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Transcription Factor STE12 Has Distinct Roles in Morphogenesis, Virulence, and Ecological Fitness of the Primary Pathogenic Yeast Cryptococcus gattii

Mycology,¹ Anatomic Pathology Laboratories,² Electron Microscopy Core, Wadsworth Center, New York State Department of Health,³ Department of Biomedical Sciences, School of Public Health, State University of New York, Albany, New York⁴

Received 5 January 2006/ Accepted 23 March 2006

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

 
Cryptococcus gattii is a primary pathogenic yeast, increasingly important in public health, but factors responsible for its host predilection and geographical distribution remain largely unknown. We have characterized C. gattii STE12 to probe its role in biology and pathogenesis because this transcription factor has been linked to virulence in many human and plant pathogenic fungi. A full-length STE12 gene was cloned by colony hybridization and sequenced using primer walk and 3' rapid amplification of cDNA ends strategies, and a ste12 gene knockout mutant was created by URA5 insertion at the homologous site. A semiquantitative analysis revealed delayed and poor mating in ste12 mutant; this defect was not reversed by exogenous cyclic AMP. C. gattii parent and mutant strains showed robust haploid fruiting. Among putative virulence factors tested, the laccase transcript and enzymatic activity were down regulated in the ste12 mutant, with diminished production of melanin. However, capsule, superoxide dismutase, phospholipase, and urease were unaffected. Similarly, Ste12 deficiency did not cause any auxotrophy, assimilation defects, or sensitivity to a large panel of chemicals and antifungals. The ste12 mutant was markedly attenuated in virulence in both BALB/c and A/Jcr mice models of meningoencephalitis, and it also exhibited significant in vivo growth reduction and was highly susceptible to in vitro killing by human neutrophils (polymorphonuclear leukocytes). In tests designed to simulate the C. gattii natural habitat, the ste12 mutant was poorly pigmented on wood agar prepared from two tree species and showed poor survival and multiplication in wood blocks. Thus, STE12 plays distinct roles in C. gattii morphogenesis, virulence, and ecological fitness.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

 
Cryptococcus gattii is an encapsulated yeast that causes cryptococcal meningoencephalitis, a serious brain infection both in immunity-impaired and healthy individuals. A majority of cryptococcosis cases are diagnosed among immunocompromised individuals in whom the causal pathogen is Cryptococcus neoformans var. grubii; a much smaller number of infections are caused by C. neoformans var. neoformans. C. gattii and C. neoformans are closely related pathogenic species, but there are distinct differences in their biological, ecological, genetic, and disease-associated attributes (7, 13-16, 18, 26, 49, 81, 82). C. neoformans var. grubii and C. neoformans var. neoformans remain some of the most intensively studied human fungal pathogens, while experimental studies on C. gattii are still in their infancy. C. gattii was until recently considered a tropical and subtropical pathogen with a prominent association with Eucalyptus trees. Earlier reports from Australia indicated that C. gattii infections are less common among human immunodeficiency virus-AIDS patients than C. neoformans infections. However, as the AIDS epidemic spread around the world, reports started to appear on C. gattii cryptococcosis in human immunodeficiency virus-AIDS patients from Thailand, parts of Africa, and South and Central America (4, 37, 42, 71). Similarly, our analysis of a collection of Cryptococcus isolates from AIDS patients in Southern California revealed about 12% C. gattii strains (12). More recently, an ongoing C. gattii outbreak in healthy humans and animals on Vancouver Island (British Columbia, Canada) has caused multiple fatalities; this is the first documented outbreak in North America (43, 83). Thus, C. gattii continues to pose serious public health problems for immunocompromised and healthy individuals worldwide. Concomitant reports of severe and often fatal disease in animals also raise important concerns for the health of pets and wildlife. Along similar lines, a number of recent reports described the natural isolations of C. gattii from multiple tree species other than the Eucalyptus in Canada, Brazil, and India, thereby expanding the known geographical range and ecological niche of this pathogen around the globe (50, 51, 73). Still, the mechanisms behind host predilection and geographical distribution of C. gattii remain largely unknown, in part due to a paucity of systematic investigations.

STE12 was first identified among a group of Saccharomyces cerevisiae sterile mutants defective in sexual conjugation and related processes (30). Subsequent studies have shown that STE12 is a transcription factor downstream of the mitogen-activated protein kinase (MAPK) cascade that controls mating, filamentation, and cell wall integrity (25, 29). The STE12 is activated by two MAPKS, KSS1 and FUS1; has a transcription partner, TEC1; and has two negative regulators, DIG1 and DIG2 (59). More recently, STE12 was reported to directly regulate expression of over 29 yeast genes that mediate a range of cellular processes, cell cycle, mating projections, cell fusion, polarized growth and budding, stress and/or starvation, and signal transduction (31, 75). The roles of STE12 homologues in various biological processes have thus so far been characterized in few fungi other than S. cerevisiae. In the filamentous model fungus Aspergillus nidulans, the steA mutant is sterile without ascogenous tissue and fruiting body, but there are no effects on either the sexual cycle-specific Hülle cells or a number of asexual developmental programs (87). Among the few pathogenic fungi studied, STE12 homologues have been implicated in the pathogenic process itself. In the rice blast pathogen Magnaporthe grisea, MST12 disruption caused a serious loss of virulence, as the mutant failed to infect rice leaves or onion epidermal cells, even through wound sites (68, 69). The mutation of the STE12 homologue CST1 in Colletotrichum lagenarium, the causal agent of anthracnose disease of cucumber, led to failure of infectious hyphal production from the penetration structure appressoria. This caused a nonpathogenic phenotype on intact leaves but produced disease on wounded leaves (86). The STE12 homologue CPH1 from the common human yeast pathogen Candida albicans was found to be only partially involved in hyphal formation, when a mutant strain was tested on solid medium. However, a double mutation in CPH1 and another gene, PHD1, caused complete loss of filamentation as well as attenuation of virulence in mice (56, 58). In contrast, STE12 from the haploid yeast Candida glabrata, which is increasingly implicated in drug-resistant candidiasis, was found necessary for nitrogen starvation-induced filamentation and for a wild-type level of virulence in mice (6). In the opportunistic human pathogen Penicillium marneffei, stlA gene mutation caused no defects in growth, asexual division, or dimorphic switching, while CLS12, the STE12 homologue in Candida (Clavispora) lusitaniae, was required for mating but dispensable for filamentation (5, 94).

In attempts to understand hyphal formation, a C. neoformans var. neoformans STE12 homolog of the S. cerevisiae STE12 gene was identified. Its overexpression caused hyphal projections and induction of the MF pheromone gene, important for mating reaction, and CnLAC1, the gene that encodes the important virulence factor laccase; the possibility is therefore raised that STE12 provides a bridge between C. neoformans mating type and virulence via melanin production (90). Subsequent study of C. neoformans var. grubii by gene knockout revealed that STE12 was essential for haploid fruiting but was not essential for mating and virulence (95). The results of an STE12 overexpression study by Chang and coworkers were subsequently verified by gene knockout in C. neoformans var. neoformans to show that STE12 was essential for haploid fruiting, melanin production, and virulence but was dispensable for mating (11). A second homolog of C. neoformans var. neoformans STE12 was subsequently identified as MATa specific; it was essential for mating and virulence (10). Interestingly, C. neoformans var. grubii STE12 was later shown to be involved in reversal of hypervirulence of a crg1 mutant, which encodes the regulator of G protein signaling (89). Taken together, these findings suggested that STE12 is co-opted to perform distinct regulatory control functions between closely related C. neoformans varieties. Therefore, we surmised that C. gattii STE12 is potentially a valuable target in studies aimed at unraveling the genetic basis for functional divergence among pathogenic Cryptococcus species.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

 
Strains and media. NIH444 (ATCC 32609, MAT) the wild-type (WT) host for genetic manipulations, NIH198 (MATa; courtesy of K. J. Kwon-Chung, Bethesda, MD), NIH444-ura5 (61), C. gattii BPR17 (ste12 mutant), and C. gattii BPR53 (ste12 plus STE12 reconstituted) were routinely maintained on YPD (yeast extract-peptone-dextrose) agar medium and were stored in 15% glycerol at –70°C. Complete synthetic medium without uracil for STE12 gene disruption and 5-fluoroorotic acid (5-FOA) medium (46) for STE12 reconstitution in the ste12 mutant were used. Niger seed agar (77), Christensen's urea agar, egg yolk agar (19), and limited iron medium with EDTA and bathophenanthroline disulphonic acid (70) were used for the determination of melanin production, urease activity, phospholipase B activity, and capsule induction.

C. gattii STE12 gene characterization and mutation. Primers V564 and V565 were used to PCR amplify a 420-bp fragment of the STE12 gene from the genomic DNA of C. gattii NIH444 (see Table S1 in the supplemental material). The resulting 420-bp fragment was used as a probe for colony hybridization analysis of the C. gattii cosmid library (75). After selection of positive clones, a primer walk strategy was used to obtain the complete sequence of STE12. This sequence was deposited in GenBank (see "Nucleotide sequence accession number" below). To obtain the amino acid sequence of C. gattii Ste12p, we confirmed the C terminus of Ste12p by establishing the polyadenylation site of the STE12 transcript by 3' rapid amplification of cDNA ends. The resulting 1.8-kb product of PCR rapid amplification of cDNA ends was ligated into the TOPO-2.1 TA vector (Invitrogen) and was sequenced.

Phylogenetic analysis of deduced Ste12p amino acid sequences was done with the PAUP v4.0b4a program (84), using a bootstrap method with a neighbor-joining or maximum parsimony search.

The ste12 mutant was generated by homologous recombination of the ste12::URA5 disruption cassette (see Fig. S1A in the supplemental material). The transformants were selected on complete synthetic medium without uracil medium and confirmed for gene deletion at the homologous site by PCR and Southern blotting. The reconstituted strain was generated by homologous integration of the 5.3-kb fragment containing the full-length STE12 gene. Transformants were selected on 5-FOA medium to produce uracil auxotrophic strains resulting from replacement of URA5 at the ste12 locus with the wild-type copy of STE12. The homologous reconstitution of STE12 in the ste12 mutant was again confirmed by PCR and Southern blotting (see Fig. S1B and C in the supplemental material). The original ura5 mutated by selection on 5-FOA of the reconstituted STE12 strain was restored as described previously (62). The reverse transcription (RT)-PCR was performed to confirm the absence and presence of the STE12 message in mutant and reconstituted strains (see Fig. S1D in the supplemental material).

Phenotypic characterization. Capsule production was assayed by incubating cultures in YPD broth overnight at both 30°C and 37°C or in LIM medium for 7 days at 30°C with shaking (180 rpm). The size of the capsule was assessed qualitatively under the light microscope using India ink mounts. The urease, phospholipase B and Cu,Zn superoxide dismutase (SOD) enzyme activities of the test strains were determined as described previously (22, 23, 61).

In vitro growth assessment of all the strains were determined by growing yeast cells in the YPD broth at 30° and 37°C with shaking (180 rpm). An aliquot of cell suspension was withdrawn at 3-h intervals, and the A₆₀₀ was recorded.

A commercial yeast identification system was used to compare assimilation patterns (API 20C AUX; BioMerieux). Additionally, the YT MicroPlate (BiOLOG) was used for the comparison of 94 biochemical tests. The API ZYM test (BioMerieux) was performed per the manufacturer's instructions to compare various enzymatic activities of the test strains.

The cell wall, cell membrane, or specific biosynthetic pathway defects, if any, in the ste12 mutant were analyzed by using a number of chemicals and antifungals per published reports (44). Serial 10-fold dilutions of YPD-grown log-phase cultures of WT, ste12 mutant, and ste12 plus STE12 strains on YPD agar supplemented with calcofluor white (20, 60, 120, or 240 µg/ml), Congo red (20, 50, 100, 200, or 400 µg/ml), sodium dodecyl sulfate (0.005%, 0.01%, 0.03%, or 0.06%), brefeldin (1.0 or 10 µg/ml), mycophenolic acid (5 or 20 µg/ml), amphotericin B (0.5, 1.0, 5.0 or 20 µg/ml), caspofungin (5 or 20 µg/ml), fluconazole (3.0 or 12 µg/ml), itraconazole (0.06, 0.25, or 1.0 µg/ml), ketoconazole (0.03 or 0.06 µg/ml), miconazole (0.03 or 0.06 µg/ml), terbinafine (1.0 or 5.0 µg/ml), voriconazole (0.015 or 0.03 µg/ml), and griseofulvin (2.0, 4.0, 8.0, or 16.0 µg/ml), followed by incubation at 30°C for 7 days.

Melanin production and laccase expression and regulation. Melanin production by the WT, ste12 mutant, and ste12 plus STE12 strains was assayed on Niger seed agar (46). Five microliters of cell suspension (10⁷ cells/ml) from each strain was spotted on the agar surface, and cultures were incubated at 30°C for 3 to 6 days. Copper or cyclic AMP (cAMP)-mediated reversal of melanin pigmentation was tested on Niger seed agar supplemented with either 10 µM to 200 µM CuSO₄ (97) or 2 mM to 50 mM cAMP (3). The laccase activity in the test strains was determined by a previously published method (95). In brief, equal numbers of glucose-starved cells of each strain were used to determine the oxidation of the diphenolic substrate 2,2'-azinobis(3-ethylbenzthiazolinesulfonic acid) (ABTS) (IU of activity = 0.01 A₄₂₀ absorbance unit in 30 min). The transcription of LAC1 was estimated with semiquantitative RT-PCR using the primer pair V1380 and V1381 (78).

Mating and haploid fruiting. The WT, ste12, and ste12 plus STE12 strains were mixed with the compatible mating strain C. gattii NIH198 (MATa, serotype B) on V8 juice agar (pH 7.0) and were incubated at room temperature in the dark for up to 14 days (45, 48). Plates were periodically checked for the appearance of hyphae at the edge of the fungal growth. These edges were examined under the light microscope for the presence of characteristic basidia and basidiospores. Fifty nonoverlapping areas were selected to estimate the extent of mating. V8 juice agar plates supplemented with 2 mM to 50 mM cAMP (Sigma) were used to rescue any mating defect in test strains (1). To further characterize the mating reactions, we used a scanning electron microscope (SEM). The petri plates with mating cultures were flooded with 2% glutaraldehyde in 0.1 M sodium cacodylate buffer (pH 7.4) and were allowed to stand for 3 to 4 h. The fixed cell cultures were flooded with 0.1 M sodium cacodylate buffer once, and blocks, about 4 mm³ in size, of the agar showing hyphal growth on the surface were cut out. These blocks were dehydrated using a graded ethanol series, and they were then critical point dried using liquid carbon dioxide. The dried agar blocks were sputter coated with pure gold and viewed in the SEM.

For the haploid fruiting assay, test strains were patched individually on dry, nitrogen-limited filament agar and incubated for 3 weeks at room temperature in the dark. The edges of fungal growth were photographed under the light microscope (91).

Virulence assays. The pathogenic potentials of the WT, ste12, and ste12 plus STE12 strains were compared in mice models of meningoencephalitis (16, 61). BALB/c and A/Jcr mice (male, 6 to 8 weeks) were procured from Charles River Laboratories, Inc. All procedures for safe and pain-free handling of animals were followed, per the recommendations of the Institutional Animal Care and Use Committee. The log-phase cultures of test strains were resuspended in sterile phosphate-buffered saline, pH 7.4, at a concentration of 1 x 10⁷ cells/ml. Groups of five or six mice were injected intravenously (i.v.) with 10⁶ cells of each strain. The animals were given food and water ad libitum and were observed twice daily for any sign of distress. Mice that appeared moribund or in pain were sacrificed using CO₂ inhalation and cervical dislocation. Survival data from the mouse experiments were analyzed by Kaplan-Meyer survival curves using the SAS system (SAS Institute, Inc.).

Histological lesions were examined in groups of three mice infected with 1 x 10⁵ cells (16). The mice were sacrificed on day 7 postinfection, and the whole brains were removed and fixed in Bouin's fixative. After 24 h of fixation, tissues were sectioned, and brain slices were washed in distilled water for several hours. Processing was done in a vacuum infiltration processor, the Tissue-Tek VIP 5 (Sakura Finetech), starting with 70% alcohol and proceeding through a series of dehydrating alcohols and xylenes into paraffin, for 15 min per station. Tissues were then embedded in paraffin blocks and sectioned at a 7-µm thickness. Sections were stained with hematoxylin and eosin and mucicarmine (Richard Allen Scientific).

To determine the in vivo capsule size of the test strains, 2 mice per strain were injected with 10⁶ cells i.v. At 3 days postinfection, mice were sacrificed using CO₂ inhalation, and the brain tissues were smeared on a glass slide, digested with KOH, and examined under a light microscope using Nomarski optics (Olympus).

Neutrophil (PMN) fungicidal activity. Polymorphonuclear leukocytes (PMNs) were isolated from the peripheral blood of healthy human volunteers by Ficoll-Paque (Pharmacia LKB Biotechnology) centrifugation, as described previously (17). One-hundred-microliter aliquots of PMN, 100 µl of viable yeasts (5 x 10³), and 20 µ1 of pooled human serum were added to the wells of a 96-well tissue culture plate and incubated at 37°C in 5% CO₂-95% air. After incubation for 4 h, the plates were centrifuged at 2,000 rpm for 10 min, and the supernatants were carefully aspirated through 27-gauge needles. The PMN were lysed by the addition of 100 µl of 0.05% Triton X-100, and the yeasts were serially diluted and plated on YPD agar. The YPD agar plates were incubated at 30°C for 2 to 4 days for quantitation of CFU. The results were expressed as the percentage of C. gattii killed [= 1 – (CFU of experiment x CFU of inoculum) x 100]. Values of zero indicated no killing. The study involving human subjects was performed under the guidance of a protocol approved by the Institutional Review Board.

Assessment of pigmentation and growth on wood-based media. The pigmentation and growth of the test strains were assessed on both wood chip and wood extract agar media. Black cherry (Prunus serotina Ehrh) chips were received courtesy of Roger Dziengeleski, Finch, Pruyn & Co., Inc., Glens Falls, NY. Chips were also prepared from Juniperus virginiana (red cedar), Tsuga canadensis (eastern hemlock), Populus tremuloides (trembling aspen), and Acer saccharum (sugar maple) collected from a local forest. These materials were not pretreated with any physical or chemical processes.

The wood agar was prepared by autoclaving 2.0 g of chips at 110°C for 30 min, followed by mixing with 100 ml of autoclaved 2% agar solution. Twenty-five-milliliter aliquots were dispensed in sterile petri plates and were designated wood agar.

Wood extract agar was prepared by mixing of 5.0 g chips in 250 ml of water. This mixture was stirred with magnetic stirrer for 3 h in the cold room, followed by centrifugation at 13,000 rpm for 30 min at 4°C. It was filter sterilized through a 0.22-µm membrane, mixed with 250 ml of autoclaved water containing 4% agar, and dispensed in 25-ml aliquots into sterile petri dishes.

Both wood agar and wood chip agar plates were inoculated with a 5-µl suspension of yeast cell suspensions (10⁷ cells/ml), were incubated for 10 days at 30°C, and were observed periodically for growth and pigmentation.

Wood section microscopy. Black cherry wood blocks (1-cm cubes) were prepared from freshly pruned branches. The blocks were autoclaved at 110°C for 30 min. Sterile blocks were set on 2% sterile water agar in petri plates so that the vessel elements were vertically oriented. The blocks were inoculated with 5 µl of cell suspension (optical density at 600 nm [OD₆₀₀] = 1.0), incubated at 30°C, and observe for up to 8 weeks. Adequate moisture was maintained throughout the incubation period. Finally, the blocks with fungal growth were removed, fixed in formalin for 24 h, and embedded in paraffin, and tangential sections (5 to 7 m) were cut on a rotary microtome. Sections were deparaffinized, covered with glass coverslips, and examined without any staining under the light microscope.

Nucleotide sequence accession number. The complete sequence of STE12 was deposited in GenBank under accession number AY168185.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

 
STE12 gene characterization. The cloned C. gattii STE12 gene was a single copy with approximately 85% nucleotide identity to that of STE12 from C. neoformans var. grubii and C. neoformans var. neoformans (GenBank accession no. AAD 44111 and AAN 75715, respectively). The phylogenetic analysis of protein alignment of the C. gattii STE12 sequence with that of STE12 from C. neoformans var. neoformans, C. neoformans var. grubii, and 11 other fungal species revealed that this protein is segregated into distinct clades of ascomycetous yeasts, molds, and basidiomycetous yeasts, with good bootstrap support. Among basidiomycetes, C. neoformans var. grubii and C. neoformans var. neoformans formed one sister clade distinct from C. gattii. Interestingly, this clustering pattern was not evident for STE12a homologs (Fig. 1). Detailed characterization of the C. gattii STE12 protein revealed STE (amino acids 91 to 203) and C₂H₂-Zn²⁺ motifs (amino acids 543 to 565) (see Fig. S2 in the supplemental material). The STE motif is common in STE12 homologs reported from all fungi, while two C₂H₂-Zn²⁺ motifs have been reported only from STE12 homologs of ascomycetes (6, 30, 53, 66, 86). In silico analyses with deduced amino acid sequences using the PROSITE program (79) found a number of putative phosphorylation sites, including protein kinase C phosphorylation (11 sites), casein kinase II (19 sites), and cAMP- and cGMP-dependent protein kinase (3 sites). Transcriptional activation of STE12 by phosphorylation has been extensively studied in S. cerevisiae (64, 80, 93). The presence of phosphorylation sites has also been reported by bioinformatic analyses of STE12 of Magnaporthe grisea and Colletotrichum lagenarium (68, 69, 86).

View larger version (24K): [in this window] [in a new window]   FIG. 1. Maximum parsimony phylogram of STE12. The alignment of the predicted Ste12p from various fungi was performed using MacVctor 7.1.1 (Accelrys) ClustalW multiple-sequence alignment, with the open gap penalty set at 15.0 and the extend gap penalty set at 0.3. The tree was arbitrarily rooted using Mucor racemosus Ste12p as an out-group. Organism sources and NCBI database accession numbers for sequences are as follows: C. gattii NIH444, AY168185; C. gattii WM276, AY710430; C. gattii E566, AY710429; C. neoformans var. neoformans JEC21, AAN75715; C. neoformans var. neoformans JEC20 STE12, AF542530; C. neoformans var. grubii H99, AAD44111; C. neoformans var. grubii 125.91 STE12, AF542528; Candida glabrata, AJ515385; Emericella nidulans, AAC31206; Kluyveromyces lactis, Q08400; Mucor racemosus, AJ400724; Neurospora crassa, AAK14814; S. cerevisiae, M24502; Candida albicans, A54767; Clavispora lusitaniae, AAD51741; Colletotrichum lagenarium, AB090340; Gibberella zeae, AAM34282; Magnaporthe grisea, AF432913; Penicillium marneffei, AAK21854.

STE12 is required for efficient mating but not for haploid fruiting.

View larger version (98K): [in this window] [in a new window]   FIG. 2. STE12 is required for C. gattii mating. The light microscopic (left panel; magnification, x100) and SEM (right panel; magnification, x6,000) analyses of mating reactions of the WT, ste12, and ste12 plus STE12 strains crossed with the MATa (NIH198) strain are shown. Note the following: profuse filamentation of the WT strain at 5 days postincubation with characteristic hyphae, basidia, and basidiospores; no evidence of mating of the ste12 mutant at 5 days postincubation but sparse mating with occasional basidia and basidiospores observed under SEM; more evidence of mating of the ste12 mutant at 11 days postincubation; recovery of delayed mating in the ste12 plus STE12 strain.

View larger version (76K): [in this window] [in a new window]   FIG. 3. Role of STE12 in C. gattii mating is independent of cAMP pathway. The light microscopic (magnification, x100) analyses of mating reactions of the WT, ste12, and ste12 plus STE12 strains crossed with the MATa (NIH198) with or without cAMP are shown after 5 days of incubation on V8 juice agar. cAMP did not reverse the poor and delayed mating observed in the ste12 strain, while a higher concentration inhibited mating in the WT and ste12 plus STE12 strains.

View larger version (128K): [in this window] [in a new window]   FIG. 4. STE12 is not required for C. gattii haploid fruiting. The light microscopic (left panel; magnification, x100) and SEM (right panel; magnification, x6,000) analyses of haploid fruiting of the WT, ste12, and ste12 plus STE12 strains are shown. The C. gattii strains were patched on dry, nitrogen-limited filament agar medium. The plates were incubated for 3 weeks at room temperature in the dark. The morphological assay showed characteristic filaments, basidia, and basidiospores.

STE12 is not required for several cellular functions.

STE12 is required for melanin pigmentation and laccase expression. Melanization via C. neoformans laccase is an important virulence attribute, and it is down regulated in C. neoformans var. neoformans ste12 mutants (10, 11, 76, 92). Interestingly, the C. gattii ste12 mutant was also defective in melanization and showed weak yellowish pigmentation compared to the dark brown pigmentation formed by WT and ste12 plus STE12 strains on Niger seed agar at 3 days postincubation (Fig. 5A). Supplementation of Niger seed agar with CuSO₄, a metal important in laccase induction, did not restore melanin pigmentation in the mutant strain (data not shown). However, supplementation of the medium with cAMP, important in transcriptional regulation of laccase via parallel or multipath pathways (39), restored melanin pigmentation in the C. gattii ste12 mutant (Fig. 5A). The reduced melanin pigmentation in the C. gattii ste12 mutant was caused by defects in laccase enzyme activity and laccase transcript levels under glucose repression condition (Fig. 5B and C). These results indicated that STE12 regulates the expression of laccase in C. gattii.

View larger version (37K): [in this window] [in a new window]   FIG. 5. STE12 is required for melanin production, laccase enzyme activity, and LAC1 transcript expression. (A) C. gattii strains grown in YPD broth overnight were washed with phosphate-buffered saline, and a 5-µl suspension of 107 cells/ml was spotted on Niger seed agar with or without cAMP and incubated for 3 days at 30°C for melanin production. (B) Laccase enzyme activity from equal numbers of glucose-starved cells (5 h) was determined by measuring the oxidation of the diphenolic substrate ABTS (IU of activity = 0.01 A420 absorbance unit in 30 min). Results are the means ± standard deviations from three individual experiments. The absence of laccase activity in the mutant is consistent with the initial loss of melanization in this strain. (C) Semiquantitative RT-PCR to examine the expression of the LAC1 gene in all of the test strains. Total RNA from each strain was isolated and reverse transcribed (cDNA) with 100-ng aliquots in 1:5 serial dilutions. Actin was used as a control.

STE12 is required for a wild-type level of virulence in mice.

View larger version (40K): [in this window] [in a new window]   FIG. 6. STE12 is required for virulence. (A) C. gattii strains were grown overnight in YPD broth, washed with phosphate-buffered saline, and counted, and 100 µl of suspension containing 106 cells was injected intravenously into 5 (each) BALB/c and A/Jcr mice. Mice were monitored twice daily until moribund. (B) Two mice infected i.v. with 106 cells were sacrificed at 3 days postinfection, and brain tissues were smeared on microscope slides and examined under a microscope using Nomarski optics (magnification, x380).

View larger version (9K): [in this window] [in a new window]   FIG. 7. STE12 is required for fungicidal activity of human neutrophils (PMNs). Human PMN at the effector-to-target cell ratio of 10:1 were inoculated with opsonized C. gattii strains (5 x 103) for 4 h at 37°C in 5% CO2-95% air. The percent C. gattii killed was determined by using the following equation: 1 – (CFU of experiment x CFU of control) x 100. Results are means ± standard deviations from PMNs of three individual donors. The asterisk denotes a P value of <0.05 compared to wild-type and reconstituted strains.

STE12 is involved in wood utilization.

View larger version (72K): [in this window] [in a new window]   FIG. 8. STE12 is involved in C. gattii ecological fitness. (A) C. gattii strains grown overnight in YPD broth were washed in phosphate-buffered saline and counted, and a 5-µl suspension of 107cells/ml was spotted on wood chip-based agar media; (B) 10-fold dilutions of each C. gattii strain, prepared similar to description for panel A, was spotted on wood chip extract agar media. YPD agar was used as a spotting control. All plates were incubated at 30°C for 10 days.

View larger version (93K): [in this window] [in a new window]   FIG.9. STE12 is involved in C. gattii utilization of wood. The black cherry wood blocks (1-cm cubes) were surface inoculated with a 5-µl suspension of 108 cells/ml of each C. gattii strain. These blocks were placed on water agar in petri plates and incubated for 8 weeks at 30°C. Adequate moisture was maintained throughout the incubation period. Blocks with fungal growth were removed and processed for sectioning as illustrated in the accompanying schematics. The diagonal sectioning and selection of wood sections away from the inoculated surfaces allowed an estimation of fungal invasion (schematics). (a, b) WT-inoculated wood sections showing several pigmented yeast cells; (c, d) ste12 mutant-inoculated wood section with few yeast cells with negligible brown pigment; (e, f) wood section inoculated with the ste12 plus STE12 strain showing abundant brown-pigmented yeast cells. V, vessels; P, parenchyma; F, fiber; R, rays. Both rays and vessels showed fungal growth.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Previously, it was reported that STE12 was located within the MAT locus of the C. gattii genome, along with elements of the MAPK signaling cascade, pheromones, receptors involved in mating, housekeeping genes, and putative open reading frames of unknown function (31, 75). The overall organization of the mating locus in C. gattii is quite similar to that in C. neoformans var. grubii and in C. neoformans var. neoformans (31, 41, 75). However, the order and orientation of STE12 vis-à-vis other genes in the locus are not conserved in these fungi, raising the strong possibility that changes in STE12 expression can have occurred due to the positional effect of neighboring genes, as has been reported for other eukaryotic genomes (2, 20, 35, 85).

C. gattii STE12 was required for robust mating, as the ste12 mutant showed poor mating compared to the wild-type and reconstituted strains. Thus, unlike S. cerevisiae and other ascomycetes, the C. gattii ste12 mutant was not sterile but merely mating impaired; it shared this property with similar mutants from C. neoformans var. grubii and C. neoformans var. neoformans (11, 95). Taken together, our study and the two studies just cited provide a unique demonstration of a gene function conserved across all three pathogenic Cryptococcus forms (Table 2). Future studies with a congenic pair of C. gattii strains (MAT and MATa) and genetic epistasis experiments are clearly warranted to define the extent of the conserved role of STE12 in C. neoformans and C. gattii. Conventionally, mating studies in C. neoformans are carried out over a week, a length of time which, in our experience, proved insufficient for the knockout strain. However, when the observation period was extended to 2 weeks and when SEM was used for closer scrutiny of cells at edges of cocultures, a few spots with sparse mating reactions were found in mutant strain. Almost all fungal STE12 knockout mutants to date are reported to have mating or morphogenetic defects, a fact which affirms the central role of this transcriptional regulator in developmental programs. Our current data, taken together with the published literature from C. neoformans var. grubii and C. neoformans var. neoformans, do not identify the mechanism behind the observed partial defect in mating in the mutant strains. Perhaps other transcription factors play an important role in this process, either in association with or independent of STE12.

View this table: [in this window] [in a new window]   TABLE 2. Divergent roles of STE12 revealed by targeted gene disruptions in Cryptococcus neoformans and Cryptococcus gattii

The profound defects in laccase expression, enzyme activity, and melanin production in the C. gattii ste12 mutant strain are consistent with earlier reports from C. neoformans var. neoformans on down regulation or up regulation of laccase levels due to knockout or overexpression of C. neoformans var. neoformans STE12 (11, 90). In contrast, melanin production was reported to be unchanged in the C. neoformans var. grubii ste12 mutant (95). The latter observation highlights another instance in which gene regulation has been conserved between C. gattii and C. neoformans var. neoformans but not in C. neoformans var. grubii, even though C. neoformans var. neoformans and C. neoformans var. grubii are closely related phylogenetically. The results with ste12 mutants in C. gattii and C. neoformans var. neoformans raise the strong possibility that as-yet-undefined activators and/or suppressors of melanin participate in direct or indirect interactions with STE12. Importantly, the addition of cAMP reversed the melanin defect in the C. gattii ste12 mutant strain; a possible interpretation is that cAMP acts to rescue laccase repression by STE12 via parallel or multipath pathways (39). An important role for the cAMP signaling pathway in regulation of C. neoformans melanin production has already been established by means of a number of gene knockout mutants (3, 72). Overall, there is a strong possibility of cross talk between elements of the MAPK and cAMP pathways, which are known to play important roles in mating. A recent discovery of C. neoformans DEAD box RNA helicase VAD1 as a regulator of multiple virulence-associated genes is also highly relevant in this context (67). The vad1 mutant was melanin deficient due to up-regulation of NOT1 (CDC39); the latter acted as an intermediary transcriptional repressor of laccase. NOT1 is part of the Ccr4-Not complex involved in global control of gene expression (21). The involvement of NOT1 in the transcriptional regulation of laccase raised the possibility of direct or indirect interactions with STE12 because some earlier studies have described involvement of CDC36 and CDC39 as negative regulators of the pheromone response in yeast (24, 63). Thus, multiple lines of evidence suggest that regulatory elements in the pheromone response pathway are involved in regulation of laccase expression. Further examinations will be imperative to define the regulatory network for C. gattii laccase. The evidence for other regulatory controls of melanization in fungi comes from the plant pathogens Colletotrichum lagenarium and Magnaporthe grisea. Their respective ste12 mutants have no defects in melanin, which is uniquely produced via polyketide synthesis (34). Melanin biosynthesis is controlled in these two organisms via novel transcription factors containing a Zn(II)₂Cys₆ binuclear cluster motif and a Cys₂His₂ zinc finger similar to motifs present in STE12 (86).

The C. gattii ste12 mutant was significantly less virulent than the wild-type and reconstituted strains in both immunocompetent (BALB/c) and C5-deficient (A/Jcr) mice. This observation was intriguing because we did not observe a down regulation of SOD, phospholipase, and urease or a smaller capsule size, all prominent characteristics of the less-virulent C. neoformans var. neoformans ste12 mutant, although the C. gattii ste12 mutant had a pronounced melanin defect (10, 11). Even though the virulence defect was not seen in the C. neoformans var. grubii ste12 mutant, this mutant also produced a smaller capsule; capsule size is a very important virulence factor (95). The reduced virulence of C. gattii ste12 was one more instance in our study when C. gattii and C. neoformans var. neoformans display an important role for STE12 in animal pathogenesis, functionally diverged from C. neoformans var. grubii. Additionally, we noticed that the C. gattii ste12 strain was severely defective in replication and in cyst formation in the brains of infected mice. The mutant also showed heightened sensitivity to oxidative and nonoxidative killing by phagocytic cells, as evident from experiments with purified human PMN. A common theme in all of the virulence-related observations was the reduced laccase and melanin levels in the C. gattii ste12 mutant in vitro. Laccase in C. neoformans var. neoformans and C. neoformans var. grubii plays important roles in resistance to stress, phagocytic killing, and conversion of dopamine to immunomodulatory products in the host brain (57, 65). By implication, laccase and melanin are likely to play similar roles in C. gattii. The fact that albino strains are not usually seen in clinical cases of cryptococcosis is further evidence for an essential role of melanin in vivo.

We strongly suspected that environmental/nutritional sensing by STE12 by itself is an important fitness attribute missing from ste12 strains, perhaps sufficient to account for their poor pathogenic potential. Support for this assumption comes from mutants of the human pathogen Candida glabrata and the plant pathogens Colletotrichum lagenarium and Magnaporthe grisea, which are all less pathogenic than their wild-type counterparts, in a melanin-independent manner (6, 68, 69, 86). We carried out extensive phenotypic tests to find additional fitness defects in the mutant strain, but these efforts were not successful, possibly due to reliance on laboratory media that are unlikely to reveal subtle STE12 regulatory control over functional genes in vivo. More refined studies are needed to identify diverse gene functions regulated by C. gattii STE12, as was achieved for S. cerevisiae STE12 by means of an exquisite genome-wide location and expression profiling approach (74).

A remarkable observation in this study was the inability of the ste12 mutant strain to produce robust pigmentation on wood chips simulating C. gattii's environmental niche. To our knowledge, this is the first instance in which a gene function has been directly related to the specialized environmental niche of C. gattii or C. neoformans. Our wood chip agar model for testing environmental fitness was validated by the fact that the wild-type and reconstituted strains exhibited robust survival and multiplication on these substrates and produced copious amounts of melanin-like pigment. The poor pigmentation of the ste12 mutant strain could be due to its impaired ability to produce laccase. It may be relevant to recall that filamentous basidiomycetes are the major cause of wood damage in nature (white rot). This process involves breakdown of ligninocellulose by laccase working in concert with other fungal enzymes, mediators, and toxic radicals (52). The essential role of laccase in lignin degradation has also been confirmed by the use of laccase-deficient mutants of the white rot fungus Pycnoporus cinnabarinus (27). A corollary of these destructive fungal activities is represented by the industrial applications of purified laccase in bioremediation (40, 60). The results of our experiments suggest a model in which C. gattii STE12 senses appropriate nutrient/environment cues on the wood surface and responds by up regulation of laccase and melanization for cooperative utilization of substrate. This response was suboptimal in the mutant, due to the absence of Ste12p. Additionally, ste12 mutant cells appeared defective in penetration and proliferation inside wood blocks compared to the WT and ste12 plus STE12 strains. We interpreted this observation as another manifestation of the ste12-associated fitness defect, paralleling the observed defect in colonization and proliferation within mouse tissues (Fig. 9). Thus, STE12 appears to be an important regulatory gene for control of both the saprobic and the pathogenic aspects of the life cycle of Cryptococcus gattii.

	ACKNOWLEDGMENTS

 
We thank S. Narasipura and Adriana Verschoor for helpful discussions and editorial comments. We also thank the four anonymous reviewers for constructive criticisms and suggestions.

Nucleotide sequencing was carried out at the Molecular Genetic Core of the Wadsworth Center.

This study was supported in part by NIH grants AI-53732 (to V.C.) and AI-48462 (to S.C.).

	FOOTNOTES

 
* Corresponding author. Mailing address: Mycology Lab, Wadsworth Center, New York State Dept. of Health, 120 New Scotland Ave., Albany, NY 12201-2002. Phone: (518) 474-4177. Fax: (518) 486-7811. E-mail: vishnu{at}wadsworth.org.

Supplemental material for this article may be found at http://ec.asm.org/.

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Top Abstract Introduction Materials and Methods Results Discussion References

 

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