead to production of thiamine, a cofactor to pyruvate dehydrogenase (PDH), which produces acetyl CoA from pyruvate, whose production is increased by the action of pyruvate kinase (Figure 4).
Ergosterol is produced by the action of erg enzymes [20]. Here, the action of itraconazole on ergosterol biosynthesis and its distribution on Paracoccidioides Pb01 and Pb18 yeast cells surface was documented. Ergosterol is an essential component of fungal plasma membranes; it affects membrane permeability and the activities of membrane-bound enzymes. This sterol is a major component of secretory vesicles and has an important role in mitochondrial respiration and oxidative phosphorylation [21,22]. It can thus be expected that changes in ergosterol levels and in sterol structure could influence the activities of several metabolic pathways. The mechanism responsible for the global up-regulation of ERG genes in response to azoles remains unclear. One theory postulates that depletion of ergosterol or another sterol formed late in the pathway increases global ERG expression; another argues that accumulation of an early substrate or toxic sterol by product induces ERG expression [23].
The correlation between cell wall integrity and perturbation of the ergosterol pathway in T. rubrun suggests that changes in the cell wall may compensate for stress in the plasma membrane [9]. The phospholipid level in the cell membrane seems to be affected in Paracoccidioides Pb01, as indicated by up-regulation of DGAT and phosphatidyl synthase (PHS), which produce phospholipids. DGAT has been found in several transcriptomes to date, indicating it may be important for the fungi response to azoles [15,24].
CHS and their regulatory genes are important for the growth and virulence of human fungal pathogens, including C. albicans [25,26]. It has been observed that high ergosterol levels can inhibit chitin synthases, whereas C. albicans mutants with low ergosterol content showed increased levels of chitin synthesis [27]. CHSr was upregulated in Paracoccidioides Pb01 in the presence of itraconazole.
Glutathione S-transferases, which are important for the detoxification of many xenobiotic compounds, are a family of multifunctional enzymes that play a role in cellular detoxification and excretion of a wide variety of xenobiotic substances [14]. It has been reported that Glutathione S-transferases correlate with fungi defense in response to damage caused by oxidative stress, xenobiotics and antifungal compounds [28]. GST was up-regulated in Paracoccidioides in the presence of itraconazole.
In Paracoccidioides Pb01, genes encoding several classes of transporters were up-regulated upon exposure to itraconazole. MFS transporter and TETA, for example, have been implicated in azole resistance [29]. Drug resistance is often associated with the overexpression of genes encoding efflux pumps, which is presumed to prevent intracellular accumulation of itraconazole in fungus [9,30]. The up-regulation of Paracoccidioides Pb01 MFS, GST and CHSr transcripts also occur in vivo, as demonstrated here by qRT-PCR using RNAs extracted from spleens of mice.
It should be noted that a number of genes involved in small molecule transport, especially in ion transport, were differentially expressed in Paracoccidioides Pb01 in response to itraconazole. Up-regulated genes included CAV, IMP and HLYiii. Down-regulated genes included (CAR) and integral membrane MPV17/PMP22. The inhibition of ergosterol, which is an essential component of fungal biological membranes, including the plasma Figure 4 Hypothetical model for the mode of action of itraconazole against Paracoccidioides. The up-regulation of transcripts such as hormone-sensitive lipase, ADH, IVD and ACO from different metabolic pathways would produce acetyl CoA that would be used for ergosterol synthesis by ERG enzymes. Acetyl CoA would produce phospholipids for the membrane by the action of DGAT and PHS. The induction of BADH and CYSD would lead to production of thiamine, a cofactor of PDH, which would also produce acetyl CoA. GST would conjugate glutathione to xenobiotics and would remove itraconazole from the cell using transporters, allowing for detoxification. membrane, can lead to destabilization of the membrane, leakage of cellular components and influx of extracellular ingredients. Therefore, the regulation of transporter genes is necessary to maintain ionic homeostasis within the fungal cell when membranes are damaged by itraconazole [9,31].

Conclusion
This is the first study to analyze the changes in the Paracoccidioides spp. gene expression profile following triazole exposure. Among the genes affected, we identified genes unique to Paracoccidioides Pb01, as well as genes in common with other fungi. In vitro results were validated by in vivo experiments. The results obtained here should assist in understanding the mode of action of itraconazole in Paracoccidioides spp.

Culture and cell viability
Paracoccidioides Pb01 and Pb18 have been studied at our laboratory previously [32,33]. Pb01 and Pb18 yeast phase was maintained in vitro by subculturing at 36°C in Fava Netto's semisolid medium [34] every seven days. Fava Netto's semisolid medium components were as follows: 1% (w/v) peptone, 0.5% (w/v) yeast extract, 0.3% (w/v) proteose peptone, 0.5% (w/v) beef extract, 0.5% (w/v) NaCl, 4% (w/v) glucose and 1.2% (w/v) agar, pH 7.2. The determination of IC 50 was performed according to Santos et al. [23] and in accordance with the macro dilution method described in the Clinical and Laboratory Standards Institute (CLSI) M27-A2(2005), with modifications. To determine the IC 50 , yeast cells in the exponential growth phase were maintained in the chemically defined Figure 5 Distribution of genes responding to itraconazole in P. brasiliensis isolate Pb01. Data are shown for a subset of genes that were significantly up or down regulated (e-values ≤10 −10 ). The search for functional categories was performed by using the Blast2GO program that joints in one application GO annotation based on similarity searches with statistical analysis and highlight visualization on directed acyclic graphs. GO terms shown are those that were considered significantly over represented by the analysis. Sequences were grouped in functional categories according to the classification of the MIPS functional catalog (Munich Center for Protein Sequences; http://mips.gsf.de/). Specific genes for P. brasiliensis isolate Pb01 are underlined, genes found in other fungi when exposed to itraconazole and other azoles are represented with * and represented with ◊, respectively. Numbers in parentheses represent changes in gene expression. Positive signal indicate induction, and negative indicate repression. solid medium McVeigh Morton (MMcM) [35], for seven days at 36°C and inoculated in liquid MMcM. A stock solution (1 mg/ml) containing sterile itraconazole (Sigma-Aldrich, St. Louis, MO, USA) was prepared in dimethylsulfoxide (DMSO). The final concentration of the solvent in the medium never exceeded 2% (v/v) and had no effect on the cell growth. From this stock solution, the drug was serially diluted in sterile MMcM (pH 7.0), producing a final concentration of 1.25-320 μg/ml (5-1260 mM). The drug concentration range was selected based on previous studies [36]. The controls without antifungal and DMSO were included. The concentrations of inoculums were determined by spectrophotometer using a yeast cell suspension in sterile 0.85% NaCl with 10% transmittance at 520 nm. The mixture was stirred to disperse aggregated cells. Yeast cells were collected from the liquid MMcM and counted in a Neubauer chamber. An initial inoculum containing 5 × 10 6 cells/ml was collected, and 0.1 ml aliquots were added to 2.4 ml of MMcM containing the drug dilutions. The fungus was grown at 36°C under agitation at 150 rpm for five days. The IC 50 was determined using measurements of the turbidity of the medium [37]. The experiments were processed in triplicate.
For viability experiments, yeast cells were grown in the presence or absence of 4 μg/ml (IC 50 ) of itraconazole and were kept in liquid MMcM [35] for 1, 2, 3, 4 and 5 h at 36°C before the viability of the cells was determined by Trypan Blue method [38]. In brief, cells from all incubation times were incubated with a dye solution (0.1% Trypan Blue Stain) for 5 min at room temperature, and viability was assessed by counting viable and unviable cells in a Neubauer chamber.

RDA: RNA extraction and cDNAs synthesis
Paracoccidioides Pb01 yeast cells were cultured in MMcM broth medium in the presence or absence of 4 μg/ml of itraconazole for 1 h and 2 h, corresponding to a viability of 95% and 85%, respectively. For RNA isolation, cells were harvested by centrifugation, washed in cold water and the RNA from driver and tester cultures were extracted with Trizol (Invitrogen, Carlsbad, CA, USA) according to the manufacturer's instructions. RNA quality was assessed using the A 260nm /A 280nm ratio. The RNA was treated with DNAse I RNAse-free (Invitrogen) to remove chromosomal DNA. The concentration and purity of RNA were determined by spectrophotometer, and RNA integrity was visualized after electrophoresis on 1.2% agarose gel. The RNAs were used to construct subtracted libraries and qRT-PCR experiments.
The cDNA fragments used for processing the RDA were generated according to the protocol previously described by Hubank and Schatz [39] and modified by Pastorian et al. [40]. Briefly, first-strand cDNA synthesis was performed with 1 μg total RNA, obtained from driver and tester cultures, using SuperScript III reverse transcriptase (Invitrogen). The first-strand cDNA obtained (3 μl) was used as template to synthesize the second-strand of cDNA. The cDNA was prepared using the SMART PCR cDNA synthesis kit (Clonetech Laboratories, Palo Alto, CA, USA).

RDA: Subtractive hybridization
The cDNAs were digested with the restriction enzyme Sau3AI. Two successive rounds of subtraction employing different adapters (J-Bam and N-Bam, Table 2) were performed to enrich the differentially expressed sequences. Four cDNA-subtracted libraries were constructed. The cDNA libraries containing up-regulated genes were constructed from driver cDNA obtained from Paracoccidioides Pb01 yeast cells grown for 1 h and 2 h in MMcM medium and from tester cDNA, which was synthesized from RNA extracted from Paracoccidioides Pb01 yeast cells grown for 1 h and 2 h in MMcM medium plus itraconazole. The cDNA libraries containing down-regulated genes were constructed from driver cDNA, obtained from Paracoccidioides Pb01 yeast cells, grown for 1 h and 2 h in MMcM medium plus itraconazole and tester cDNA, which was synthesized from RNA extracted from Paracoccidioides Pb01 yeast cells grown for 1 h and 2 h in MMcM medium. The resulting products were purified using a GFX kit (GE Healthcare, Uppsala, Sweden). The tester-digested cDNA, from 1 h and 2 h samples, was linked to adapters (a 24-mer annealed to a 12-mer) and amplified by PCR.
For the generation of the differentially up-and downregulated products, the tester and driver cDNAs of both conditions were mixed separately; the hybridization occurred at 67°C for 18 h and the amplification occurred by PCR using the oligonucleotide matching the 24-mer adaptor [41]. The successive rounds of subtraction and amplification were performed using hybridization testerdriver ratios of 1:10 and 1:100. Adapters (Table 2) were changed between cross-hybridization, and the different products were purified using the GFX kit. After the second subtractive reaction, the cDNA was purified and cloned directly into the pGEM-T Easy vector (Promega, Madison, WI, USA). Escherichia coli XL1 Blue competent cells were transformed with the ligation products. The plasmid DNAs were prepared from selected clones of subtracted libraries and sequenced with the ET Dye Terminator kit Dyenamic (GE Healthcare) in a Mega-BACE 1000 DNA sequencer (GE Healthcare) using primers corresponding to the pGEM-T Easy vector.

Processing and annotation of ESTs
The sequences of at least 75 nucleotides, with a PHRED score ≥ 20 were considered for the assembly and formation of clusters. The assembly of these ESTs was performed using CAP3 [42] and clustered to generate contigs and singlets, which were analyzed. All these tools were integrated in a specific pipeline (http://www.lbm.icb.ufg.br/pipeli-neUFG/). The annotation of genes was performed using the program Blast2GO (http://www.blast2go.org/), which provides a comparison between clusters of sequences obtained from public databases. The BLAST program from the National Center for Biotechnology Information (NCBI) (http://www.ncbi.lm.nih.gov/BLAST), processed with the non-redundant sequences (nr) GenBank and the nucleotide database generated from Paracoccidioides spp. structural genome (http://www.broad.mit.edu/annotation/genome/pa racoccidioides_brasiliensis/MultiHome.html), was used for the annotation. The database sequence matches were considered significant at e-values ≤10 −5 . The program INTER-PROSCAN (http://www.ebi.ac.uk/interpro/) [43] was used

Analysis of RNA transcripts by qRT-PCR
An aliquot of RNA from treated and untreated samples was used to perform reverse transcription qRT-PCR. Total RNAs from Paracoccidioides Pb01 yeast cells cultured in the presence or absence of itraconazole were obtained as previously described, in independent experiments from those used in the RDA assays. After treatment with DNAse, cDNAs were synthesized from total RNA using Superscript III reverse transcriptase (Invitrogen) and oligo (dT) 15 primer according to the supplier's instructions. Gene-specific primers were designed for the selected genes and for the control gene, α-tubulin, using Primer Express software (Applied Biosystems, Foster City, CA, USA) ( Table 2). qRT-PCRs were performed in triplicate in a StepOnePlus™ real time PCR system (Applied Biosystems). The PCR thermal cycling program consisted of 40 cycles of 95°C for 15 sec; 60°C for 1 min. The SYBR green PCR master mix (Applied Biosystems) was supplemented with 1 ρmol of each gene-specific oligonucleotide and 40 ng of template cDNA in a final volume of 20 μl. A curve melting analysis was performed to confirm the amplification of a single PCR product. The data were normalized to the α-tubulin transcript amplified in each set of qRT-PCR experiments. A notemplate control was included. Samples of each cDNA were pooled and serially diluted 1:5 to generate a relative standard curve. Relative expression levels of genes were calculated using the standard curve method for relative quantification [45]. Statistical comparisons were performed using Student's t-test and samples with p-values < 0.05 were considered statistically significant. The specific sense and antisense primers are listed in Table 2. Itraconazole-regulated transcripts were selected for qRT-PCR validation assays.
Preparation of protein extracts and validation of data obtained by specific activity of Glutathione S-Transferase (GST) GST activity was measured with GST assay kit (Sigma-Aldrich). Briefly, the GST Assay Kit employs 1-Chloro-2, 4-dinitrobenzene (CDNB) to produce 1-glutathionyl-2,4-dinitrobenzene (GS-DNB) by conjugation of the thiol group of glutathione (GSH). The reaction product GS-DNB absorbs at 340 nm, and the rate of increase in the absorption is directly proportional to the GST activity of the sample. Protein extracts from Paracoccidioides Pb18 yeast cells were prepared by inoculating 50 ml of Fava Netto's liquid medium with 10 6 cells/ml. Cultures were incubated overnight at 36°C with gentle shaking for 16 h. Cells were centrifuged at 5,000 x g for 5 min and transferred into MMcM media containing itraconazole for 1 h. Control cells were incubated in MMcM without drug. The cells were centrifuged at 10,000 x g for 15 min at 4°C, frozen in liquid nitrogen and disrupted by maceration [46]. Extraction buffer (20 mM Tris-HCl pH 8.8; 2 mM CaCl 2 ) containing a mixture of protease inhibitors (serine, cysteine and calpain inhibitors) (GE Healthcare) was added to the yeast cells. After the addition of glass beads (0.45 mm), the cells were lysed in a bead-beater, followed by centrifugation at 10,000 x g for 15 min at 4°C. The supernatant was collected, and the protein concentrations were determined using Bradford reagent (Sigma-Aldrich). The samples were stored in aliquots at −80°C.
The increase in absorbance is directly proportional to the GST activity. The GST-specific activity is defined as mmol of GS-DNB per mg of total protein per min (mmol/mg/min). The enzymatic activity results represent the mean of three independent determinations, and statistical comparisons were performed using Student's t test. The samples with p-values ≤0.05 were considered statistically significant.

Sterol quantification method
The quantification of total intracellular ergosterol was performed as previously described [47], with slight modifications. Cell extracts from Paracoccidioides Pb01 and Pb18 yeast cells were prepared as already described above. Five ml of 25% alcoholic potassium hydroxide solution (25 g KOH and 35 ml sterile distilled water added to 100 ml 100% ethanol) was added to each tube, and the samples were mixed on a vortex for 2 min. The cell suspensions were incubated in an 85°C water bath for 3 h and allowed to cool to room temperature. Sterols were extracted by addition of 2 ml of sterile distilled water and 5 ml n-heptane (Sigma-Aldrich), followed by vigorous mixing in a vortex mixer for 5 min. The samples were kept at room temperature for 1 to 2 h to allow the phases to separate or were stored at 4°C overnight. One ml of the heptane layer (containing ergosterol) was transferred to a 1.5 ml quartz cuvette and analyzed spectrophotometrically by scanning at wavelengths between 200 and 300 nm. If necessary, the samples were diluted five fold with 100% ethanol and reanalyzed. The ergosterol content as a percentage of the wet cell weight was calculated by the following equations: value 1 = [(A 281.5 / 290) × F]/wet cell weight, value 2 = [(A 230 /518) × F]/wet cell weight, and percent ergosterol = value 1 -value 2. F is the factor for dilution in ethanol, and 290 and 518 are fixed values determined for crystalline ergosterol and 24 (28) dihydroergosterol, respectively.

Fluorescence microscopy
Filipin stained samples were prepared using a previously described protocol for fixing and staining filamentous fungi [48]. Paracoccidioides Pb01 and Pb18 yeast cells were prepared by inoculating 50 ml of Fava Netto's liquid medium with 10 8 cells/ml. Cultures were incubated overnight at 36°C under gentle shaking for 16 h. Cells were centrifuged at 5,000 × g for 5 min and transferred in MMcM media containing itraconazole. Control cells were incubated in MMcM without drug. The fungus was then removed and fixed for 30 min in 3.7% formaldehyde and rinsed with ddH 2 O. A 5 mg/ml stock solution of filipin (Sigma-Aldrich) dissolved in DMSO was diluted to 25 μg/ml and used to stain the fixed samples for 10 min. Samples were then rinsed with ddH 2 O, mounted on a microscope slide and sealed with nail varnish.

BALB/c mice infection with Paracoccidioides Pb18
The animals were bred at the Universidade Federal de Goiás animal facility under specific-pathogen-free conditions. All animal experiments were performed in accordance with the international rules for animal experimentation. The animal protocol was approved by the Universidade Federal de Goiás committee of the ethical treatment of animals (Number: 008/11 CEUA-UFG).
Female BALB/c mice, 8-12 weeks old, were inoculated with 1 × 10 7 of Paracoccidioides Pb18 yeast cells growth in liquid MMcM. In brief, yeast cell suspension in the 7th day of in vitro growth were washed in PBS 1× and inoculated intraperitoneally in mice. The mice were divided into three groups of five animals to be sacrificed 21 days post-challenge. Each group was subdivided by treatment options as follows: five uninfected mice (negative controls), five yeast cell-infected mice (positive controls) and five yeast cell-infected mice treated with itraconazole starting at the third week post-infection. The animals were sacrificed in the sixth week after infection. The spleens were removed and homogenized in 5 ml of sterile PBS 1X. The homogenized sample was plated in brain heart infusion agar supplemented with 4% (v/v) fetal calf serum and 2% (w/v) glucose. The plates were incubated at 36°C and colony-forming units were determined after 20 days.
Gene expression analyses of Paracoccidioides Pb18 from infected mice were performed by isolating yeast cells from spleens as previously described with minor modifications [49]. The spleens of infected mice were homogenized in 1× PBS using a tissue grinder. The homogenate was then filtered using nylon mesh to remove large pieces of animal tissue. The sample was frozen in liquid nitrogen and then centrifuged at 500 × g for 5 min to remove any remaining animal tissue. Next, the sample was centrifuged at 7,000 × g for 15 min to isolate fungal cells. Total RNA was extracted from recovered cells using TRI-ZOL reagent (Invitrogen), according to the manufacturer's instructions. RNA was used to perform qRT-PCR as described above.