Figures
Abstract
Cryptococcus neoformans, an AIDS-defining opportunistic pathogen, is the leading cause of fungal meningitis worldwide and is responsible for hundreds of thousands of deaths annually. Cryptococcal glycans are required for fungal survival in the host and for pathogenesis. Most glycans are made in the secretory pathway, although the activated precursors for their synthesis, nucleotide sugars, are made primarily in the cytosol. Nucleotide sugar transporters are membrane proteins that solve this topological problem, by exchanging nucleotide sugars for the corresponding nucleoside phosphates. The major virulence factor of C. neoformans is an anti-phagocytic polysaccharide capsule that is displayed on the cell surface; capsule polysaccharides are also shed from the cell and impede the host immune response. Xylose, a neutral monosaccharide that is absent from model yeast, is a significant capsule component. Here we show that Uxt1 and Uxt2 are both transporters specific for the xylose donor, UDP-xylose, although they exhibit distinct subcellular localization, expression patterns, and kinetic parameters. Both proteins also transport the galactofuranose donor, UDP-galactofuranose. We further show that Uxt1 and Uxt2 are required for xylose incorporation into capsule and protein; they are also necessary for C. neoformans to cause disease in mice, although surprisingly not for fungal viability in the context of infection. These findings provide a starting point for deciphering the substrate specificity of an important class of transporters, elucidate a synthetic pathway that may be productively targeted for therapy, and contribute to our understanding of fundamental glycobiology.
Author summary
Cryptococcus neoformans, the leading cause of fungal meningitis, kills almost a quarter of a million people each year. Carbohydrate structures, including a complex polysaccharide capsule, enable this microbe to resist host defenses and cause disease. The machinery to build these structures is located inside of specific subcellular compartments. However, most of the reactions require as precursors activated sugar molecules that are made in the cell cytosol. To bring these compounds, called nucleotide sugars, to the site of synthesis, the cell expresses specific transporters. One precursor of particular interest is UDP-xylose, which is the donor of the sugar xylose for the synthesis of cryptococcal capsule, proteins, and lipids. We have identified two UDP-xylose transporters, the first discovered in a fungal organism, and characterized their biochemical properties and role in biology and infection. We found that although this pair of proteins shares biochemical functions, including additional transport of UDP-galactofuranose, the two transporters differ in terms of where they are in the cell, when they are expressed, and their transport properties. Cryptococcal cells lacking both proteins do not cause disease in mice, demonstrating the importance of this synthetic pathway. These findings elucidate fundamental biology as well as fungal pathogenesis.
Citation: Li LX, Rautengarten C, Heazlewood JL, Doering TL (2018) Xylose donor transport is critical for fungal virulence. PLoS Pathog 14(1): e1006765. https://doi.org/10.1371/journal.ppat.1006765
Editor: Robin Charles May, University of Birmingham, UNITED KINGDOM
Received: August 9, 2017; Accepted: November 22, 2017; Published: January 18, 2018
Copyright: © 2018 Li et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Data Availability: All relevant data are within the paper and its Supporting Information files.
Funding: This work was funded by National Institutes of Health grants R21 AI109623, R01 GM066303, and R01 AI087794 to TLD, and a Mizutani Foundation for Glycoscience grant to JLH and CR (160151). LXL was partly supported by a National Research Science Award (T32 GM007200), a Sondra Schlesinger Graduate Fellowship (Washington University St. Louis Microbiology Department), and a National Institute of Allergy and Infectious Diseases award (F30AI120339). JLH was supported by an ARC Future Fellowship (FT130101165). Substrates from Carbosource Services (Athens, GA) were supported in part by a NSF-RCN grant (0090281). Glycan compositional and linkage analyses at the Complex Carbohydrate Research Center (Athens, GA) were supported by the Chemical Sciences, Geosciences and Biosciences Division, Office of Basic Energy Sciences, U.S. Department of Energy grants DE-FG02-93ER20097 and DE-FG02-96ER20220. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Introduction
Glycans are critical for the normal development, growth, and viability of organisms across all kingdoms of life. The extensive glycoconjugate repertoire of Cryptococcus neoformans, a ubiquitous environmental fungus, enables this pathogen to cause serious respiratory disease in the setting of immune compromise. This pulmonary infection often progresses to a lethal meningoencephalitis, even with treatment, leading to several hundred thousand deaths each year [1–3].
The major virulence factor of C. neoformans, a polysaccharide capsule, acts as a physical barrier against host defenses when associated with the cell wall and as an immune modulator when shed into the extracellular space [4,5]. This material consists primarily of two complex polysaccharides, glucuronoxylomannan (GXM) and glucuronoxylomannanogalactan (GXMGal) [4]. The more abundant capsule component, GXM, is a linear mannose (Man) polymer with single glucuronic acid (GlcA) and xylose (Xyl) side chains [6]. The second polysaccharide, GXMGal, consists of a galactose backbone modified with single galactofuranose (Galf) residues and galactomannan side chains bearing a variable number of GlcA and Xyl residues [7–9].
Beyond the capsule, C. neoformans glycoconjugates include proteins with N- and O-linked glycans that resemble the corresponding mannose structures of the model yeast Saccharomyces cerevisiae, although they are further modified with Xyl or Xyl-phosphate residues [10–13]. Cryptococcal glycosphingolipids range from simple mannose modification of lipids to more complex structures that also incorporate galactose (Gal) and Xyl [14], and the cryptococcal cell wall consists of glucans, chitin, chitosan, and mannoproteins, many of which bear GPI anchors [15]. These glycans play integral structural and regulatory roles to facilitate fungal survival and pathogenesis [16].
Consistent with the abundant glycosylation of C. neoformans, a significant portion of its genetic machinery and metabolic energy is dedicated to glycan synthesis. These synthetic reactions typically occur in the secretory pathway, although they rely on nucleotide sugar donors that are synthesized in the cytosol [17]. The charged donors enter the luminal space via nucleotide sugar transporters (NSTs), which exchange activated sugars for the corresponding nucleoside monophosphates [18,19]. NSTs thus mediate a limiting step in glycan biosynthesis, and are consequently required for cryptococcal viability and pathogenicity [20–22].
Our focus is on defining glycan synthesis in C. neoformans, motivated by its unique biology and critical role in a deadly disease. Cryptococcal NSTs comprise a key subset of this machinery, which has stimulated us to identify these proteins and their functions. This effort is complicated by the observations that NST homology is not always a reliable predictor of substrate specificity and that NSTs may be functionally redundant. Individual NSTs also range from highly specific single-substrate transporters to more promiscuous, multi-substrate proteins [23–28]. NST substrate specificity may also be modulated by localization to a particular cellular compartment and/or association with other glycan biosynthetic enzymes [21,29].
In prior work, protein structure predictions and homology facilitated identification of the cryptococcal NSTs responsible for GDP-Man [21,30] and UDP-Gal [20,22] transport. We have now used product analysis and mass spectrometry based assays to discover Uxt1 and Uxt2, which both transport UDP-Xyl and UDP-Galf although they exhibit distinct subcellular localization, expression patterns, and kinetic parameters. Cells without these two proteins lack Xyl in all analyzed glycoconjugates and exhibit growth defects and metabolic abnormalities that are present to a lesser extent in single mutant strains. We further made the unexpected finding that transporter function is required for virulence in a mouse model of disease, but not for persistence in that context.
Results
In examining the cryptococcal genome for genes encoding putative NSTs, we discovered a pair of sequences (CNAG_02036 and CNAG_03695) that encoded closely related proteins (57% identity at the amino acid level; S1A Fig). We were interested in these sequences because the level of identity could indicate functional redundancy to ensure the transport of a key glycan precursor, or, in the absence of shared activity, could shed light on mechanisms of substrate specificity.
To assess the biological role of the novel protein pair we had identified, we generated single and double deletion strains. We first tested whether these mutations affected the major cryptococcal virulence factor, its polysaccharide capsule. Composition analysis of capsule GXM showed complete loss of Xyl from the double mutant, while single mutants were less affected (Fig 1A). This suggested that both proteins transported the Xyl precursor UDP-Xyl, so we designated them as UDP-Xyl transporters 1 and 2 (Uxt1 and Uxt2). uxt1Δ GXM had only 20% of the Xyl found in WT material, while uxt2Δ exhibited no defect in composition. Consistent with these results, linkage analysis of GXM mannose residues showed a dramatic shift to less substitution of the mannose backbone in the double mutant, with a slightly lesser shift in uxt1Δ (S1 Table).
(A) Glycan composition of GXM. (B) Cell wall and capsule staining with Calcofluor white (CFW; blue) and anti-GXM mAb F12D2 (green), respectively. Bright field, single channel, and merged images are shown; scale bar = 10 μm.
To further examine the mutant capsules, we used a Xyl-dependent monoclonal antibody to GXM [31]. This antibody, F12D2, labeled both single mutant strains, but not uxt1Δ uxt2Δ (Fig 1B). In this respect the double mutant resembled uxs1Δ, a strain that does not synthesize UDP-Xyl [32]. Both uxt1Δ uxt2Δ and uxs1Δ still bind Xyl-independent anti-GXM monoclonal antibodies (S2 Fig, S2 Table).
We next used an unbiased approach to directly measure UDP-Xyl transport activity and assay for additional transport substrates. To do this, we prepared proteoliposomes from S. cerevisiae heterologously expressing Uxt1 and Uxt2 (Fig 2A). When these were preloaded with UMP we observed import of UDP-Xyl (Fig 2B–2D), consistent with our composition studies and antibody binding results. Transport of UDP-Xyl by both proteins was saturable with substrate concentration (Fig 2E) and time (Fig 2F). Uxt1 had an apparent KM of 1.0 ± 0.2 μM and Vmax of 20.4 ± 0.6 nM s-1 (mean ± SEM of n = 4) with a turnover rate of 0.9 s-1, while Uxt2 exhibited lower affinity and catalytic efficiency with an apparent KM of 2.2 ± 0.5 μM, Vmax of 2.2 ± 0.1 nM s-1, and a turnover rate of 0.4 s-1. These KM values were consistent with the estimated μM physiological concentration of UDP-Xyl (S3 Table).
(A) Immunoblot analysis of microscomes (M) and proteoliposomes (P) prepared from S. cerevisiae expressing vector alone (Control) or V5-tagged Uxt1 or Uxt2 (2.5 μg protein per lane; S, standards; C, control; 1, Uxt1; 2, Uxt2). (B and C) Representative LC-MS/MS spectra of proteoliposomes prepared from (B) control or (C) Uxt1-expressing S. cerevisiae cells, preloaded with 30 mM UMP, and incubated with a mixture of 16 nucleotide / nucleotide sugar substrates (50 μM each, 10 min, 37°C); Peak 1, UDP-Arap; Peak 2, UDP-Xyl; Peak 3, UDP-Araf. (D) Nucleotide sugar uptake into proteoliposomes preloaded with 30 mM UMP. Values were normalized to the total protein content of the proteoliposome preparations. Data represent the mean ± SD of n = 4 assays. *, mixture of UDP-GalNAc and UDP-GlcNAc. (E and F) Proteoliposomes preloaded with 10 mM UMP were incubated for 2 min with UDP-Xyl (E) at variable concentrations (0–100 μM) or (F) for the indicated times with 50 μM UDP-Xyl. Values were normalized to the actual NST content in proteoliposome preparations (S4 Table). Data are the mean ± SEM of n = 4 assays. (G) Nucleotide sugar uptake into proteoliposomes preloaded with 30 mM GMP analyzed as in (D).
We further observed transport of UDP-Galf, the donor of a known capsule component, although assessment of its transport kinetics was hindered by its instability, which necessitates simultaneous synthesis and assay. We also observed transport of UDP-Arap and UDP-Araf (Fig 2C and 2D; S3 Fig), although arabinose has never been reported in C. neoformans. Neither of these donor molecules was detected in our nucleotide sugar analyses (S3 Table).
Surprisingly, Uxt2 was almost as efficient in using GMP as UMP as an antiport substrate for UDP-Xyl and UDP-Galf. In contrast, we observed minimal transport activity over control when Uxt1-bearing proteoliposomes were preloaded with GMP (Fig 2G, S3E Fig). Although Uxt1 and Uxt2 have similar activity, they are clearly not functionally identical at the enzymatic level.
We wondered how Uxt1 and Uxt2, the first reported fungal UDP-Xyl/UDP-Galf transporters, compared to other NSTs with similar substrate specificities. Phylogenetic analysis with known transporters of UDP-Xyl and UDP-Araf placed Uxt1 and Uxt2 closest to the A. thaliana UDP-Araf transporters (UAfT1-4) even though, as mentioned above, arabinose has never been detected in C. neoformans (S1B Fig). Interestingly, Uxt1 and Uxt2 were more divergent from known UDP-Xyl transporters, such as those from human and A. thaliana (S1B Fig), which may be of therapeutic relevance.
Our biochemical and phylogenetic studies did not explain why C. neoformans has two transporters for UDP-Xyl and UDP-Galf, and raised the question of whether they have distinct roles in vivo. To define the physiological roles of Uxt1 and Uxt2, we first examined the expression of UXT1 and UXT2 under nutrient rich and deficient (capsule-inducing) conditions; the latter was tested because of the central role capsule plays in virulence and the differences we had noted in capsule composition. We found that UXT1 expression was not affected by capsule induction, while UXT2 had a lower basal level of expression in rich media (0 h) that was upregulated 15-fold upon capsule induction (Fig 3).
Reads from RNA-Seq data (mean ± SD) during capsule induction (see Materials and Methods) were compiled from three independent experiments, each with RNA prepared from three biological replicates as in [56].
When we expressed FLAG-tagged Uxt1 and Uxt2 in S. cerevisiae to assess their subcellular localization, we found that Uxt2 localized to the ER (Fig 4A). In contrast, Uxt1 exhibited a Golgi distribution (Fig 4B), consistent with its predicted N-terminal ER export signal (two di-acidic motifs). Swapping the N-terminal cytosolic domains of the two proteins caused each to shift to the other secretory compartment (Fig 4, bottom row of each panel).
Sec7-3xGFP S. cerevisiae cells transformed with vector alone (Vector) or vector expressing FLAG-tagged Uxt1, Uxt2, or chimeras of Uxt1 and Uxt2 were stained with DAPI and probed with the indicated antibodies. Bright field, single channel, and merged images are shown (scale bars, 1 μm). Blue, DAPI; red, α-Kar2p/BiP to mark the ER (A) or α-GFP to localize the Golgi marker Sec7 (B); green, α-FLAG. Images are representative of three independent studies.
We wondered if the observed differences in protein expression and localization had phenotypic consequences beyond alterations in GXM. All of the mutants grew normally at 37°C, except for a modest increase in the doubling time of uxt1Δ uxt2Δ, which was further exacerbated by nutrient limitation (S4 Fig). We saw no changes in growth when these strains were challenged with stressors that target the cell wall, consistent with their wild-type patterns of cell wall staining (S2 Table). At this temperature, however, uxt1Δ uxt2Δ growth was abolished by SDS (that of uxt1Δ was slightly inhibited), and the growth of both of these strains was slightly inhibited by high salt (Fig 5A).
(A) 5-fold serial dilutions of the indicated strains, grown on the indicated media at 37°C and photographed after three days. uxs1Δ is included as a control. (B and C) The indicated strains were placed in capsule-inducing conditions (see Materials and Methods) for 24 h, and then visualized by light microscopy after negative staining with India Ink (B, scale bar = 5 μm) or by electron microscopy (C, scale bar = 0.5 μm). Additional EM images are provided in S5D Fig.
Both single uxt mutants showed normal capsule thickness (Fig 5B; S5A Fig), cell diameter (Fig 5B, S5B Fig), and GXM shedding (S5C Fig). The uxt1Δ cells, however, aggregated more than wild type (Fig 5B), and differed from wild-type cells in capsule organization, despite the similarity in overall capsule radius: individual fibers seemed thicker and appeared to form a sparser network over the cell surface (Fig 5C, S5D Fig). The capsule changes were more striking in uxt1Δ uxt2Δ cells; these showed significantly thinner capsules (S5A Fig) and reduced GXM shedding (S5C Fig). Their capsule fibers also appeared shorter and coarser than those of uxt1Δ, resembling those of uxs1Δ cells, which do not synthesize UDP-Xyl (Fig 5C, S5D Fig).
The observed differences in capsule did not explain the increased sensitivity of uxt1Δ and uxt1Δ uxt2Δ to stress, because even acapsular cells grow normally under these conditions [33,34]. We hypothesized that this sensitivity instead results from reduced Xyl in other glycoconjugates, such as protein-linked glycans. In support of this idea, the Xyl content of glycoproteins isolated from uxt1Δ and uxt2Δ was 15% and 90% of their respective complements. We detected no Xyl in samples purified from uxt1Δ uxt2Δ or the control uxs1Δ.
We wondered whether the stress sensitivity and altered glycoconjugate xylosylation of the uxt mutants would translate into aberrant interactions with host cells. Since host macrophages are critical for determining the outcome of cryptococcal infection [35], we investigated the ability of our mutants to interact with bone marrow macrophages (BMM) in vitro. We found that the level of internalization by BMMs was inversely related to the degree of xylosylation: uxt1Δ uxt2Δ was taken up more readily than WT cells while uxt1Δ exhibited an intermediate phenotype (Fig 6A). Notably, while WT and the single deletion strains replicated ~2-fold over 24 h after internalization by BMM, the level of uxt1Δ uxt2Δ did not change (Fig 6B). This reflected both decreased replication and increased clearance, which negated the small growth that occurred (Fig 6C).
(A) Percent phagocytosis (engulfed fungi/initial inoculum) of opsonized fungi. (B) Fold-change in colony-forming units (CFU) 24 h:0 h after internalization. (C) Proportion of daughter cells in the population of WT (dashed line) and uxt1Δ uxt2Δ (black line) cells incubated with BMMs for 0, 24, and 48 h. Data are the mean ± SEM of three independent experiments. *, p < 0.05 by (A, B) one-way ANOVA with Tukey’s post hoc test or (C) Student t-test. (D) Survival of A/JCr mice after intranasal inoculation with 5 × 104 cells of the indicated strains (n = 8–9). (E) Lung CFU of infected mice at the time of death (for WT, uxt1Δ, uxt2Δ, and complemented mutants; n = 8) or at the indicated time points (for uxt1Δ uxt2Δ; n = 3). Open circles, individual mice; black bar, mean; dashed line, initial inoculum. **, p < 0.01 by one-way ANOVA with Tukey’s post hoc test.
The altered host interactions we observed in vitro suggested a potential defect in pathogenicity of the uxt strains. Studies using an inhalational model to mimic the natural route of infection showed that uxt2Δ and, more surprisingly, uxt1Δ, caused disease with normal kinetics (Fig 6D) and organ burdens (Fig 6E, S7 Fig). In contrast, uxt1Δ uxt2Δ was attenuated for virulence in both A/JCr and C57BL/6 mice (Fig 6D, S6 Fig). More detailed studies using A/JCr mice showed that the double mutant was unexpectedly detectable in the lungs out to 100 days post infection (dpi), when the experiment was terminated (Fig 6E). Despite the persistent pulmonary burden, uxt1Δ uxt2Δ failed to disseminate from the lungs; it was never detected in the spleen and was only transiently detected in the brain (S7 Fig).
Discussion
C. neoformans encodes an unusual pair of highly homologous UDP-Xyl/UDP-Galf transporters, which together are critical for virulence. Uxt1 and Uxt2 are unique for their high affinity for UDP-Xyl (Fig 2), with KM values almost two orders of magnitude lower than those of the Arabidopsis UDP-Xyl transporters [36]. Despite transporting the same nucleotide sugars, the two proteins are not completely functionally redundant, likely due to differences in expression, enzyme kinetics, and localization.
Beyond nucleotide sugars known to occur in C. neoformans, in vitro Uxt1 and Uxt2 also transport UDP-Arap and UDP-Araf (Fig 2), potentially enabled by the similar structures of Xyl and Ara (D-Xyl and L-Ara are epimers). While the NSTs most closely related to Uxt1 and Uxt2 (At UAfT1-4) are highly specific for UDP-Araf [37], the substrate range of the cryptococcal proteins most closely resembles that of plant UDP-Xyl transporters (UXT1-3;[36]) despite their sequence divergence (S1B Fig). These observations highlight the importance of using rigorous biochemical analysis to test functional assumptions based on homology.
Since UDP-Ara is not found in cryptococcal cells and abrogating UDP-Galf synthesis does not alter cryptococcal growth or virulence [8], the phenotypes associated with loss of Uxt1 and Uxt2 likely result from disruption of UDP-Xyl transport into the secretory compartment. Notably, capsule material was still produced (Fig 5) even when no Xyl was detected in GXM because both transporters were absent (Fig 1A). This suggests that Xyl incorporation is not required for GXM backbone synthesis or elongation, or for incorporation of GlcA. However, lack of the Xyl donor did reduce the amount of shed capsule material by over 75% (S5C Fig). Since Xyl constitutes only 20–30% of the capsule mass, loss of this moiety alone does not explain this reduction. Instead, it may be a direct effect of the reduced Xyl incorporation, if these side chains are needed for capsule recognition by synthetic or trafficking machinery, or an indirect effect, for example if synthetic enzymes must be xylosylated to function efficiently. Lack of UDP-Xyl transport also yielded thinner capsules (Fig 5B, S5A Fig) with abnormal fiber morphology (Fig 5C, S5D Fig); this presumably results from the lack of Xyl substitution, which may be required for proper conformation or organization of capsule polysaccharides.
Why does C. neoformans express two UDP-Xyl transporters? Judging by the severity of mutant phenotypes (Fig 5) and the gene expression levels (Fig 3), Uxt1 is the major transporter of the pair, but loss of both is required to eliminate Xyl incorporation (Fig 1). These data exclude the possibility of a third UDP-Xyl transporter of any significance, while highlighting the unequal contribution of these two proteins. One factor in this inequity is likely the higher affinity and catalytic efficiency for UDP-Xyl transport of Uxt1 compared to Uxt2 (Fig 2). Another is probably their distinct regulatory patterns, with UXT1 expressed constitutively, while UXT2 expression levels is upregulated in response to greater glycan biosynthetic demands (Fig 3). Curiously, expression of the two genes was not optimally regulated to enable compensation in the single mutants: expression of UXT1 did not change in response to the loss of UXT2 even in capsule-inducing conditions, and the normal UXT2 induction was muted in the absence of UXT1 (S8 Fig). Future studies will address this regulatory relationship.
The distinct roles of Uxt1 and Uxt2 also potentially reflect their association with other glycan synthetic proteins, such as glycosyltransferases. We found no evidence of association with specific xylosyltransferase(s), as for example preferential loss of β-1,2 or β-1,4 linked Xyl in the GXM of either mutant (S1 Table). However, the full cryptococcal glycan repertoire is not known; future studies may enable us to identify specific protein or lipid modifications enabled by each enzyme. Another factor in the dominant role of Uxt1 is likely its localization to the Golgi (Fig 4B), the probable site of capsule and protein xylosylation [10,11,14], in contrast to the ER localization of Uxt2 (Fig 4A). The latter is intriguing, as this compartment is upstream of most glycan synthesis. It is possible that Uxt2 has transport-independent functions, or that it supplies novel synthetic processes that have yet to be described. These will be exciting areas for future investigation.
The increased sensitivity to stress (Fig 5A) and greater uptake by host phagocytes (Fig 6A) of uxt1Δ were insufficient to alter its behavior in animal infection (Fig 6D). We expected the highly impaired double mutant uxt1Δ uxt2Δ, which cannot transport UDP-Xyl into the secretory pathway, to behave like strains that cannot synthesize UDP-Xyl (uxs1Δ), which are avirulent and completely cleared by 7 days post-infection [38]. Surprisingly, this mutant persisted in the lungs (Fig 6E), suggesting either a cytosolic role for UDP-Xyl or a UDP-Xyl-independent role for Uxs1; these possibilities remain to be investigated.
The double mutant population increased very slowly in both A/JCr and C57BL/6 mice, likely due to its slower growth rate under stress (Fig 6C, S4 Fig) and reduced ability to resist host defenses (Fig 6A and 6B). Xyl modifications have been identified as immunodominant epitopes in antibody responses to allergens and pathogens [39,40], and the absence of Xyl modifications in uxt1Δ uxt2Δ did increase immune detection and clearance of the pathogen in vitro (Fig 6A and 6B). The mutant also remained confined to the lungs of A/JCr mice (S7 Fig) and was slow to cause lethal meningoencephalitis in C57BL/6 mice (S6 Fig). This may reflect an inability to disseminate or to efficiently establish infection at distal sites, or may be the result of active restriction by the immune system. Notably, phagocytes have a multifaceted role in cryptococcal infection, potentially aiding and/or inhibiting fungal survival and dissemination depending on the circumstance [35]. Elucidating the complex interplay between Uxt mutants and the infected host will be the focus of future work. Further studies may also uncover facets of this infection that could be exploited for therapeutic intervention and potentially inform vaccine design.
C. neoformans is unusual among yeast for its extensive utilization of Xyl, in capsule polysaccharides, N- and O-linked glycans (including a unique Xyl-phosphate modification), and glycoplipids. By elucidating UDP-Xyl transport, we have expanded our understanding of this aspect of cryptococcal glycan biosynthesis, including the sequence and localization of capsule synthetic events, and of NSTs as a protein family. We have identified the first fungal UDP-Xyl/UDP-Galf transporters and also set the stage for studies of an unusual mutant that may help elucidate mechanisms of cryptococcal pathogenesis and host response.
Materials and methods
Sequence and phylogenetic analysis
Uxt1 and Uxt2 were identified by BLASTP searches of known NSTs against C. neoformans predicted proteins (Broad Institute; Cryptococcus neoformans var. grubii H99 database); the closest related sequence was that of the Aspergillus fumigatus UDP-Galf transporter (ACR56866.1). The online Phylogeny.fr program (http://www.phylogeny.fr/.version2_cgi/index.cgi) with default settings [41,42] was used for multiple sequence alignment (MUSCLE; [43]), phylogenetic analysis (PhyML; [44]), and tree rendering (TreeDyn; [45]) of Uxt1 and Uxt2 and other NSTs. These included transporters of UDP-Galf (Aspergillus fumigatus, Af), UDP-Xyl (Homo sapiens, Hs, UXT NP_116215.1; Arabidopsis thaliana, At, UXT1 NP_850120.3 (At2g28315), At UXT2 NP_180604.4 (At2g30460), and At UXT3 NP_172172.2 (At1g06890)), and UDP-arabinofuranose (At UAfT1 NP_568469.1, At5g25400; At UAfT2 NP_196684.1, At5g11230; At UAfT3 NP_194965.1, At4g32390; At UAfT4 NP_180122.1, At2g25520), as well as other cryptococcal (Cn) NSTs.
Sequence alignment between Uxt1 and Uxt2 was analyzed using T-coffee (http://tcoffee.crg.cat/apps/tcoffee/do:regular) and formatted using Boxshade (http://www.ch.embnet.org/software/BOX_form.html). The protein sequences were analyzed for predicted localization signals using LocSigDB (http://genome.unmc.edu/.LocSigDB/; [46]).
Cell growth
C. neoformans strains were grown in YPD medium (1% w/v BactoYeast Extract, 2% w/v BactoPeptone, 2% w/v dextrose) at 30°C with shaking (230 rpm) unless otherwise noted. For phenotypic analysis, cells were grown overnight (O/N), washed in sterile phosphate buffered saline (PBS), and diluted to 106 cells/mL in PBS. 4 μL aliquots of serial 5-fold dilutions were plated and grown at 30 or 37°C as indicated. The stress conditions tested included YPD containing 0.01% SDS, 1.2 M NaCl, 1.2 M KCl, Tris pH 8.8, 1.5 M Sorbitol, 0.05% Congo Red (CR), or 2% Calcofluor White (CFW). To test oxidative and nitrosative stress sensitivity, dilutions were spotted onto solid YNB medium (0.67% w/v yeast nitrogen base without amino acids, 2% w/v glucose, 2% w/v agar, 25 mM sodium succinate, pH 4.0) supplemented with 0.5 mM hydrogen peroxide (H2O2) or 0.5 mM sodium nitrite (NaNO2). To assess cell-associated melanin production, 5 μL of a 106 cells/mL solution was plated on agar plates containing 8 mg/mL KH2PO4, 2 mg/mL glucose, 2 mg/mL L-glycine, 1 μg/mL D-biotin, 1μg/mL thiamine, 0.92 mg/mL MgSO4 7H2O, and 0.4 mg/mL L-3,4-dihydrohyphenylalanine (L-DOPA; Sigma-Aldrich). To assay growth, cells were cultured O/N; washed in sterile PBS; resuspended at 105 cells/mL in 30 mL of YPD, YNB, DMEM, or RPMI; and incubated at 37°C for 120 h, with triplicate samples counted by hemocytometer at various times.
C. neoformans strains
We replaced UXT1 in KN99α (WT) with a nourseothricin (NAT) resistance marker using a split marker strategy [47]. Transformants of interest were identified by resistance to NAT and validated by PCR verification of gene replacement. We used a similar strategy to complement the uxt1 deletion strain at the endogenous locus by replacing the deletion cassette with UXT1 in tandem with a G418 resistance marker. Transformants resistant to G418 and sensitive to NAT were verified by PCR and assessed for reversal of mutant phenotypes (see Results). We generated uxt2Δ and UXT2 with an identical approach, using G418 and NAT markers in the deletion and complement constructs, respectively. To obtain an uxt1Δ uxt2Δ double mutant, we crossed the single mutants on V8 agar plates [48]. Double mutants were selected for by resistance to both drugs and verified by PCR amplification.
Capsule induction and visualization
O/N cultures of C. neoformans were collected by centrifugation, washed twice with sterile PBS, diluted to 106 cells/mL in DMEM and incubated at 37°C in 5% CO2 for 24 h in T-75 tissue culture flasks or 24-well plates. The cells were then washed and resuspended in PBS, mixed with 1.5 parts India Ink, and viewed by light microscopy with a ZEISS Axioskop2 MOT Plus microscope (Carl Zeiss Microscopy, LLC).
For antibody detection of cell wall-associated GXM, strains were induced as above for 24 h, fixed for 1 h in 3.7% formaldehyde, washed in PBS, and then incubated for 1 h at room temperature (RT) with 1 mg/mL of anti-GXM monoclonal antibody (mAb) F12D2 or 302 (from Dr. Thomas R. Kozel, University of Nevada School of Medicine) conjugated to AlexaFlour 488. Stained cells were washed twice with PBS, resuspended in PBS, and examined on a ZEISS Axioskop 2 MOT Plus microscope.
GXM ELISA
GXM content of supernatant fractions from cell cultures was quantified by ELISA according to previous methods [49], using anti-GXM mAb 339 (from Dr. Thomas R. Kozel, University of Nevada School of Medicine).
Glycan isolation and analysis
GXM was isolated from strains of interest by selective precipitation of culture supernatants with hexadecyltrimethylammonium bromide (CTAB) as detailed in [11]. For isolation of soluble glycoproteins, O/N cultures were diluted into YPD and grown to 107 cells/mL. 2 x 107 cells per strain were collected, washed in Tris-EDTA buffer (100 mM Tris pH 8.5, 0.1 mM EDTA pH 8.0), and resuspended in 40 mL Tris-EDTA buffer with protease inhibitors. Samples were then subjected to 15 cycles of bead beating (3 min) alternating with 3 min on ice, which yielded ~75% cell lysis (as judged by microscopy). All subsequent steps were performed at 4°C. Lysates were collected, pooled with three 10 mL rinses of the beads, and subjected to a clearing spin (1000 x g; 25 min). Supernatant fractions were then transferred to fresh tubes, adjusted to a final concentration of 1% CHAPS, incubated with rocking for 2 h, and subjected to ultracentrifugation (75000 x g; 45 min). The CHAPS extract was then dialyzed (8000 Mr) against 2 L of 50 mM NH4HCO3 with three buffer changes over 48 h, lyophilized, and washed with 80% acetone to reduce detergent and polymeric contaminants.
For compositional analysis, per-O-trimethylsilyl (TMS) derivatives of monosaccharide methyl glycosides were produced from the GXM samples by acidic methanolysis using methods described in [50,51]. Glycosyl composition was then determined by combined gas chromatography/mass spectrometry (GC/MS) on an Agilent 7890A GC interfaced to a 5975C MSD (mass selective detector, electron impact ionization mode; Agilent Technologies) with a Supelco EC-1 fused silica capillary column (30 m × 0.25 mm ID; Sigma-Aldrich). For linkage analysis, GXM samples were permethylated, depolymerized, reduced, and acetylated as described in [7]. The resultant partially methylated alditol acetates (PMAAs) were then analyzed as above but using a 30 m Supelco SP-2331 bonded phase fused silica capillary column (Sigma-Aldrich).
Heterologous expression, reconstitution, and transport assays
The UXT1, UXT2, GMT1, and GMT2 coding regions were amplified from WT cDNA and introduced into the pENTR/SD/D-TOPO vector (Life Technologies) according to the manufacturer’s protocols to generate pENTR-UXT1, pENTR-UXT2, pENTR-GMT1, and pENTR-GMT2. Recombination of each entry clone with destination vector pYES-DEST52 (Life Technologies) using LR clonase II (Life Technologies) produced a C-terminal His/V5 epitope fusion that was verified by sequencing before transformation into S. cerevisiae strain INVSc1 (Thermo Fisher Scientific). Heterologous expression, reconstitution into proteoliposomes, and transport assays were performed as previously described [52]. UDP-Galf was prepared from UDP-galactopyranose (UDP-Galp) according to [53]. Protein expression and incorporation was verified by polyacrylamide gel electrophoreses and immunoblot analysis of 2.5 μg of microsomes or proteoliposomes using anti-V5 antibody (Thermo Fisher Scientific), also as previously described [52]. Kinetic parameters were calculated by non-linear regression using the Prism 6 application (GraphPad Sofware). The assay was validated and its sensitivity confirmed using the well-characterized GDP-Man transporters Gmt1 and Gmt2 (S9A Fig). Both proteins transported GDP-Man and smaller amounts of other GDP-sugars in exchange for GMP and, significantly less efficiently, UMP (S9D and S9E Fig).
Nucleotide sugar measurement
Nucleotide sugars were extracted from approximately 50 mg of ground cells (wet weight) as previously described [54]. Four biological replicates were processed per strain and condition, and then analyzed in duplicate by LC-MS/MS using porous graphitic carbon as the stationary phase on an 1100 series HPLC system (Agilent Technologies) and a 4000 QTRAP LC/MS/MS system (Sciex) equipped with a TurboIonSpray ion source as in [55]. Results in pmol mg-1 wet weight were converted to concentrations using a cell volume of 47.7 μm3 (based on the average radius of 107 cells, measured by cellometer (Nexcolom Bioscience LLC; n = 3)) and a mass of 4.35 x 10−8 mg/cell (based on weighing a known number of cells; n = 3).
Protein localization
For expression in S. cerevisiae, UXT1 and UXT2 were amplified from WT cDNA, cloned into the copper-inducible expression vector pYEScupFLAGK [26], and transformed using lithium acetate into S. cerevisiae strain Sec7-3xGFP (from Dr. Benjamin S. Glick, University of Chicago). To generate N-terminal swaps of Uxt1 and Uxt2, we amplified both genes from the start codon to the beginning of the first predicted transmembrane domain (UXT1 bp 1–135, UXT2 bp 1–180) and from the first transmembrane domain until the stop codon (UXT1 bp 136–1032; UXT2 bp 181–1068), using WT cDNA as a template. We then PCR amplified to fuse the N-terminal region of UXT1 to the transmembrane region of UXT2 and vice versa, cloned each construct into pYEScupFLAGK, and transformed into S. cerevisiae Sec7-3xGFP as above. All constructs were verified by sequencing.
For localization, cultures were grown O/N in synthetic complete media without uracil (SC-URA), adjusted to OD 0.5 and 0.5 mM CuSO4, and cultured for an additional hour. The cells were then fixed for 30 min in 1% paraformaldehyde, washed and resuspended in 0.1M KPO4/1.2 M sorbitol, and incubated for 15 min in the same buffer containing β-mercaptoethanol and zymolase (100 μg/mL). 15 μL of the cells were then spotted onto polylysine-coated slides (Electron Microscopy Sciences), incubated for 10 min, and plunged into methanol for 5 min followed by acetone for 30 sec. The samples were blocked with 5% goat serum in PBS for 30 min, and stained O/N at 4°C with anti-FLAG (Mouse, 1:1000; Invitrogen) and anti-Kar2p/BiP antibody (Rabbit, 1:1000; from Dr. Jeff Brodsky, University of Pittsburgh). Finally, cells were incubated for 2 h with AlexaFluor 594-tagged goat anti-mouse IgG, AlexaFluor 488-tagged goat anti-rabbit IgG (Thermo Fisher Scientific), and DAPI (Thermo Fisher Scientific), and viewed with a ZEISS Axioskop2 MOT Plus microscope.
Fungal gene expression
Wild-type cells cultured O/N in YPD were placed in DMEM capsule-inducing conditions and sampled at 0, 1.5, 3, 8, and 24 h for RNA isolation and sequencing as in [56]. Additional samples were collected at 0 and 24 h for qPCR analysis. Levels of UXT1, UXT2, and the reference gene ACT1 were quantified using the CFX96 Real Time System (BioRad). All sample reactions contained 1 μL cDNA (100 ng), 4 μL of each primer (200 nM), and 10 μL SYBR Select Master Mix (Applied Biosystems). qRT-PCR was performed in triplicate for each sample and non-template controls (for each set of primers) using 15 min activation and denaturation at 95°C followed by 40 cycles of 15 sec at 95°C, 30 sec at 60°C, and 30 sec at 72°C. Baseline and threshold values were determined for all reactions using CFX manager software (BioRad) and exported to Microsoft Excel for additional analysis using the ΔCq method.
Electron microscopy
Strains were induced for capsule (as above), collected by centrifugation, fixed for 1 h at RT with 2% glutaraldehyde (Polysciences Inc.) in 100 mM phosphate buffer (pH 7.2), and incubated for 1 h in 1% osmium tetraoxide (Polysciences Inc.). Cells were then dehydrated with ethanol and propylene oxide and embedded in Eponate 12 resin (Tel Pella Inc.). 70 to 90 nm sections were cut with an UCT ultramicrotome (Leica Microsystems Inc.) and stained with uranyl acetate and lead citrate for visualization with a JOEL 1200EX transmission electron microscope (Joel Inc.).
Macrophage assays
Bone marrow (BMMs) from the femurs and tibiae of C57BL/6 mice (Jackson Laboratory) was incubated for one week at 37°C and 5% CO2 in BMM medium (20% FBS, 30% L-cell supernatant, 1% Penicillin-Streptomycin in RPMI), which was refreshed 4 and 6 days after plating. Cells were harvested on day 7 by incubation in ice-cold PBS for 10 min and BMM were purified from the population by positive selection using biotinylated α-F4/80 antibody (eBioscience) and anti-biotin conjugated magnetic beads (Miltenyi Biotec). BMMs were then plated in 24-well plates at 3.5 x 105 cells/mL of R10 media, and incubated O/N at 37°C and 5% CO2. On the following day, log-phase fungi were collected by centrifugation, washed, and opsonized with mouse serum (40%) for 30 min at 37°C. The strains were then washed with PBS, resuspended at 3.5 x 104 cells/mL in DMEM, and incubated with macrophages for 1 h. Samples were washed twice with PBS, and lysed using water either immediately or after 24 h incubation in DMEM at 37°C and 5% CO2. For CFU quantification, the lysates and initial inocula were plated on YPD agar. Results were analyzed using one-way analysis of variance (ANOVA) with Tukey’s post-hoc test. For assays distinguishing parental and daughter cells, fungi were also stained with Oregon Green 488 dye (2 μg/mL; ThermoFisher) in 0.1 M sodium bicarbonate (pH 8.0) for 1 h at room temperature prior to opsonization and then treated as described above. Following lysis, cells were stained with calcofluor white (2 mg/mL PBS) for 30 min before flow analysis with a BD LSRFortessa X-20 using OneComp eBeads (eBioscience) for compensation controls. Data were analyzed using FlowJo (Treestar) and compared using Student’s t-tests.
Animal studies
Fungal strains were cultured O/N in YPD, washed, and diluted to 106 cells/mL in sterile PBS. 50 μL aliquots of each strain were inoculated intranasally into groups of eight 6- to 8-week-old female A/JCr (National Cancer Institute) or C57BL/6 (Jackson Laboratory) mice. Infected mice were weighed daily and sacrificed if they lost >20% relative to peak weight, or on day 49, 63, or 100 post infection, whichever came first. Lung, brain, and spleen homogenates were harvested and plated for CFU at time of death or indicated time points, and organ burdens were analyzed by ANOVA with Tukey’s post-hoc test.
Ethics statement
All animal studies were approved by the Washington University Institutional Animal Care and Use Committee (Protocol #20140184). All research involving animals was carried out in strict accordance with the “Guide for the Care and Use of Laboratory Animals” published by the National Research Council and endorsed by the Association for the Assessment and Accreditation of Laboratory Animal Care.
Supporting information
S1 Fig. Conservation of cryptococcal nucleotide sugar transporters.
(A) Protein sequence alignment of Uxt1 and Uxt2 (CNAG_02036 and CNAG_03695) with conserved residues highlighted (black, identical residues; grey, conserved substitutions). (B) Phylogenetic relationships of C. neoformans (Cn) NSTs (including Uxt1 and Uxt2, in bold), and UDP-Xyl, UDP-Galf, and UDP-Arap transporters from other organisms (Hs, Homo sapiens; Af, Aspergillus fumigatus; At, Arabidopsis thaliana) using MUSCLE, PhyML, and TreeDyn software (see Materials and Methods). Branch lengths are drawn to scale.
https://doi.org/10.1371/journal.ppat.1006765.s001
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S2 Fig. uxt1Δ uxt2Δ is recognized by Xyl-independent capsule antibodies.
Cells from the indicated strains were incubated with calcofluor white (CFW; blue) to stain the cell wall and anti-GXM mAb 302 to visualize the capsule (green). Bright field, single channel, and merged images are shown; scale bar = 10 μm. cap59Δ is an acapsular strain included as a control.
https://doi.org/10.1371/journal.ppat.1006765.s002
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S3 Fig. Uxt1- and Uxt2-mediated UDP-Galf uptake into proteoliposomes.
(A) LC-MS/MS analysis of UDP-Galf prepared from UDP-Galp utilizing E. coli UDP-galactopyranose mutase (GLF). (B-D) Proteoliposomes prepared from S. cerevisiae expressing vector alone (B), Uxt1 (C), or Uxt2 (D) were preloaded with 30 mM UMP, and analyzed by LC-MS/MS after a 10 min incubation with 700 μM UDP-Galp and 10 μg purified GLF. Based on mass and retention time, the minor peak between UDP-Galp and UDP-Galf is likely UDP-Glc, presumably present in the reaction starting material. (E and F) Quantification of nucleotide sugar uptake into proteoliposomes preloaded with 30 mM UMP (E) or 30 mM GMP (F). Amounts were calculated using a UDP-Galp standard and normalized to the total protein content of the proteoliposome preparations and the mean ± SD of four assays are plotted. All assays were performed at 37°C.
https://doi.org/10.1371/journal.ppat.1006765.s003
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S4 Fig. uxt1Δ uxt2Δ growth is restricted at 37°C.
The indicated C. neoformans strains were grown overnight at 30°C in YPD, diluted to 105 cells/mL in the media indicated, and incubated at 37°C with 5% CO2. The results shown are the averages of three measurements. Black, WT; red, uxt1Δ; green, UXT1; purple, uxt2Δ; blue, UXT2; grey, uxt1Δ uxt2Δ (continuous and dashed lines, representing three independently obtained double deletion strains).
https://doi.org/10.1371/journal.ppat.1006765.s004
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S5 Fig. Morphological defects of uxt1Δ uxt2Δ.
Induced cells were stained with India Ink, and the radius of the capsule (A) and diameter of the cell body (B) were measured using ImageJ (100 cells counted per strain; mean ± SEM of three biological replicates). (C) GXM shed from equal numbers of each of the indicated strains was quantitated by ELISA (see Materials and Methods). Data is the mean ± SEM of three independent experiments. *, p < 0.05, one-way ANOVA with Tukey’s post-hoc test. (D) Electron micrographs of the indicated strains induced for capsule as in Fig 5. Two representative images are displayed for each strain. Scale bar = 0.5 μm.
https://doi.org/10.1371/journal.ppat.1006765.s005
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S6 Fig. uxt1Δ uxt2Δ is severely attenuated for virulence in C57BL/6 mice.
Survival of C57BL/6 mice after intranasal inoculation with 5 × 104 cells of WT (n = 5) or uxt1Δ uxt2Δ (n = 19). C57BL/6 mice naturally skew towards a non-protective Th2-type response, which increases their susceptibility to cryptococcal infection compared to A/JCr mice [57].
https://doi.org/10.1371/journal.ppat.1006765.s006
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S7 Fig. uxt1Δ uxt2Δ does not colonize extrapulmonary sites.
Brain (A) and spleen (B) CFU of infected A/JCr mice at the time of death (for WT, uxt1Δ, uxt2Δ, and complemented mutants; n = 8) or at the indicated time points (for uxt1Δ uxt2Δ; n = 3). Open circles, individual mice; black bar, mean; dashed line, initial inoculum. **, p < 0.01 by one-way ANOVA with Tukey’s post hoc test.
https://doi.org/10.1371/journal.ppat.1006765.s007
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S8 Fig. UXT1 and UXT2 transcription levels.
Expression of UXT1 and UXT2 measured by qRT-PCR with RNA prepared from the indicated strains after growth in nutrient rich (YPD) or capsule-inducing conditions (DMEM, 37°C and 5% CO2). Values are normalized to the WT sample grown in YPD and are the mean ± SEM of six biological replicates.
https://doi.org/10.1371/journal.ppat.1006765.s008
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S9 Fig. Nucleotide sugar uptake into Gmt1- and Gmt2- containing proteoliposomes.
(A) Immunoblot analysis of microsome (M) and proteoliposome (P) preparations from S. cerevisiae expressing vector only (Control) or V5-tagged Gmt1 or Gmt2 (2.5 μg protein per lane; S, molecular weight standards; C, control; 1, Gmt1; 2, Gmt2). (B and C) Representative LC-MS/MS spectra of GMP-preloaded proteoliposomes (B, Control; C, Gmt1) incubated for 10 min at 37°C with a mixture of 16 nucleotide / nucleotide sugar substrates, each 50 μM. Peak 1, GDP-Man; Peak 2, GDP-Glc; Peak 3, GDP-fucose (D and E) Quantification of nucleotide sugar uptake into proteoliposomes preloaded with (D) 30 mM GMP or (E) 30 mM UMP. Data were normalized to the total protein content of the proteoliposome preparations and show the mean ± SD of four assays. These results are consistent with prior studies [21,30] and yield new information about Gmt substrate specificity.
https://doi.org/10.1371/journal.ppat.1006765.s009
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S1 Table. Methylation analysis of GXM for the indicated strains.
https://doi.org/10.1371/journal.ppat.1006765.s010
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S2 Table. Staining and stress sensitivity of Cryptococcus neoformans strains.
https://doi.org/10.1371/journal.ppat.1006765.s011
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S3 Table. Nucleotide sugar contents of Cryptococcus neoformans strains.
https://doi.org/10.1371/journal.ppat.1006765.s012
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S4 Table. Uxt1 and Uxt2 content of proteoliposomes used for transport assays.
https://doi.org/10.1371/journal.ppat.1006765.s013
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Acknowledgments
We thank the members of the Doering laboratory for insightful discussions and assistance with experiments (Cara Griffith for initial gene identification; Dr. Zeke Maier and Dr. Stacey Gish for transcriptional analysis; Matthew Williams for mouse studies; and Dr. Camaron Hole for macrophage experiments). We also thank Dr. Wandy Beatty (Washington University School of Medicine) for TEM, Dr. Jeff Brodsky (University of Pittsburgh) for αKar2p/BiP antibody, Dr. Benjamin S. Glick (University of Chicago) for the Sec7-3xGFP S. cerevisiae strain, Dr. Joe Heitman (Duke University) for C. neoformans KN99α, Dr. Thomas R. Kozel (University of Nevada School of Medicine) for anti-GXM mAbs, and Dr. Jennifer Lodge (Washington University School of Medicine) for plasmid pMH12-T.
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