Host Iron Withholding Demands Siderophore Utilization for to Survive Macrophage Killing
The fungal pathogen Candida glabrata has risen from an innocuous commensal to a major human pathogen that causes life-threatening infections with an associated mortality rate of up to 50%. The dramatic rise in the number of immunocompromised individuals from HIV infection, tuberculosis, and as a result of immunosuppressive regimens in cancer treatment and transplant interventions have created a new and hitherto unchartered niche for the proliferation of C. glabrata. Iron acquisition is a known microbial virulence determinant and human diseases of iron overload have been found to correlate with increased bacterial burden. Given that more than 2 billion people worldwide suffer from iron deficiency and that iron overload is one of the most common single-gene inherited diseases, it is important to understand whether host iron status may influence C. glabrata infectious disease progression. Here we identify Sit1 as the sole siderophore-iron transporter in C. glabrata and demonstrate that siderophore-mediated iron acquisition is critical for enhancing C. glabrata survival to the microbicidal activities of macrophages. Within the Sit1 transporter, we identify a conserved extracellular SIderophore Transporter Domain (SITD) that is critical for siderophore-mediated ability of C. glabrata to resist macrophage killing. Using macrophage models of human iron overload disease, we demonstrate that C. glabrata senses altered iron levels within the phagosomal compartment. Moreover, Sit1 functions as a determinant for C. glabrata to survive macrophage killing in a manner that is dependent on macrophage iron status. These studies suggest that host iron status is a modifier of infectious disease that modulates the dependence on distinct mechanisms of microbial Fe acquisition.
Published in the journal:
. PLoS Pathog 7(3): e32767. doi:10.1371/journal.ppat.1001322
Category:
Research Article
doi:
https://doi.org/10.1371/journal.ppat.1001322
Summary
The fungal pathogen Candida glabrata has risen from an innocuous commensal to a major human pathogen that causes life-threatening infections with an associated mortality rate of up to 50%. The dramatic rise in the number of immunocompromised individuals from HIV infection, tuberculosis, and as a result of immunosuppressive regimens in cancer treatment and transplant interventions have created a new and hitherto unchartered niche for the proliferation of C. glabrata. Iron acquisition is a known microbial virulence determinant and human diseases of iron overload have been found to correlate with increased bacterial burden. Given that more than 2 billion people worldwide suffer from iron deficiency and that iron overload is one of the most common single-gene inherited diseases, it is important to understand whether host iron status may influence C. glabrata infectious disease progression. Here we identify Sit1 as the sole siderophore-iron transporter in C. glabrata and demonstrate that siderophore-mediated iron acquisition is critical for enhancing C. glabrata survival to the microbicidal activities of macrophages. Within the Sit1 transporter, we identify a conserved extracellular SIderophore Transporter Domain (SITD) that is critical for siderophore-mediated ability of C. glabrata to resist macrophage killing. Using macrophage models of human iron overload disease, we demonstrate that C. glabrata senses altered iron levels within the phagosomal compartment. Moreover, Sit1 functions as a determinant for C. glabrata to survive macrophage killing in a manner that is dependent on macrophage iron status. These studies suggest that host iron status is a modifier of infectious disease that modulates the dependence on distinct mechanisms of microbial Fe acquisition.
Introduction
Candida glabrata has emerged as an opportunistic fungal pathogen that causes life-threatening infectious disease in humans [1]. The dramatic rise in the number of immunocompromised individuals due to HIV infection and tuberculosis, and as a result of immunosuppressive regimens in cancer treatment and transplant interventions, have provided fertile ground for unchecked C. glabrata proliferation. While Candida species now account for over 10% of all bloodstream infections [2], the poor susceptibility of C. glabrata to antifungal therapeutics is in great part responsible for the high mortality rate of up to 50% associated with C. glabrata candidemia [3], [4]. The limited knowledge of virulence factors that contribute to the pathogenesis of C. glabrata demands insights into the biology of this opportunistic pathogen that contribute towards the successful colonization of the mammalian host.
Iron (Fe) is an essential metal for virtually all organisms. The ability of Fe to cycle between the reduced ferrous (Fe2+) and oxidized ferric (Fe3+) forms endows it with redox versatility that is utilized in both catalysis and structural biology. However, Fe2+ also has the potential to generate damaging reactive oxygen species (ROS) via Fenton/Haber Weiss chemistry [5] and, as a consequence, organisms have evolved sophisticated homeostatic mechanisms to tightly regulate the acquisition, utilization, storage and mobilization of Fe [6], [7].
Eukaryotic Fe homeostasis has best been described in the budding yeast, Saccharomyces cerevisiae that possesses two high-affinity mechanisms of Fe acquisition [7]. In an aerobic environment, Fe is oxidized and largely insoluble [8] and one mechanism relies on the reduction of environmental Fe sources by cell surface reductases and transport through a ferroxidase/permease complex composed of the Fet3 and Ftr1 proteins, respectively. The activity of the Fet3 Cu-dependent ferroxidase is essential for Fe transport through Ftr1 and, thus, reductive high-affinity Fe assimilation is dependent on adequate cellular Cu bioavailability. Alternatively, S. cerevisiae expresses cell surface siderophore transporters. Synthesized and secreted by most bacteria and fungi as well as some higher plants, siderophores are low molecular weight organic chelators with high affinity for Fe3+ (binding constants between 1023 M and 1049 M). Given the low Fe bioavailability in an aqueous environment (free Fe3+ concentration below 10−9 M at pH 7) and the further strict active withholding of Fe within mammalian hosts (free serum Fe concentration of approximately 10−24 M) [9], siderophores represent a powerful and widespread mechanism for microbial Fe scavenging. This is underscored by the fact that bacteria and fungi have evolved transporters that allow them to utilize siderophores they themselves do not produce (xenosiderophores) and several fungi, such as Candida species, and bacteria do not possess the ability to synthesize siderophores yet express transporters for xenosiderophores [7]. Although the mechanisms of Fe homeostasis in Candida albicans, similar to most fungi, differ significantly from that of S. cerevisiae and C. glabrata [10], iron-regulated CaSit1 shares high homology with S. cerevisiae siderophore transporters and its deletion compromises utilization of fungal ferrichrome-type hydroxamate siderophores. CaSit1 has been shown to be required for the invasion and penetration of human epithelial cells in an in vitro model of oral candidiasis but was not required for murine systemic candida dissemination [11], possibly reflecting the sterile environment of the serum in which siderophore concentrations are predicted to be negligible. The absence of an identifiable heme receptor in C. glabrata present in Candida albicans [12], suggests that C. glabrata may rely predominantly on the solubilization of the circulating exchangeable Fe pool to meet its requirements for Fe. Given that mammals are host to a formidable number of microbial species, the aggressive exploitation of local siderophore reservoirs that allows for high-affinity Fe uptake from virtually any host ligand is likely to play a critical role in microbial virulence.
Mammalian cellular immunity relies heavily on the action of macrophages, cells that also play a critical role in systemic Fe homeostasis [13]. A key mechanism through which macrophages mediate microbial containment is through the localized reduction of serum transferrin-bound Fe, decreased Fe export and the depletion of Fe from the macrophage phagosome, an intracellular compartment that surrounds ingested microorganims. These macrophage activities promote the killing of microorganisms by depriving them of Fe essential not only for cellular biochemistry but also for incorporation into microbial ROS-detoxifying enzymes, such as catalase or superoxide dismutase, that are critical to resistance to high levels of oxidative stress generated in the phagosome [14]. Emerging evidence for increased infections in patients with Fe overload disease highlights the strict requirement for tight host Fe restriction in microbial containment [15]. Hereditary hemochromatosis (HH) is the most common single-gene disorder affecting Caucasian individuals of European descent [16]. Mutations associated with HH are found in the gene encoding the Fe exporter, ferroportin (Fpn), in HAMP, encoding the peptide hormone hepcidin and negative regulator of Fpn, as well as in genes encoding regulators of HAMP expression. Hepcidin expression and release from the liver leads to targeted Fpn degradation at a systemic level resulting in a block in dietary Fe uptake through enterocytes and a block in Fe release from macrophage and hepatocyte stores [17]. Although several of the mutations that underlie HH lead to similar outcomes of pathophysiological Fe overload in parenchymal organs, the clinical presentations differ with regard to macrophage Fe levels which are low when hepcidin levels are low or fails to be recognized by Fpn, and high when hepcidin levels increase or Fpn Fe-export activity is compromised. Given the critical role of macrophages in immunity, the dominant effects of Fpn activity on macrophage Fe status may be predicted to impinge on their immuno-protective functions.
Here we describe the C. glabrata Sit1 siderophore transporter, its regulation under Fe deficiency and substrate siderophore specificity. In infection assays using both mouse and human macrophage cell lines we observe a strong Sit1-mediated, siderophore-dependent increase in C. glabrata survival that is blunted with increased macrophage Fe levels. Genetic manipulation of macrophage Fe status to parallel that which is observed in human diseases of Fe overload revealed an inverse correlation between macrophage Fe and C. glabrata dependence on siderophore-Fe as indicated by yeast survival rates as well as by SIT1 expression in the macrophage phagosome. Consistent with this, infection of primary macrophages derived from a mouse model of Ferroportin disease in which macrophage Fe levels are chronically elevated demonstrated enhanced C. glabrata survival that is independent of Sit1-mediated siderophore utilization. These observations are consistent with reports of greater microbial burden in patients with Fe overload disease [15], [18], [19], [20], [21] and predict that mutations affecting macrophage Fe levels may not only compromise microbial containment, but may also dictate the dependence of microbes on distinct mechanisms of Fe uptake.
Results
The Candida glabrata genome encodes a single siderophore transporter
Fe acquisition is a critical microbial virulence determinant due to the Fe-restricted nature of the mammalian host. The great majority of body Fe is compartmentalized within red blood cells bound as heme to hemoglobin. Several microorganisms, including C. albicans, can access this rich Fe source by secreting hemolytic factors that results in red blood cell lysis [22]. Heme can then be taken up, often by means of a dedicated receptor (such as Rbt5 and Rbt51 in C. albicans [12]) and the porphyrin ring hydrolysed by intracellular heme oxidases [23]. To test whether red blood cells represent an efficient source of Fe for C. glabrata, we grew the wild type strain as well as that of C. albicans and S. cerevisiae, on sheep blood agar plates containing 5% whole blood. Formation of a hemolytic halo surrounding yeast colonies was evaluated after 48–72 hours growth at 30 °C or 37 °C with 5% CO2. Unlike the robust growth and associated hemolytic activity observed for C. albicans, C. glabrata and S. cerevisiae displayed very weak hemolysis when grown on blood sheep agar (Figure 1A). Furthermore, whereas C. albicans was able to efficiently utilize heme as a source of Fe at sub-micromolar hemin concentrations, C. glabrata required 100-fold higher hemin concentrations to achieve the same level of growth. In the same way, higher hemin concentrations were required for a slower growth of C. glabrata due to hemin toxicity when compared to C. albicans (Figure 1B). The observed differences in growth when heme is the sole Fe source may due to the absence of an identifiable heme receptor in the C. glabrata genome that is present in C. albicans. To address this possibility, C. albicans and C. glabrata were cultured in Fe-deficient medium supplemented or not with 20 µM zinc protoporphyrin (ZPP) for 3 hours. In contrast to heme, which is non-fluorescent due to the quenching of the intrinsic porphyrin fluorescence by Fe, ZPP fluoresces and its cellular uptake can be evaluated by in vivo microscopy. Figure 1C shows that in contrast to C. albicans that showed intense intracellular fluorescence, this was not observed for C. glabrata, the intracellular fluorescence of which did not rise above background as determined by comparison to the signal obtained by growth under Fe deficiency alone. This suggests that C. glabrata is not capable of taking up heme. Thus, given its weak hemolytic activity and inability to efficiently import heme, we predict that C. glabrata relies primarily on circulating host Fe sources to satisfy its requirements for Fe.
Analysis of the Candida glabrata genome [24] predicts the existence of orthologues to the Saccharomyces cerevisiae high affinity reductive Fe assimilation pathway as well as a single open reading frame, CAGL0E04092g, encoding a predicted membrane protein with 14 transmembrane domains and a high degree of identity (72%) to the siderophore-Fe transporter, Arn1, that we have designated SIT1 (Siderophore Iron Transporter 1) (Figure 2A and Figure S1A). Computational topological analyses of Sit1 identified sequence signatures characteristic of members of the Major Facilitator Superfamily of transporters (data not shown). In addition, Sit1 orthologues predicted to exist across the ascomycetes, and to lesser extent basidiomycetes, share high sequence identity within the carboxyl terminus of the protein. Protein BLAST analysis [25] of a 51 amino acid sequence comprising the last extra-cellular loop (from amino acid residue 531 to 581) exclusively returned known siderophore transporters and uncharacterized proteins predicted to encode fungal siderophore transporters (data not shown). This SIderophore Transporter Domain (SITD) is conserved in many pathogenic fungi (Figure 2A).
Sit1 mediates siderophore-Fe utilization under conditions of Fe deficiency
To investigate the effects of Fe availability on SIT1 expression, C. glabrata was grown under conditions of Fe-repletion or Fe-deficiency. Figure 2B shows that steady state SIT1 mRNA levels are elevated under Fe deficiency and that this elevation is sustained throughout the time-course of the experiment over 6 hours. To analyze the levels of Sit1 protein as a function of Fe availability, a Flag epitope was introduced at the carboxyl terminus of SIT1 and the fusion gene, encoding a functional protein, was integrated at the endogenous SIT1 genomic locus (Figure S1B). Similar to what was observed for SIT1 mRNA, Sit1Flag fusion protein expression is low under Fe repletion but robustly accumulates under conditions of Fe deficiency (Figure 2C).
Siderophore production is common among most microorganisms and is a major mechanism of Fe solubilization and acquisition. The very high Fe-binding constants observed for siderophores of fungal origin (approximately 1030 M at pH 7) are several orders of magnitude higher than that of the Fe2+ chelator BPS, which inhibits the Fet3/Ftr1 pathway of Fe2+ uptake. We reasoned that if a siderophore biosynthetic pathway exists in this microorganism, C. glabrata would exhibit growth in the presence of BPS. As shown in Figure 2D, growth of the wild type strain was severely compromised in Fe-deficient medium chelated with 100 µM BPS. This is consistent with a predicted lack of siderophore biosynthetic machinery in C. glabrata based on the absence of identifiable orthologues to the gene encoding ornithine-N5-oxygenase that catalyses the first committed step in fungal siderophore biosynthesis (the DNA and protein sequences of the Aspergillus nidulans ornithine-N5-oxygenase SidA were used to perform the BLAST analyses) [26]. To address the role of the Sit1 transporter in xenosiderophore utilization, a mutant lacking the SIT1 gene, as well as the reconstituted strain in which the wild type SIT1 gene was integrated in the sit1Δ strain at the endogenous genomic locus, were generated and evaluated for growth in Fe-deficient medium alone or in the presence of several structurally distinct fungal and bacterial siderophore substrates. Supplementation of Fe-deficient media with the fungal hydroxamate-type siderophores ferrichrome, ferrirubin or coprogen promoted robust growth of the wild type and SIT1-reconstituted strains (Figure 2D). In contrast, the sit1Δ mutant strain was unable to use siderophore-Fe, strongly supporting the notion that Sit1 is a siderophore transporter capable of utilizing these xenosiderophores. Neither the ester-linked siderophore triacylfusarine C, nor the bacterially-derived siderophores enterobactin, salmochelin, yersiniabactin or desferrioxamine were able to complement the growth of C. glabrata under iron deficiency (Figure S1C) suggesting that these siderophores are either not transported by Sit1 or C. glabrata lacks a mechanism of releasing the Fe from these siderophores intracellularly.
The subcellular localization of Sit1 was evaluated using the Sit1Flag and Sit1mCherry fusion proteins. Previous studies in S. cerevisiae have shown that during Fe deficiency the Arn1 siderophore transporter is not localized to the plasma membrane but rather to intracellular endosomal vesicles [27]. Trafficking of Arn1 to the plasma membrane is a substrate-dependent process that occurs in a dose-dependent manner [28], [29]. In contrast to this, indirect immunofluorescence as well as live microscopy of C. glabata Sit1 revealed strong accumulation of the Sit1 protein at the plasma membrane under Fe deficiency in the absence of siderophore substrate and this accumulation was largely unaltered by the addition of ferrichrome (Figure 2E and Figure S1D).
Siderophore utilization is functional under Cu deficiency
High-affinity elemental Fe uptake requires the activity of the Fet3/Ftr1 ferroxidase/permease complex, with the protein complex assembled in the ER and 4 Cu ions loaded onto Fet3 within the Golgi. Under Cu deficiency, apo-Fet3-Ftr1 is assembled and targeted to the plasma membrane, but the absence of ferroxidase activity abolishes high-affinity Fe2+ transport through Ftr1 [30]. As such, elemental Fe uptake is a copper-dependent mechanism. In contrast, siderophore transporters are not known to require Cu for activity and would be predicted to be functional under low Cu conditions. Figure 2F shows that siderophore utilization is functional under Cu deficiency as imposed by growth in the presence of the Cu chelator BCS suggesting that Fe-siderophore transport is likely to be critical as the sole mechanism of high affinity Fe acquisition under conditions of Cu deficiency.
Sit1-mediated siderophore utilization enhances the survival of C. glabrata to macrophage killing
The ability of C. glabrata to exploit local xenosiderophore reservoirs in the absence of an endogenous siderophore biosynthetic pathway suggests a selective advantage imparted by this mechanism of Fe uptake that may impact on the survival of this fungal pathogen. Fe acquisition is challenging within the mammalian host, in which Fe is tightly bound to proteins and ligands in extracellular and intracellular environments. The further active depletion of Fe from the phagosomal compartment amplifies the microbicidal potency of macrophages as microorganisms defend themselves from ROS under conditions that are expected to compromise ROS-detoxifying enzyme activity. We tested whether Fe deficiency would increase the susceptibility with which C. glabrata resists macrophage killing and if this might be circumvented by exposure of C. glabrata to substrate siderophore. Using the mouse macrophage-like cell line, J774A.1, isogenic wild type, sit1Δ and sit1Δ::SIT1 C. glabrata strains were grown under Fe limiting conditions and briefly incubated in the absence or presence of ferrichrome prior to co-culture with activated macrophages (Figure 3A). C. glabrata cells were recovered by cell lysis and survival was evaluated by quantitating colony forming units (CFU) and comparing percentage yeast survival relative to the wild type strain grown under Fe deficiency (represented by a dashed line). Figure S2A shows that when C. glabrata cells were grown under Fe deficiency prior to macrophage infection, differences were not observed in the survival of the three strains to macrophage killing. However, growth of both the wild type and reconstituted sit1Δ::SIT1 strains in the presence of ferrichrome significantly increased survival when compared to the sit1Δ strain, indicative of enhanced C. glabrata ability to survive macrophage killing as a result of siderophore-Fe utilization (Figure 3B, left columns). This suggests that Sit1-mediated ferrichrome utilization provides a survival advantage to phagocytosed C. glabrata cells that is not observed in the strain that cannot internalize this Fe source. To address whether the decreased survival of the sit1Δ strain could be attributed to altered levels of phagocytosis of the mutant yeast cells rather than decreased Fe satiety, CFU were monitored 2 hours post-infection and no significant differences between the wild type, sit1Δ and sit1Δ::SIT1 strains were observed in the presence or absence of ferrichrome, strongly suggesting equally efficient phagocytosis of the three yeast strains by macrophages (Figure S2A).
To test whether the Sit1-dependent increase in C. glabrata survival in the presence of siderophore was a consequence of macrophage Fe status, macrophages were Fe-loaded prior to infection with the C. glabrata strains and the levels of ferritin, the primary intracellular Fe storage protein, were evaluated by immunoblotting. As shown in Figure S2B, activated macrophages cultured under Fe supplementation (lane 4) showed higher ferritin protein levels than those cultured in normal medium (lane 2). Under these conditions of exogenous Fe loading, differences in survival were not observed between the wild type, sit1Δ and sit1Δ::SIT1 yeast strains grown in the presence or absence of ferrichrome (Figure 3B, right columns). Furthermore, significantly higher CFU were recovered from Fe-loaded macrophages under all conditions tested when compared to infection of macrophages growing in the absence of Fe supplementation, suggesting that elevated Fe compromises the ability of macrophages to contain C. glabrata proliferation within the phagosome. To ascertain whether Fe-loading compromises macrophage activation and the ability to mount an inflammatory response, secreted levels of TNF-alpha, an acute phase inflammatory cytokine secreted by activated macrophages, were assayed and no significant changes were observed between that secreted from activated Fe-loaded macrophages and activated macrophages cultured in standard growth media (Figure S2C).
Despite the fact that the overall mechanisms of innate and adaptive immunity are relatively conserved between mice and humans, there are striking immunological differences between the two species [31]. In particular, there is some controversy over whether human macrophages express functional inducible nitric oxide synthase (iNOS). This enzyme catalyzes the production of NO from L-arginine that, in the oxidative environment of the phagosome, reacts with superoxide leading to the generation of peroxynitrite, a powerful oxidant used by macrophages and neutrophils in microbial killing during the oxidative burst. Given this and other differences in mouse and human macrophage immunobiology, we asked whether Sit1-mediated siderophore utilization enhanced C. glabrata survival to killing by human macrophages. To test this, we used the U937 cell line derived from a hystiocystic lymphoma whose differentiation and activation have been previously described [32], [33]. Upon differentiation into mature macrophages, U937 cells were infected with the wild type, sit1Δ and sit1Δ::SIT1 C. glabrata strains grown under Fe deficiency, with or without a brief exposure to ferrichrome, and yeast CFU quantitated after 18, 24 and 36 hours of co-culture. Figure 3C shows that when exposed to ferrichrome, the wild type and SIT1 reconstituted strains displayed enhanced survival at all time points in contrast to the sit1Δ mutant strain that is unable to transport the siderophore. Pre-loading U937 cells with Fe by culturing in the presence of 20 µM FAC promoted the growth of C. glabrata and abrogated the requirement for Sit1-mediated siderophore utlization in enhanced C. glabrata survival (Figure 3D). These results recapitulate the observations made in the J744A.1 mouse macrophage cell line and suggest that Sit1-mediated siderophore utilization protects C. glabrata against the intracellular microbicidal activities of macrophages. Given the generation of ROS in the phagosome of activated macrophages (Figure S2D), indicative of higher levels of oxidative stress, we hypothesize that siderophore-Fe plays a role in providing the Fe required for DNA replication and cellular proliferation as well as for defence against oxidative stress. Moreover, these results indicate that macrophage Fe-withholding from phagocytosed microorganisms is fundamental for the containment of microbial growth and also impacts on the mechanisms available for microbial iron uptake, imposing a strict dependence of C. glabrata on the availability and utilization of xenosiderophores via Sit1.
Macrophage Fe status dictates the dependence of C. glabrata on Sit1 function
Based on the effect of macrophage Fe loading on C. glabrata Sit1-mediated siderophore-dependent survival, we asked whether mutations that alter macrophage Fe homeostasis might similarly modulate the dependence of C. glabrata on siderophore-Fe acquisition. The sole mammalian Fe exporter Fpn is expressed on the surface of enterocytes, macrophages, hepatocytes and placental cells where it plays a fundamental role in systemic Fe homeostasis. Type IV hemochromatosis, or Ferroportin disease, is an autosomal-dominant condition that arises from missense mutations in Fpn that compromise regulated Fe export activity. Two often contrasting clinical presentations observed in patients result from distinct mutations in Fpn that either abolish the hepcidin binding site or compromise Fe export, leading to differential effects on macrophage Fe levels [16], [34], [35], [36]. We modulated macrophage Fe status by stably expressing a cDNA encoding the FPNC326Y hepcidin-insensitive disease mutation, associated with low macrophage Fe levels, or the FPNH32R allele identified in the flatiron mouse that fails to localize to the plasma membrane, leading to Fe-overload. Using ferritin protein levels as a biomarker of macrophage Fe loading, macrophages expressing the FPNH32R transgene were chronically iron-loaded in the absence of hepcidin when compared to macrophages expressing the wild type gene due to the loss in ability to export cellular Fe (Figure 4A, lanes 1 and 3). Incubation with hepcidin increased ferritin levels in cells expressing wild type FPN, as would be predicted from Fpn internalization and degradation, resulting in increased cellular Fe accumulation (Figure 4A, lane 2). In contrast, hepcidin had only a mild effect on FPNH32R-expressing macrophages (Figure 4A, lane 4). Given that Fpn functions as a dimer [37], this modest increase in ferritin levels may reflect the contribution of hepcidin-sensitive endogenous wild type homodimers that correctly localize to the plasma membrane. In contrast, macrophages expressing the FPNC326Y transgene show lower than wild type ferritin levels when grown under Fe-replete conditions in the presence of hepcidin, consistent with a chronic Fe efflux under conditions that induce Fpn turnover of the wild type protein (Figure 4B, lanes 2 and 4). Indirect immunofluorescence in macrophages expressing the wild type and mutant FPN transgenes was performed to monitor protein localization. Both the wild type and FpnC326Y-expressing cells, but not cells expressing FpnH32R, show plasma membrane ferroportin accumulation in the absence of hepcidin (Figure S3A). Exposure to hepcidin leads to a predominantly intracellular localization of the wild type protein, whereas the hepcidin-insensitive FpnC326Y protein remains at the cell surface.
Using these macrophages with altered Fe homeostasis, we ascertained whether genetically programmed differences in macrophage Fe levels impinge on the dependence of C. glabrata on siderophore-Fe for resistance to macrophage killing activities. Macrophages stably expressing the wild type and mutant forms of FPN were infected with wild type, sit1Δ and the SIT1-reconstituted C. glabrata strains that had been grown under Fe deficiency and exposed or not to ferrichrome. As shown in Figure 4C, wild type and SIT1-reconstituted C. glabrata yeast cells, but not sit1Δ cells, showed enhanced survival to macrophages expressing wild type Fpn only when grown in the presence of ferrichrome prior to infection, as interpreted from the increased number of CFU when compared to the wild type C. glabrata strain grown in the absence of FC (dashed line set at 100). No differences were observed in the survival of the three C. glabrata strains grown in the absence of ferrichrome supplementation (data not shown). This recapitulates the results obtained in non-transfected J774A.1 mouse macrophages and human differentiated U937 cells in the absence of Fe supplementation (Figure 3B, left columns). In contrast, siderophore-dependent differences in C. glabrata survival were not observed between the yeast strains recovered from the chronically Fe-loaded macrophages expressing the FPNH32R transgene, supporting our previous results using exogenously Fe-loaded macrophages (Figure 3B, right columns). This is consistent with the high levels of labile intracellular Fe in FPNH32R macrophages that elevate the abundance of ferritin and might be inefficiently withheld from C. glabrata. In contrast, C. glabrata recovered from FPNC326Y macrophages cultured in the presence of hepcidin exhibit increased dependence on siderophore-Fe utilization for survival when compared to those recovered from macrophages expressing wild type Fpn (Figure 4D). This is consistent with the refractility of FpnC326Y to hepcidin-stimulated degradation and Fe levels in these macrophages that are lower than wild type. To ascertain whether Fe overload or deficiency might compromise the ability of macrophages to mount an inflammatory response, the levels of TNF-alpha were quantified from the culture medium of activated macrophages expressing the FPN, FPNC326Y and FPNH32R transgenes and no difference was found between cell lines (Figure S3B). Taken together, these data suggest that elevated macrophage Fe accumulation increases Fe accessibility to internalized C. glabrata. This ameliorates the strict requirement for Sit1-mediated siderophore utilization observed in macrophages with limited intracellular Fe.
Macrophage Fe status modulates the expression of C. glabrata SIT1
The results presented here suggest that Sit1-dependent siderophore utilization enhances C. glabrata survival to activated macrophages in a manner that is dependent on macrophage labile Fe status. SIT1 characterization demonstrated that expression is responsive to environmental Fe bioavailability, showing low levels of expression under Fe repletion and robust mRNA and protein accumulation under Fe deficiency (Figure 2B and 2C). Using a reporter strain expressing a SIT1mCherry fusion gene from the endogenous SIT1 locus, we ascertained whether internalized C. glabrata cells sense differences in genetically-programmed macrophage Fe status. As shown in Figure 5A by live microscopy, C. glabrata cells phagocytosed by macrophages expressing the FPNC326Y transgene showed enhanced Sit1mCherry accumulation when compared to yeast internalized by macrophages that were Fe-loaded by virtue of FpnH32R expression, suggesting that C. glabrata cells experienced different degrees of Fe deficiency in these macrophages. Fluorescein-conjugated dextran beads were included in the infection medium to allow for a clearer visualization of intra- versus extra-cellular yeast. To quantitatively evaluate the influence of macrophage Fe status on the Fe satiety of C. glabrata, SIT1 transcript levels were monitored in yeast cells recovered from macrophages by semi-quantitative RT-PCR. Figure 5B shows that cells recovered from FPNH32R-expressing macrophages exhibited lower levels of the SIT1 transcript when compared to cells recovered from FPNC326Y-expressing macrophages two and four hours post-infection, consistent with an increased Fe satiety within the phagosome. These results support the hypothesis that chronic perturbations in macrophage Fe levels translate into altered microbial Fe availability that may impact on the mechanisms of microbial Fe uptake.
Ex-vivo infection of mouse primary macrophages supports a critical role for macrophage Fe loading on the dependence of C. glabrata on Sit1-mediated siderophore utilization
Given the effects of macrophage Fe status on the dependence of C. glabrata siderophore utilization using well-established macrophage cell lines, we ascertained whether this could be recapitulated in an ex-vivo infection of primary mouse macrophages. Bone marrow cells were recovered from the femurs of control mice and of the flatiron (ffe) mouse model of human Ferroportin Disease, which harbors the FPNH32R mutation [36]. Cells were differentiated into mature macrophages in culture and endogenous Fpn expression stimulated by incubating cells in 10 µM ferric ammonium citrate for 2 days prior to activation and infection with C. glabrata (Figure 6A). Consistent with the results obtained using the J774A.1 and U937 cell lines, when grown in the presence of ferrichrome, C. glabrata wild type and SIT1-reconstituted cells showed enhanced survival to the killing activities of wild type primary macrophages when compared to the sit1Δ strain (Figure 6B). However, siderophore-dependent survival was significantly diminished in infected ffe macrophages, supporting our previous observations that increased macrophage labile Fe pools promote the growth of C. glabrata independently of siderophore utilization.
Integrity of the Sit1 SITD is critical for ferrichrome utilization
Computational analysis of the Sit1 SITD (Figure 2A) revealed a high degree of conservation among orthologous siderophore transporters in a large number of fungal species, including several animal and plant pathogens, a representative number of which are shown in Figure S4. To begin to evaluate a potential role for the SITD in Sit1-mediated siderophore utilization in C. glabrata, the predicted extracellular topological orientation of the carboxyl-terminal loop between transmembrane domains 13 and 14 was first evaluated experimentally. Sit1 was tagged with a 2XFLAG epitope within the carboxyl-terminal loop between residues G542 and D543 (Figure S5A). Cells expressing this tagged Sit1 protein, or the empty vector, were cultured under Fe deficient conditions and the accessibility of the anti-Flag antibody for its cognate epitope evaluated in non-permeabilized cells by indirect immunofluorescence. As shown in Figure S5B, plasma membrane accumulation of the Flag antibody was observed in non-permeabilized cells expressing carboxyl-loop-Flag Sit1. This immunofluorescence signal was absent in cells expressing vector alone and is consistent with an orientation of this loop region, and therefore the SITD, toward the extracellular face of the plasma membrane.
To test whether the Sit1 SITD may be of functional importance, we mutated the conserved residue, Y575 to alanine (Figure S4), and tested whether this might compromise Sit1-mediated ferrichrome utilization. A strain carrying the SIT1Y575A allele integrated at the endogenous genomic locus (Figure S5C) was strongly impaired in its ability to use ferrichrome as an Fe source (Figure 7A) despite exhibiting levels of protein expression (Figure S5D) and plasma membrane localization (Figure 7B and Figure S5E) comparable to the wild type strain. The observed decrease in the ability of the Sit1Y575A mutant to utilize ferrichrome prompted us to evaluate the ability of this strain to survive macrophage killing when grown in the presence of this siderophore. In contrast to wild type C. glabrata cells, neither the sit1Δ nor the strain bearing the Sit1Y575A substitution in Sit1 showed the Sit1-mediated siderophore-dependent increase in the ability to survive macrophage killing, suggesting that although this mutation does not lead to a complete loss of Sit1 function (see Figure 7A), the remaining activity is insufficient to meet the cellular demand for Fe within the phagosome (Figure 7C).
Discussion
Candida glabrata has risen from relative obscurity as a relevant opportunistic human fungal pathogen to an increasing cause of serious infectious disease particularly in immunocompromised individuals. Yet, the significant phylogenetic relatedness of C. glabrata to Saccharomyces cerevisiae argues for some fundamental differences in the biology of this microorganism, either through the functions of the as yet poorly studied 400 genes unique to Candida glabrata and/or through the enhancement or acquisition of novel functions of shared genes. Our results underscore a role for siderophore utilization in the successful existence of C. glabrata as a human commensal as well as during pathogenesis, primarily with respect to survival to phagocytosis by mammalian macrophages. Furthermore, our studies support a pivotal contribution for unregulated host Fe acquisition in the outcome of fungal infection.
The severe Fe restriction imposed by mammalian hosts as an antimicrobial strategy dictates that Fe acquisition is a bona fide virulence determinant. The existence of clinical correlations between elevated Fe bioavailability and increased microbial burden extend beyond diseases of Fe overload for which the higher susceptibility to bacterial infection, notably to Vibrio vulnificus, has been described [15], [18]. In the same way, transfusion-dependent thalassemia patients present with increased susceptibility to widespread microbial infection that correlates with the degree of Fe overload [19]. Treatment of HH and thalassemia patients is further complicated by the fact that the sole FDA-approved Fe chelator desferrioxamine, a naturally occurring bacterial siderophore, effectively further solubilises Fe in a form that is readily utilized by a diversity of bacterial and fungal species, thus elevating the potential for infectious disease in these patients. Individuals with malignant hematological disorders, such as acute myeloid leukemia, who typically present with very high serum Fe, serum ferritin and transferrin saturation, are known to sustain increased mycoses, especially by Candida and Aspergilli [38], [39]. Furthermore, clinical evidence also indicates that Fe overload is an independent risk factor for post-transplant infection [20], [21] and correlates with poor prognosis and in patients infected with HIV, a virus known to depend on and manipulate target cellular Fe accumulation [40]. What then are the implications of Fe overload diseases to the susceptibility to fungal infections? Previous studies support the notion that optimal immunity operates within a range of physiological Fe concentrations [41]. This is ensured in part through Fpn activity, mobilizing dietary and systemic Fe, and the regulatory action of hepcidin. Hereditary Hemochromatosis presents with different genetic etiologies that impart distinct effects on macrophage Fe levels. Using mutations associated with Ferroportin Disease, an autosomal dominant disease in humans, we provide evidence that C. glabrata dependence on the siderophore-Fe uptake machinery is inversely correlated to labile macrophage Fe levels and that Fe overloaded macrophages are markedly less efficient at killing and containing C. glabrata. We infer that this results from the inability of Fe-laden macrophages to withhold this essential metal from internalized C. glabrata cells given the decreased dependence of C. glabrata on siderophore-Fe, decreased SIT1 expression indicative of increased Fe satiety, increased C. glabrata fitness and the increased levels of host cell ferritin expression. Previous studies have shown that activated macrophages accumulate Cu within the phagosome [42] suggesting perhaps that inefficiently withheld macrophage Fe can be mobilized through reductive Fe uptake and supporting a host-dependent modulation of high-affinity mechanisms of Fe assimilation. This notion of a host modulatory action over the mechanisms utilized for microbial Fe acquisition is further evidenced in a study by Lesuisse [43] that compared the effects of exposure of C. albicans to either fetal bovine serum or synthetic Fe-deficient medium supplemented with distinct Fe sources. The results obtained showed that reductive Fe uptake from ferric citrate was downregulated in the presence of serum, as evidenced by decreased Fe uptake and reduced ferrireductase activity, whereas that from ferrichrome-type siderophores was elevated.
In contrast to Fe-loaded macrophages, the low macrophage Fe levels associated with FpnC326Y expression impose Fe deficiency on phagocytosed C. glabrata cells, as demonstrated by elevated SIT1 expression and further supported by the increased dependence on ferrichrome and Sit1 for proliferation. As a result of chronic Fe-deficiency, hepcidin-insensitive macrophages are expected to represent a formidable challenge for microbial proliferation. The FPNC326Y disease-associated mutation results in a similar clinical outcome to that observed in patients carrying HFE mutations present in approximately 80% of HH patients and exhibiting an allelic frequency of over 10% in Caucasians of European descent [13]. Given the high prevalence of HFE mutations, it has been postulated that this mutation was positively selected for conferring protection during outbreaks of infections caused by intracellular pathogens such as Chlamydia and Yersinia [44], [45] highlighting the intimate association between host Fe status and infectious disease.
Whilst siderophore utilization is also undoubtedly critical to microbial colonization of healthy immunocompetent individuals in its state of commensalism, our study prompts an as yet unresolved question in the field regarding the origin of xenosiderophore substrates that are utilized by non-siderophore producers such as Candida and Cryptococcus species. A recent study by Ghannoum et al. characterizing the mycobiome of the oral cavity of healthy individuals identified in this host milieu a complex and dynamic profile of fungal species, the number of which parallels that observed for bacteria [46]. Among the fungi found to colonize the oral cavity of humans are several siderophore-producers that include Aspergillus and Fusarium species known to copiously produce siderophores that include coprogens and ferrichromes, both substrates for Sit1-facilitated utilization in C. glabrata. In particular, Aspergillus fumigatus, one of the most prevalent air-borne human pathogens, synthesizes chemically distinct siderophores for the solubilization of extracellular Fe as well as for its safe intracellular storage [47]. In fact, siderophore utilization by this saprophytic fungus has been shown to be required for virulence, in contrast to reductive Fe assimilation [48], and the conidia of a siderophore-deficient mutant exhibit decreased levels of stored Fe and higher sensitivity to oxidative stress [47]. Given the ubiquitous nature of siderophore production and the mixed nature of the mammalian microbiome localized siderophore reservoirs are likely available to C. glabrata and other non-siderophore producers. In particular, it is tempting to speculate that the higher microbial burden associated with immunocompromised patients generates higher concentrations of microbial siderophores that might tip the balance towards the transition from commensalism to pathological C. glabrata proliferation and subsequent infectious disease.
Given the inability of C. glabrata to efficiently use heme, Sit1-dependent siderophore utilization represents a likely mechanism for high-affinity Fe uptake under conditions of Cu insufficiency, conditions under which elemental high affinity Fe uptake is compromised. This suggests that siderophore utilization might contribute toward the virulence of C. glabrata in both the Fe- and Cu-restricted mammalian host [49]. Sit1 is syntenic to its orthologous gene in S. cerevisiae, Arn1, with which it shares high sequence identity that translates into similar siderophore substrate specificity, which includes ferrichromes and coprogen. Yet, Sit1 and Arn1 differ in their subcellular localization. The routing of trans-Golgi Arn1 away from the plasma membrane and to the vacuolar protein-sorting pathway requires the monomeric clathrin adaptor, Gga2 [50]. Given the existence of a putative orthologue for Gga2 in C. glabrata, it is unclear whether differences in transporter localization reflect distinct protein-protein interactions or another mechanism of siderophore transport altogether - pore versus receptor, for instance. Interestingly, C. albicans Sit1 as well as S. cerevisiae Enb1 [7], also localize predominantly to the plasma membrane in either the absence or presence of substrate siderophore [51]. It is tempting to speculate that under the pressure of harsh competition for Fe and local xenosiderophore reservoirs, C. glabrata and C. albicans have evolved to become more competitive for siderophore binding by expressing the transporter constitutively at the cell surface. Further studies are required to elucidate the mechanism of siderophore recognition and uptake by Sit1 as well as its intracellular fate, an aspect of siderophore utilization that is currently poorly understood in fungi.
Materials and Methods
Yeast strains and growth conditions
C. glabrata strains, BG2 and BG14 (ura3::KAN), were a gift from Dr. Brendan Cormack at the Johns Hopkins School of Medicine, Maryland. Growth under Fe-replete conditions was achieved by supplementing media with 5 µM ferrous ammonium sulfate. Fe-deficient media contained 100 µM bathophenantroline disulphonate (BPS). For spot assays, cells were grown in synthetic complete medium (SC) to mid-logarithmic phase and serial dilutions were spotted on SC or SC supplemented with 100 µM BPS or 150 µM bathocuproine sulfonate (BCS) with or without the indicated siderophores. Ferrichrome, desferrioxamine, hemin and zinc protophorphyrin were purchased from Sigma Aldrich, St. Louis, MO; ferrirubin, coprogen, enterobactin, salmochelin, triacylfusarine C and yersiniabactin were purchased from EMC Microcollections, Tuebingen, Germany. Alexa Fluor-conjugated dextran was purchased from Invitrogen, Carlsbad, CA. For macrophage infection experiments, yeast cells cultured in low Fe medium for 5 hours were exposed or not to ferrichrome [10 µM] 30–35 minutes and the yeast cultures were washed three times with PBS prior to infection. The BG14 strain was used to generate the sit1Δ strain by the PRODIGE PCR-based approach [52]. The SIT1FLAG knock-in cassette was created by overlap PCR of the SIT1 ORF and 964 bp upstream promoter was used to generate the in-frame SIT1FLAG-fusion DNA subcloned upstream of the nourseothricin resistance (NATR) cassette with a further 400 bp of the SIT1 3'UTR cloned downstream of NATR. The sit1Δ::SIT1mCherry strain was generated by targeted integration of a SIT1mCherryNATR cassette cloned into pBM46. Generation of SIT1 tagged with two FLAG epitopes between residues G542 and D543 within the carboxyl-terminal loop was generated by overlap PCR. The Sit1Y575A mutation was generated by site-directed mutagenesis (QuikChange Site-Directed Mutagenesis Kit, Stratagene, La Jolla, CA) and either integrated at the endogenous genomic locus or expressed episomally. For C. glabrata transformation, overnight cultures were transformed with 5 µg DNA using the Frozen-EZ Yeast Transformation II Kit (Zymo Research, Orange, CA) according to the manufacturers instructions. Transformants were selected by growth on YPD media containing 200 µg/ml nourseothricin (Werner BioAgents, Jena, Germany) at 30 °C for 2–4 days.
RNA and protein analyses
Cells were cultured in SC containing ferrous ammonium sulfate [5 µM] in the absence or presence of BPS [80 µM] and samples harvested at the indicated time points and processed for RNA and protein extraction. Total RNA was extracted using the hot acid phenol method [53]. PCR-amplified probes were gel-purified and radiolabeled with alpha-P32-dCTP (GE Healthcare, Piscataway, NJ) using Random Primed DNA Labeling Kit (Roche Applied Science, Indianapolis, IN). Semi-quantitative PCR was performed on cDNA generated by reverse transcription of isolated total RNA (Superscript III first strand; Invitrogen, Carlsbad, CA) using primers specific for SIT1 and ACT1. SIT1 expression levels were normalized against those of ACT1. Total protein was extracted in ice-cold lysis buffer (Tris 25 mM, pH7.5, NaCl 150 mM, 1 mM EDTA) supplemented with protease inhibitors (Roche complete tablet; Roche Applied Science, Indianapolis, IN) using the Triton X-100/glass bead method and total protein quantified using BCA reagent (Pierce, Rockford, IL). Sit1Flag was detected using an HRP-conjugated α-Flag antibody (Sigma Aldrich, St. Louis, MO). An alpha-Pgk1 antibody was used as loading control.
Fluorescence and indirect immunofluorescence microscopy
The sit1Δ::SIT1mCherry cells were visualized with a Zeiss Axio Image widefield fluorescence microscope. In vivo visualization of macrophages infected with C. glabrata strain sit1Δ::SIT1mCherry was performed using a Zeiss Axio Observer Z1 fluorescence microscope. Indirect immunofluorescence of Fpn was observed and captured using a motorized Zeiss Axio Observer Z1. Cells were fixed in methanol at −20 °C for 5 minutes, incubated with Fpn antibody (a gift from Drs. Jerry Kaplan and Ivana de Domenico, University of Utah) and incubated with a secondary fluorochrome-conjugated antibody (Alexa-fluor 488; Molecular Probes, Invitrogen, Carlsbad, CA).
ROS measurement
J774A.1 macrophages seeded at 2×105 cells/ml were activated with 1 µg/ml LPS and 5 ng/ml LPS for 3 hours and 2 µM 2′,7 dichlorofluorescein diacetate (DCFH-DA) added during the last 15 minutes. Fluorescence was monitored 450 nm excitation and 530 nm emission using a fluorescence plate reader (Perkin-Elmer 1420 Victor 3).
Mammalian cell infection assay
The mouse macrophage cell line J774A.1 was maintained in Dulbecco's Modified Eagles Medium 4.5 g/L D-glucose (Gibco, Invitrogen, Carlsbad, CA), 10% FBS, 100U penicillin and 100 mg/ml streptomycin, at 37 °C and 5% CO2. For iron loading experiments, J774A.1 macrophages were cultured in 20 µM ferric ammonium citrate for 2 days and washed 3 times with warm DMEM prior to infection with C. glabrata. Macrophages seeded at 2×105 cells/ml overnight were activated with IFN-gamma [5 ng/ml] (Sigma Aldrich, St. Louis, MO) and LPS [1 µg/ml] (Sigma Aldrich, St. Louis, MO) 3 hours prior to infection with C. glabrata strains at a multiplicity of infection of 1:4 (macrophage:yeast). At the indicated time points infected macrophages were lysed with water, and dilutions of the lysates plated on YPD. Colony forming units (CFU) were counted after growth at 30 °C for 2 days. U937 cells were maintained in RPMI-1640 medium (Gibco, Invitrogen, Carlsbad, CA), supplemented with 2 mM glutamine, 10% FBS, 100U penicillin and 100 mg/ml streptomycin, at 37 °C and 5% CO2. Differentiation of these pro-monocytic cells into mature macrophages was induced by the addition of 10 nM phorbol myristate acetate (PMA) to 1×106 cells/ml for 48 hours. Cells were washed 3 times with warm culture medium and incubated for a further 48 hours at 37 °C and 5% CO2. LPS (1 µg/ml) was added to the macrophages 3 hours prior to infection with C. glabrata (MOI of 1:1) and yeast cell recovery and CFU counting performed as described above. For primary macrophage infection assays, mouse femurs were kindly supplied to us by Drs. Jerry Kaplan and Ivana De Domenico, at the University of Utah. Primary bone marrow cells were harvested by flushing the femurs of 3–5 month-old female control (C3H) or flatiron (ffe) mice and macrophage differentiation induced by culturing in RPMI 1640 containing 20% FBS, 20 µM ß-mercaptoethanol, 2 mM L-glutamine, 100U penicillin and 100 mg/ml streptomycin and GM-CSF [3 ng/ml]. Macrophages were seeded for infection assays at 2×105 cells/ml.
For the generation of stable cell lines expressing wild type and mutant forms of FPN, full-length mouse FPN cDNA (TrueORF, OriGene, Rockville, MD) was used as a template to introduce the H32R and C326Y mutations through site-directed mutagenesis. FPN, FPNH32R and FPNC326Y plasmid DNA were stably transfected into J774A.1 macrophages using Lipofectamine reagent (Invitrogen, Carlsbad, CA). Total protein was extracted in lysis buffer as described above supplemented with 0.1% SDS and a phosphatase inhibitor cocktail (HALT, Pierce, Rockford, IL). Antibodies against ferritin and α-tubulin were purchased from Abcam (Cambridge, MA). IL-6 and TNF-alpha secretion was measured by enzyme-linked immunosorbent assay (ELISA) (R&D Systems, Minneapolis, MN). Fluorescence was measured using a SpectraMax Plus luminometer (Molecular Devices, Sunnyvale, CA).
Accession numbers
The SIT1 DNA, protein sequence and functional description were deposited in GenBank with the Accession Number HQ734814.
Supporting Information
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