Macrophage Internalization of Fungal {beta}-Glucans Is Not Necessary for Initiation of Related Inflammatory Responses

Cell wall ß-glucans are highly conserved structuralcomponents of fungi that potently trigger inflammatory responsesin an infected host. Identification of molecular mechanismsresponsible for internalization and signaling of fungal ß-glucansshould enhance our understanding of innate immune responsesto fungi. In this study, we demonstrated that internalizationof fungal ß-glucan particles requires actin polymerizationbut not participation of components of caveolar uptake mechanisms.Using fluorescence microscopy, we observed that uptake of 5-([4,6-dichlorotriazin-2-yl]amino)-fluorescein hydrochloride-Celite complex-labeled Saccharomycescerevisiae ß-glucan by RAW macrophages was substantiallyreduced in the presence of cytochalasin D, which antagonizesactin-mediated internalization pathways, but not by treatmentwith nystatin, which blocks caveolar uptake. Interestingly,ß-glucan-induced NF- ${kappa}$ B translocation, which is necessaryfor inflammatory activation, and tumor necrosis factor alphaproduction were both normal in the presence of cytochalasinD, despite defective internalization of ß-glucan particlesfollowing actin disruption. Dectin-1, a major ß-glucanreceptor on macrophages, colocalized to phagocytic cups on macrophagesand exhibited tyrosine phosphorylation after challenge withß-glucan particles. Dectin-1 localization and othermembrane markers were not affected by treatment with cytochalasinD. Furthermore, dectin-1 receptors rather than Toll-like receptor2 receptors were shown to be necessary for both efficient internalizationof ß-glucan particles and cytokine release in responseto the fungal cell wall component.

INTRODUCTION

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Introduction

Most pathogenic fungi possess a ß-glucan-rich cellwall comprised of glucose residues arranged in ß-(1,3)-D-glucopyranosylpolymers with associated ß-(1,6)-D-glucopyranosylside chains having various length and frequency distributions(5, 13, 20). Fungal ß-glucans possess many of thecharacteristics attributed to pathogen-associated molecularpattern molecules (PAMPs). ß-Glucans are highly conservedstructural components of the fungal cell wall that potentlytrigger innate immune responses. Previous studies have demonstratedthat ß-glucans stimulate the release of inflammatorymediators, including tumor necrosis factor alpha (TNF- ${alpha}$ ), interleukin-1,MIP-2, eicosanoids, and reactive oxidants (9, 24, 25). Moreover,we have previously demonstrated that ß-glucans fromthe opportunistic pathogen Pneumocystis carinii, as well asSaccharomyces cerevisiae, act as potent inducers of macrophageactivation through NF- ${kappa}$ B translocation utilizing cellular receptorsand signaling pathways distinct from those that mediate cellularactivation in response to lipopolysaccharide (LPS) (14).

Macrophages are professional phagocytes that are one of thefirst lines of defense provided by the innate immune system.Recognition and internalization of particles are complex processesinvolving unique mechanisms and subsequent responses dictatedby the nature of the ingested particle (1). Macrophages usea variety of mechanisms for internalization, including pinocytosis,receptor-mediated endocytosis, caveola-mediated uptake mechanisms,and phagocytosis. The first two pathways are usually independentof actin polymerization; instead, they utilize clathrin-basedmechanisms and are generally involved in uptake of small molecularligands. Caveolar uptake mechanisms have been implicated inthe internalization of viruses and some bacteria (10, 11, 15).In contrast, phagocytosis, the uptake of particulate material,occurs through actin-dependent mechanisms. However, the internalizationof particles is a heterogeneous event which involves moleculesthat are not exclusive for one particular mechanism but mayparticipate in other processes within the cell.

Fungal cell wall ß-glucans have been shown to interactwith several receptors on the surface of macrophages (2, 19,22). Recently, dectin-1 has been the focus of intense investigation.Dectin-1, a small type II receptor expressed on the cell surfaceof innate immune cells, including macrophages and dendriticcells, has been shown to mediate the response of macrophagesto intact yeast and zymosan (2). However, the exact mechanismsof receptor binding and internalization of purified ß-glucanparticles, as well as downstream signaling pathways leadingto macrophage activation and proinflammatory signaling, havenot been fully studied yet.

Although considerable efforts have been directed toward understandingthe interactions between innate immune cells, such as macrophages,and bacterial PAMPs, relatively little is known about the activityof PAMPs present on fungi. Identification of the molecular mechanismsand the components responsible for internalization of ß-glucansand their impact on inflammatory signaling should lead to abetter understanding of innate immune responses to fungi. Accordingly,the present investigations were performed to define molecularmechanisms and components mediating ß-glucan internalizationand signaling by macrophages. We also investigated the roleof dectin-1 and Toll-like receptor 2 (TLR2) receptors in internalizationand signaling responses to purified fungal ß-glucans.

MATERIALS AND METHODS

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Materials and Methods

General reagents. Endotoxin-free buffers and reagents were scrupulously used inall experiments. Fungal ß-glucan particles (derivedfrom S. cerevisiae) were purchased from Sigma Chemical Co. (St.Louis, MO). The sizes of these particles predominantly rangedfrom 2 to 8 µm. LPS from Escherichia coli 026:B6, as wellas a 5-([4,6-dichlorotriazin-2-yl] amino)-fluorescein hydrochloride-Celitecomplex (DTAF), nystatin, cytochalasin D, and other generalreagents were also obtained from Sigma, unless indicated otherwise.Murine RAW 264.7 macrophages were purchased from ATCC and routinelycultured in Dulbecco modified Eagle medium containing 10% fetalbovine serum, 2 mM L-glutamine, penicillin (10,000 U/liter),and streptomycin (1 mg/liter). Cells were routinely passagedfor no more than 6 weeks, discarded, and replaced with frozenstocks. Monoclonal antibody m2A11, which recognizes the dectin-1receptor, was generously provided by Gordon Brown, Universityof Cape Town, South Africa (4). Also, a V5 epitope-tagged wild-typedectin-1 vector was provided by David Underhill, Institute forSystems Biology, Seattle, WA (6). Soluble glucan phosphate,which antagonizes binding of glucan particles to dectin-1 receptors,was a gift from David L. Williams, East Tennessee State University,Johnson City (16). TLR2^–/– mice were donated byShizuo Achira, Research Institute for Microbial Disease, OsakaUniversity, Osaka, Japan (21).

Generation of fluorescent ß-glucan particles. To visualize the internalization of ß-glucan by macrophages,S. cerevisiae ß-glucan particles were coupled to thefluorophore DTAF. This was accomplished by adding 10 mg of DTAFdissolved in 0.1 M borate buffer (pH 7.0) to 25 mg of ß-glucanparticles suspended in 0.1 M borate buffer. The mixture wasallowed to react overnight at room temperature with gentle stirring.Uncoupled DTAF was removed by extensive washing with phosphate-bufferedsaline (PBS). Labeled S. cerevisiae ß-glucan particleswere collected by centrifugation, dried, and weighed. Aftertreatment with polymyxin, the final preparation was assayedfor endotoxin. Labeled particles yielded fluorescence in thegreen range.

We scrupulously excluded endotoxin as the source of cellularresponses to our ß-glucan preparations. To do this,the ß-glucan preparations were tested after each ofthe final washes for soluble endotoxin using a standard amebocytelysate assay with a low level of sensitivity, 0.125 IU (internationalunit)/ml (quantitative chromogenic Limulus amoebocyte lysate;BioWhittaker, Walkersville, MD). In addition, since ß-glucanscan trigger the Limulus amoebocyte lysate reaction, the preparationswere also assayed with the Pyrosate assay (Associates of CapeCod Incorporated, East Falmouth, MA), which is specific forbacterial endotoxin and which has a lower limit of sensitivity,0.25 EU/ml. Only preparations with endotoxin levels below thesethresholds were employed. Furthermore, we previously determinedthat endotoxin-resistant lung cells, which lack TLR4 signaling,can still respond to our particulate ß-glucan preparations,indicating that ß-glucan responses are independentof LPS (14). Thus, we are very confident that the responsesobserved reflected responses to ß-glucan rather thanresponses to any contaminating endotoxin.

Phagocytosis assays and inhibitor treatments. To evaluate the mechanisms of macrophage internalization ofß-glucan particles, we performed phagocytosis assaysin the absence and presence of inhibitors of various uptakepathways. Our previous studies revealed parallel responses offungal ß-glucans interacting with native alveolarmacrophages and with the RAW murine macrophage cell line (14).RAW 264.7 macrophage cells, thus, provide an efficient modelsystem to study interactions of fungal cell wall componentswith macrophages. In addition, in our experience RAW cells exhibitsomewhat less autofluorescence than native macrophages, makingthem useful for fluorescence microscopy studies. Furthermore,the RAW cell line exhibits substantially better transfectionefficiency than native alveolar macrophages. For these reasons,we used these cells for most experiments in this study. RAWmacrophages were pretreated with cytochalasin D (2 µM)or nystatin (5 µg/ml) for 30 min and throughout subsequentincubation with DTAF-labeled ß-glucan. After varioustimes, particle uptake was terminated by washing cells withice-cold PBS, and unbound particles were removed by acid stripping(Hanks balanced saline solution buffered to pH 3.5), followedby fixation with 2% paraformaldehyde. Macrophage uptake of DTAF-glucanwas visualized by fluorescence microscopy. XTT {2,3-bis(2-methoxy-4-nitro-5-sulfophenyl)-5-[(phenylamino)carbonyl]-2H-tetrazoliumhydroxide} assays revealed no adverse effect of these uptakeinhibitors on RAW cell viability at the concentrations employed(7).

To evaluate the potential role of the dectin-1 receptor in mediatinginternalization and signaling from purified ß-glucanparticles, we treated cells with either monoclonal antibodym2A11 or glucan phosphate (3). RAW macrophages were placed onice and incubated with either 100 µg/ml of m2A11 or glucanphosphate for 45 min. After incubation, cells were allowed tobind DTAF-labeled ß-glucan particles for 10 min onice and then incubated at 37°C for 30 min. The RAW macrophageswere gently washed and incubated at 37°C for the times indicatedbelow. Particle uptake was determined as described above. Todetermine the role of TLR2 in mediating uptake of DTAF-labeledß-glucan, alveolar macrophages were collected fromTLR2^–/– mice (21) and strain-matched wild-type controlsby whole lung bronchoalveolar lavage (C57BL/6), and phagocytosisexperiments were performed as previously described (25). Weobtained $~$ 200,000 alveolar macrophages per mouse. In preliminarystudies, mouse native alveolar macrophages exhibited responsesparallel to those of rat macrophages in our previous studies(24, 25).

Immunofluorescence studies for markers of endocytosis and NF- ${kappa}$ B activation. RAW macrophages were cultured on glass coverslips and stimulatedwith ß-glucan particles. After stimulation and fixation,the macrophages were permeabilized with blocking buffer containing0.05% saponin and 2 mg/ml bovine serum albumin for 30 min. Primaryantibodies recognizing either the transferrin receptor (1 µg/ml;eBioscience, Inc., San Diego, CA), an early endocytic marker,or lysosomal membrane protein 1 (Lamp-1; 1 µg/ml; ResearchDiagnostics, Inc., Flanders, NJ) were diluted in blocking solutioncontaining 0.05% saponin for 30 min, rinsed three times withthe same solution, and incubated with a 1:100 dilution of TexasRed secondary conjugated antibodies for 30 min at room temperature.For actin filament visualization, cells were fixed as describedabove, permeabilized in 0.1% Triton X-100 in PBS, and stainedwith Texas Red-phalloidin (1:100; Molecular Probes, Eugene,OR) for 30 min. In additional experiments, the cells were subsequentlystained for nuclear translocation of the p65 NF- ${kappa}$ B componentas previously described (14). Nuclear counterstaining was performedwith 4',6-diamidino-2-phenylindole (DAPI) (0.1 mg/ml; Sigma).Following extensive washing, the coverslips were mounted onglass slides and analyzed by fluorescence microscopy.

Conventional fluorescence microscopy was performed using anIX70 Olympus microscope equipped with filter packs. Fluoresceinisothiocyanate and Texas Red labeling was observed under thefluorescence microscope using optics appropriate for these fluorophores(excitation at 470/40 nm and emission at 540/40 nm for fluoresceinisothiocyanate and excitation at 540/25 nm and emission at 620/60nm for Texas Red). Nuclear counterstaining with DAPI was observedat an excitation wavelength of 360/40 nm and an emission wavelengthof 460/50 nm. In any given experiment, all photomicrographswere exposed and printed in the same way. Quantitative imageanalysis was performed using the "Metamorph" image-processingsoftware (Universal Imaging Corp.) as previously described (17,18).

Macrophage release of TNF- ${alpha}$ following stimulation with fungal ß-glucan particles. To evaluate subsequent macrophage inflammatory activation byß-glucans, we measured TNF- ${alpha}$ release in the absenceor presence of the various uptake inhibitors. RAW macrophageswere grown in 96-well plates overnight at a concentration of2 x 10⁵ cells/well. Cells were pretreated for 30 min with uptakeinhibitors before stimulation with ß-glucan particles(100 µg/ml). After a subsequent 8 h of incubation, themedium supernatants were collected and clarified by centrifugation.Samples were analyzed using a mouse TNF- ${alpha}$ enzyme-linked immunosorbentassay (eBioscience, San Diego, CA) according to the manufacturer'sinstructions.

Dectin-1 phosphorylation following ß-glucan challenge. RAW macrophages (5 x 10⁶ cells) were transfected with 3 µgof a V5 epitope-tagged wild-type dectin-1 plasmid using Nucleofectorcell line solution V (Amaxa Biosystems, Gaithersburg, MD) accordingto the manufacturer's instructions. All experiments were performed24 h after transfection. RAW cells expressing V5 epitope-taggedwild-type dectin-1 were treated for 30 min with 50 µMMG132 to prevent proteosomal degradation of receptors priorto the addition of ß-glucan particles (100 µg/ml)suspended in a solution containing 1 mM sodium ortho-vanadatefor 15 min. Cells were then disrupted with lysis buffer (1%Triton X-100, 10 mM Tris, 50 mM NaCl, 0.2 mM sodium ortho-vanadate,pH 7.4, and protease inhibitors) for 30 min on ice. Sampleswere then centrifuged at 14,000 rpm at 4°C, and the supernatantswere collected. Protein concentrations in the lysates were determinedby a Coomassie blue protein assay (Pierce Chemical Co., Rockford,IL) using bovine serum albumin standards as references. Lysateswere separated by nonreducing sodium dodecyl sulfate-polyacrylamidegel electrophoresis, transferred to nitrocellulose, and blottedwith antibody to the polyclonal anti-V5 antibody (1 µg/ml;Invitrogen, Carlsbad, CA). To determine receptor tyrosine phosphorylation,the lysates were immunoprecipitated with antibody to phosphotyrosineresidues. Following preclearing, the lysates were incubatedwith phosphotyrosine antibody (4 µg/ml; Upstate Biotechnology,Lake Placid, NY) on ice for 15 min. Complexes were precipitatedwith protein G Sepharose beads overnight at 4°C. The beadswere then washed twice with lysis buffer and boiled for 3 minin nonreducing Laemmli buffer. Tyrosine-phosphorylated proteinswere separated on 10% polyacrylamide gels and transferred tonitrocellulose membranes. The membranes were blocked with 5%milk in Tris-buffered saline and incubated with phosphotyrosineantibody (1 µg/ml; Santa Cruz Biotechnology, Santa Cruz,CA). Subsequently, the membranes were washed and incubated withhorseradish peroxidase-conjugated secondary antibody and detectedby the ECL chemiluminescence detection system (Amersham Biosciences).

Statistical analysis. All data were expressed as means ± standard errors ofthe means. Differences for multigroup comparisons were initiallyassessed by analysis of variance. Differences between specificgroups were determined using a two-tailed Student t test. Statisticaltesting was performed using an SPSS/JMP software program, andstatistical differences were considered significant if the Pvalue was <0.05.

RESULTS

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Results

Fungal ß-glucan particles bind RAW 264.7 macrophages and are internalized. Macrophages are phagocytic cells that possess various receptorsand internalization mechanisms uniquely adapted for the uptakeof specific types of particles. The response to any given particledepends on the specific combination of receptors, internalizationmechanisms, and subsequent signaling cascades employed. We,therefore, investigated the kinetics and mechanisms of S. cerevisiaeß-glucan particle internalization by macrophages.RAW 264.7 macrophages were incubated with DTAF-labeled ß-glucanparticles for increasing times (Fig. 1). Following incubation,the cells were acid stripped to remove loosely bound and noninternalizedparticles. The particles, which appeared to be in the 2- to8-µm size range as determined by light microscopy, wereconsidered internalized if there was clearly a complete rimof surrounding cytoplasm. Fluorescence microscopy demonstratedthat there was association of particles with the outer surfacesof cells within minutes. However, the majority of particleswere not completely internalized until after 1 to 2 h of incubation.To determine whether similar kinetics occurred in native macrophagesand the process was not just a function of the cell line studied,we performed an additional experiment utilizing native rat alveolarmacrophages that were obtained by bronchoalveolar lavage aspreviously described (24, 25). The kinetics of particle internalizationdid not vary significantly between RAW cells and native alveolarmacrophages (data not shown).

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FIG. 1. Internalization of fungal ß-glucan particles. RAW macrophages were treated with DTAF-labeled ß-glucan particles (10 particles/cell) for the times indicated. Cells were washed, fixed, and viewed by fluorescence microscopy. Although ß-glucans bind rapidly, complete uptake of the particles required 1 to 2 h of incubation.

Internalized ß-glucan particles are associated with markers of phagosome formation. We next used antibodies specifically recognizing transferrinreceptor and Lamp-1 as membrane markers to determine interactionsof internalized ß-glucan particles with compartmentsof the endocytic pathway. Transferrin receptor, a marker forearly endocytic pathways, demonstrated staining around internalizedß-glucan particles (Fig. 2A). Staining for Lamp-1,a marker of the late endocytic pathway, also revealed a time-dependentincrease in the appearance of a fluorescent halo surroundingß-glucan particles. All ingested particles were foundto have both transferrin receptor and Lamp-1 surrounding them,which was still visible even after 4 h of incubation (Fig. 2B).

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FIG. 2. Internalized ß-glucan particles associate with early and late phagosome markers. RAW macrophages were incubated with DTAF-labeled ß-glucan particles (10 particles/cell). Panels A and D are phase-contrast micrographs, panels B and E show staining of ß-glucan particles in green and the phagosome markers in red (panel B shows the transferrin receptor, and panel E shows Lamp-1), and panels C and F show the areas indicated by the boxes in panels B and E magnified. In panels A, B, and C the macrophages were stained with antibody to the transferrin receptor, an early phagosome marker, following 60 min of incubation with the particles. The ß-glucan particles (green) were internalized and became surrounded by the transferrin receptor, an early phagosome marker (red halo) (arrows). In panels D, E, and F the macrophages were further stained with anti-Lamp-1 antibody, a late phagosome marker, after 4 h of incubation with the particles. Again, the ß-glucan particles (green) were internalized and became surrounded by Lamp-1 associated with internalized ß-glucan particles (red halo) (arrows).

Internalization of ß-glucan particles is dependent on actin cytoskeleton polymerization but not on caveolar mechanisms. Phagocytosis of particles frequently requires actin polymerization(1, 7, 8). However, additional studies have indicated that caveolaruptake mechanisms can function in the uptake of certain infectiousagents, including specific viruses and certain bacteria (10,11, 15). We therefore utilized inhibitors to target these specificpathways and evaluate their relative contributions to macrophageuptake of fungal ß-glucan particles. RAW macrophageswere incubated with DTAF-labeled ß-glucan particlesfor 4 h in the presence of these inhibitors, and the numbersof internalized particles were determined (Fig. 3A). Nystatin,a drug that binds to cholesterol and causes caveolae to flatten,thereby inhibiting uptake through this mechanism, did not alterthe number of internalized particles from the number observedfor the control group. In contrast, cytochalasin D, an antagonistof actin polymerization, significantly decreased particle internalizationby 90% (P < 0.05 compared to particle uptake in the absenceof inhibitor). These findings were determined in two independentexperiments, and in each experiment at least 250 contiguouscells were visualized. In addition, neither nystatin nor cytochalasinD caused any alteration in RAW macrophage viability. Taken together,these findings indicate that internalization of ß-glucanparticles is dependent on actin cytoskeleton polymerizationbut does not involve interactions with components of caveolaruptake pathways.

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FIG. 3. Actin depolymerization suppresses ß-glucan internalization. RAW macrophages were treated with nystatin (5 µg/ml) or cytochalasin D (CyD) (2 µM) for 30 min prior to challenge with DTAF-labeled ß-glucan particles (10 particles/cell) and during a subsequent 4-h incubation. Cells were washed, acid stripped, mounted on slides, and visualized by fluorescence microscopy. The number of particles per cell was determined by using at least 250 cells in each of two independent experimental runs. The data are means and standard errors. An asterisk indicates that the P value is <0.05 for a comparison with control uptake with no inhibitor.

Macrophage inflammatory activation is not dependent on ß-glucan particle internalization. To determine whether inhibition of ß-glucan internalizationalso alters macrophage inflammatory signaling, we evaluatedthe effect of pharmacologically inhibiting ß-glucaninternalization and subsequent nuclear translocation of p65NF- ${kappa}$ B and production of TNF- ${alpha}$ . We previously reported that cellwall ß-glucans derived from Pneumocystis induce p65NF- ${kappa}$ B activation by 2 h and that this effect is sustained forup to 6 h after the onset of ß-glucan challenge (7).We therefore evaluated p65 NF- ${kappa}$ B nuclear translocation in RAWmacrophages challenged with ß-glucan in the presenceof nystatin and cytochalasin D. Cells were pretreated with theseinhibitors and incubated with ß-glucan particles for2 h, and p65 NF- ${kappa}$ B was localized by fluorescence microscopy.NF- ${kappa}$ B activation was plotted as mean nuclear intensities forthe various treatment groups (Fig. 4A). Treatment with cytochalasinD, a potent antagonist of particle uptake through actin-dependentmechanisms, did not significantly alter fungal ß-glucan-inducedp65 NF- ${kappa}$ B nuclear translocation. Although treatment with nystatinresulted in a slight reduction in p65 NF- ${kappa}$ B nuclear translocation,this translocation was not significantly reduced compared tothat observed for untreated RAW cells challenged with ß-glucanparticles in the absence of inhibitor. These data strongly indicatethat ß-glucan particle internalization through actin-mediatedmechanisms is not necessary for the initiation of inflammatorysignaling pathways in macrophages.

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FIG. 4. Actin-dependent internalization of fungal ß-glucan particles is not necessary for inflammatory signaling. RAW cells were treated with nystatin (5 µg/ml) or cytochalasin D (CyD) (2 µM) prior to stimulation with ß-glucan particles (100 µg/ml). (A) Nuclear translocation of p65 NF- ${kappa}$ B was visualized by immunostaining with a specific antibody recognizing p65 and a Texas Red-conjugated secondary antibody after 2 h. Quantitative differences in fluorescence intensities between nuclei and cytoplasm were calculated and plotted. Inhibition of actin-dependent internalization with cytochalasin D did not alter NF- ${kappa}$ B activation. (B) Release of TNF- ${alpha}$ into the medium was determined by an enzyme-linked immunosorbent assay after 8 h of incubation with fungal ß-glucan in the presence or absence of the same inhibitors. Again, cytochalasin D did not alter TNF- ${alpha}$ release. An asterisk indicates that there was no significant difference for a comparison of macrophages stimulated with ß-glucan in the absence of any inhibitor (i.e., the second bar in each graph) and macrophages stimulated with ß-glucan in the presence of inhibitors. The data are the means and standard errors of the means obtained from three experiments.

We further evaluated the ability of ß-glucan particlesto stimulate macrophage release of TNF- ${alpha}$ , a prototypic inflammatorycytokine, under conditions under which internalization was impaired.Consistent with our previous observations, RAW macrophages werestimulated to release TNF- ${alpha}$ following challenge with ß-glucans(7). We also observed that TNF- ${alpha}$ production was not altered byinhibition of actin internalization pathways (Fig. 4B). Furthermore,TNF- ${alpha}$ release was not altered in the presence of nystatin. Tofurther exclude a defect in cytokine secretion, RAW cells werealso stimulated with LPS (0.1 µg/ml) in the presence ofthese agents. Neither cytochalasin D nor nystatin altered theability of RAW macrophages to signal, as shown by LPS-inducedTNF- ${alpha}$ release in the presence of these inhibitors (data not shown).

Dectin-1 but not TLR2 mediates binding and internalization of purified ß-glucan particles by macrophages. Various receptors have been implicated in mediating the ß-glucaneffects on macrophages. Two of these receptors, dectin-1 andTLR2, have been investigated recently, and some studies havesuggested that there are collaborative interactions betweenthese two receptors (6). To first evaluate the role of TLR2in mediating ß-glucan internalization, we harvestedalveolar macrophages from TLR2^–/– mice and challengedthese cells with fungal ß-glucan particles. Phalloidinstaining of F-actin was used to identify the accumulation ofactin filaments consistent with phagocytic cups surroundingthe ß-glucan particles (Fig. 5). The binding of fungalß-glucan particles and the formation of phagocyticcups were not significantly different for TLR2^–/–and wild-type control macrophages during 60 min of incubation.Furthermore, alveolar macrophages from TLR2^–/– miceproduced just as much TNF- ${alpha}$ as wild-type control macrophagesproduced following ß-glucan stimulation over 8 h.While wild-type C57BL/6 macrophages produced 32,045 ±11,097 pg/ml of TNF- ${alpha}$ following stimulation with ß-glucan,alveolar macrophages from TLR^–/– mice produced 30,800± 11,693 pg/ml of the cytokine (not significantly different).Hence, these data do not support a dominant independent rolefor TLR2 in mediating uptake or macrophage activation in responseto purified fungal ß-glucans.

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FIG. 5. TLR2^–/– alveolar macrophages are capable of binding and internalizing fungal ß-glucans. Alveolar macrophages were harvested from TLR2^–/– and wild-type C57BL/6 control mice. Macrophages were cultured on coverslips and incubated with unlabeled ß-glucan particles for 1 h. The preparations were then fixed, permeabilized, and stained for F-actin filaments using Texas Red-phalloidin. The arrows indicate accumulation of actin filaments consistent with phagocytic cups surrounding ß-glucan particles. The binding of fungal ß-glucan particles and the formation of phagocytic cups were not significantly different for TLR2^–/– and wild-type control macrophages.

In contrast, dectin-1 has recently been shown to participatein phagocytosis and proinflammatory signaling elicited by macrophageschallenged with intact yeast and zymosan, a yeast cell wallfraction composed of both mannoproteins and ß-glucans(2). Therefore, we were interested in evaluating the locationof dectin-1 during interactions of purified fungal ß-glucancell wall components with macrophages (Fig. 6). Dectin-1 receptorswere recruited to areas of ß-glucan particle bindingand uptake within minutes of challenge, and they were consistentlylocalized to areas of phagocytic cups on the macrophage (Fig.6). Furthermore, actin cytoskeleton disruption by cytochalasinD did not affect dectin-1 recruitment to regions of the macrophagesurface membrane interacting with the ß-glucan particles.Thus, we concluded that dectin-1 recruitment to ß-glucanparticles does not depend on the actin cytoskeleton.

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FIG. 6. Dectin-1 recruitment to macrophage membrane regions interacting with fungal ß-glucan particles. RAW macrophages were transfected with V5 epitope-tagged dectin-1 receptor, stimulated with fungal ß-glucan particles for 15 min, and stained with fluorescein isothiocyanate-conjugated anti-V5 antibody. Panels A and C are phase-contrast images, while panels B and D show the fluorescence of the dectin-1 receptor. Dectin-1 recruitment occurred within minutes of contact between ß-glucan particles and cells (A and B). Inhibition of actin polymerization (C and D) did not affect dectin-1 recruitment to the ß-glucan particles. The arrows indicate well-formed surface-localized phagocytic cups containing the dectin-1 receptors.

Dectin-1 is phosphorylated and participates in uptake and macrophage activation in response to purified fungal ß-glucans. Dectin-1 receptors contain a cytoplasmic immunoreceptor tyrosine-basedactivation-like motif. Such motifs have been shown to be involvedin recruitment and binding of signaling molecules. To addresswhether dectin-1 interactions with ß-glucans leadto receptor activation, we assessed the tyrosine phosphorylationstate of dectin-1 receptors in RAW macrophages before and afterstimulation with ß-glucan particles (Fig. 7). Thetotal amount of the recoverable dectin-1 receptor was slightlyreduced following glucan treatment, likely due to interactionswith the particles. However, tyrosine phosphorylation of dectin-1was evident as early as 15 min following fungal ß-glucanstimulation, indicating that there was receptor activation followinginteraction with the purified fungal cell wall component.

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FIG. 7. Dectin-1 interactions with ß-glucan particles results in tyrosine phosphorylation of the receptor. RAW macrophages were transfected with V5 epitope-tagged dectin-1 and stimulated with fungal ß-glucan particles for 15 min, and lysates were prepared. (Top panel) Total lysates were immunoblotted with an antibody recognizing the V5 epitope tag. Incubation of the macrophages with ß-glucan particles even in the presence of proteosomal inhibitors resulted in a slight reduction in recoverable dectin-1 receptor. (Bottom panel) Sequential immunoprecipitation and immunoblotting with an antiphosphotyrosine antibody demonstrated that dectin-1 receptors are phosphorylated following interaction with fungal ß-glucan particles.

Finally, studies were undertaken to antagonize binding of ß-glucanwith dectin-1 receptors and to assess the impact on both particleuptake and associated cytokine release. To accomplish this,dectin-1 was alternately inhibited with either a monoclonalantibody recognizing the receptor (m2A11) or with glucan phosphate,a soluble ß-glucan competitive carbohydrate antagonist(Fig. 8A). Both agents significantly decreased the uptake offungal ß-glucan particles. In addition, TNF- ${alpha}$ secretionwas also substantially antagonized by the inhibition of dectin-1binding to the ß-glucan particles, either with m2A11or with soluble glucan phosphate (Fig. 8B). To further excludeany nonspecific immunoglobulin effect, we also performed controlexperiments with nonimmune immunoglobulin G (IgG). NonimmuneIgG did not have any significant activity in altering ß-glucan-stimulatedTNF- ${alpha}$ release. Specifically, the relative TNF- ${alpha}$ release from ß-glucan-stimulatedRAW macrophages yielded a 100.0% ± 6.4% maximal responsein the absence of antibody, compared to the 120.7% ±7.0% maximal response in the presence of nonimmune IgG (100µg/ml) (not statistically different). Thus, the effectsobserved with antibody m2A11 appeared to be specifically relatedto the effect of m2A11 on dectin-1 rather than to any nonspecificimmunoglobulin activity. The greater decrease in particle internalizationobserved with glucan phosphate could have been due to bindingof receptors other than dectin-1. Together, these data indicatethat dectin-1 appears to be required for efficient ß-glucanparticle internalization and also in the signaling of cytokinerelease.

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FIG. 8. Dectin-1 is necessary for efficient internalization of ß-glucan particles and subsequent inflammatory signaling. RAW macrophages were treated with either m2A11 (100 µg/ml) or glucan phosphate (GluP) (100 µg/ml) and stimulated with DTAF-labeled ß-glucan particles. (A) Internalization of particles was measured after 4 h by fluorescence microscopy and counting. (B) Secretion of TNF- ${alpha}$ into the medium was measured after 8 h by an enzyme-linked immunosorbent assay. Both the anti-dectin-1 antibody m2A11 and the soluble glucan phosphate carbohydrate antagonist significantly reduced the internalization of ß-glucan particles and the subsequent release of TNF- ${alpha}$ . An asterisk indicates that the P value is <0.05 for a comparison with control uptake with no inhibitor.

DISCUSSION

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Discussion

Macrophages are the principal phagocytic component of innateimmunity in the lung. Upon contact with fungal pathogens, ß-glucanson the surface of the fungal cell wall activate macrophagesto release inflammatory mediators. We recently established thatthe opportunistic fungal pathogen Pneumocystis induces macrophageinflammatory activation through NF- ${kappa}$ B signaling by utilizingmechanisms distinct from those utilized during LPS stimulation.The kinetics of the macrophage NF- ${kappa}$ B response to ß-glucansshowed both delayed and sustained activation compared to LPS(7). Therefore, we sought to obtain additional insights intothe mechanisms of internalization of ß-glucan particlesand its potential effect on signaling. The current investigationrevealed that internalization of fungal ß-glucan particlesis actin dependent, but we also demonstrated that internalizationis not required for particle-induced inflammatory signaling.We also observed that dectin-1 interactions, but not TLR2, arenecessary both for efficient internalization and for macrophagecytokine release following ß-glucan stimulation.

The nature of the pathogen interacting with macrophages determinesthe distinct phagocytic mechanisms employed, as well as therelated activation of inflammatory signaling cascades. Actinreorganization, one of the first molecular events involved inphagocytosis, is required for membrane ruffling, phagosome formation,and phagolysosome maturation (1, 7, 8). The current study demonstratedthat actin polymerization at the site of contact between ß-glucanparticles and macrophages is necessary for phagocytosis. Thiswas confirmed by the marked inhibition of fungal ß-glucanparticle uptake in the presence of cytochalasin D, a drug thatinduces depolymerization of actin microfilaments. These findingsare in complete agreement with previous studies that showedthat actin polymerization is required for internalization ofintact yeast and zymosan, a cell wall fraction composed of ß-glucansand mannans (12, 26). In contrast, inhibition of caveolar uptakepathways by nystatin did not have any effect on ß-glucanparticle uptake or macrophage inflammatory signaling.

ß-Glucan particles are purified fractions of fungalcell walls. Although these preparations generally range in sizefrom 2 to 8 µm, they contain variable amounts of smallerparticles visible by light microscopy. These preparations alsoexhibit differences in particle size and relative biologicalactivity depending on the fungal species from which they arederived. Considerable evidence indicates that ß-glucansare potent immune stimulatory agents (9, 14, 25). Our preliminarystudies of macrophage NF- ${kappa}$ B activation indicated that on average,4.85 ± 3.22 particles are associated with each activatedcell over the first hour. However, we have also clearly observedNF- ${kappa}$ B activation in macrophages that do not contain visibly internalizedß-glucan particles following acid stripping, lendingfurther support to the hypothesis that particle interactionswith the cell membrane, rather than particle uptake, are necessaryfor cell activation. Depending on the host cell and conditions,ß-glucans have been shown to interact with a varietyof cell surface receptors, including CD11b/CD18, lactosylceramide,Toll receptors, and dectin-1 (1, 2, 9, 14, 25). The overallbiological effects of any given ß-glucan preparationon a particular host cell likely reflect the size and originof the glucan, which receptor or receptors are available onthe cell for interactions, and the availability of additionalhost proteins that may bind and modulate ß-glucanactivity (23).

Accumulating data indicate that Toll receptors participate ininflammatory signaling in macrophages in response to both intactyeast and zymosan. We previously demonstrated that ß-glucan-inducedTNF- ${alpha}$ secretion from macrophages was partially mediated by MyD88,a Toll receptor adaptor protein (7). Additional studies indicatedthat TLR2 receptors are recruited to phagolysosomes containingzymosan but that their basal surface expression is quite low(22). Our data demonstrate that TLR2 is not a necessary componentfor purified ß-glucan internalization or inflammatorysignaling in RAW macrophages. Alveolar macrophages from TLR2^–/–mice exhibited normal phagocytosis of ß-glucan particlesand potent ß-glucan-induced TNF- ${alpha}$ secretion equivalentto that of wild-type macrophages. Taken together, these dataindicate that while TLR receptors and signaling components maybe involved in macrophage responses, other receptors and pathwayscan compensate and transmit ß-glucan-induced responsesin the absence of TLR2.

Dectin-1 has also been shown to mediate biological effects fromintact yeast and zymosan interacting with macrophages (3). Inthe current investigation we evaluated the interaction of dectin-1with purified ß-glucan particles, which have beenshown to promote inflammatory responses in macrophages. Interactionsof dectin-1 were necessary for both efficient macrophage internalizationand inflammatory activation in response to fungal ß-glucans.Interestingly, glucan phosphate suppressed internalization moreefficiently than the m2A11 monoclonal antibody against dectin-1.It is still possible that glucan phosphate, as a soluble ß-glucancarbohydrate, can interact with multiple receptors involvedin the recognition and uptake of ß-glucans, includingpossibly CD11bCD18 (Mac-1), as well as the dectin-1 receptor(6).

In summary, this study demonstrated that internalization offungal ß-glucan particles derived from S. cerevisiaeis a complex process requiring actin polymerization but notparticipation of components of the caveolar uptake pathways.Internalization of particles through actin-dependent mechanismsis not necessary for the induction of macrophage inflammatoryresponses to ß-glucan particles. Furthermore, dectin-1rather than TLR2 is an integral part of macrophage recognitionof ß-glucan particles, mediating both internalizationand subsequent proinflammatory signaling in response ß-glucancell wall components.

ACKNOWLEDGMENTS

These studies were supported by NIH grants R01 HL55934 and R01HL62150 to A.H.L. and NIH grant R01 GM022942 to R.E.P.

We thank Zvezdana Vuk-Pavlovic and Robert Vassallo for manyhelpful discussions. We also acknowledge Gordon Brown (Universityof Cape Town, South Africa) for his generous gift of antibodym2A11 recognizing dectin-1, David Underhill (University of Washington,Seattle) for providing the V5 epitope-tagged wild-type dectin-1construct, Shizuo Achira (Osaka University, Japan) for his kindgift of TLR2^–/– mice, and David L. Williams (EastTennessee State University, Johnson City) for providing solubleglucan phosphate.

FOOTNOTES

* Corresponding author. Mailing address: 8-24 Stabile Building, Mayo Clinic, Rochester, MN 55905. Phone: (507) 284-2964. Fax: (507) 284-4521. E-mail: limper.andrew{at}mayo.edu.

Editor: T. R. Kozel

REFERENCES

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