Liver X receptors regulate dendritic cell phenotype and function through blocked induction of the actin-bundling protein fascin

doi:10.1182/blood-2006-08-043422

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Blood, 15 May 2007, Vol. 109, No. 10, pp. 4288-4295.
Prepublished online as a Blood First Edition Paper on January 25, 2007; DOI 10.1182/blood-2006-08-043422.

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IMMUNOBIOLOGY
Liver X receptors regulate dendritic cell phenotype and function through blocked induction of the actin-bundling protein fascin
René Geyeregger¹, Maximilian Zeyda¹, Wolfgang Bauer²^,3, Ernst Kriehuber²^,3, Marcus D. Säemann⁴, Gerhard J. Zlabinger⁵, Dieter Maurer²^,3, and Thomas M. Stulnig¹
¹ Department of Internal Medicine III, Clinical Division of Endocrinology and Metabolism, Medical University of Vienna, Austria; ² Division of Immunology, Allergy and Infectious Diseases, Department of Dermatology, Medical University of Vienna, Austria; ³ Center of Molecular Medicine (CeMM) of the Austrian Academy of Sciences, Vienna, Austria; ⁴ Department of Internal Medicine III, Nephrology and Dialysis, Medical University of Vienna, Austria; ⁵ Institute of Immunology, Medical University of Vienna, Austria

   Abstract

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Abstract
Introduction
Materials and methods
Results
Discussion
Authorship
References

Liver X receptors (LXRs) are nuclear receptors regulating lipidand cholesterol metabolism. Recent data revealed a cross talkbetween LXR and Toll-like receptor signaling in macrophages,indicating a role in immunity. Here, we show that LXR ${alpha}$ is expressedin human myeloid dendritic cells (DCs) and induced during differentiationof monocyte-derived DCs, whereas LXRß is expressedconstitutively at a very low level. LXR activation by 2 differentLXR agonists strongly interfered with lipopolysaccharide (LPS)–inducedbut not with CD40L-induced DC maturation by altering DC morphologyand suppressing interleukin-12—but enhancing interleukin-10—secretion.LXR activation in DCs largely blocked their T-cell stimulatoryability despite essentially unaltered expression of variousantigen-presenting and costimulatory molecules. Immunologicsynapse formation was significantly inhibited by LXR activationalong with a complete block in LPS- but not CD40L-induced expressionof the actin-bundling protein fascin. Notably, overexpressionof fascin in LXR agonist–treated DCs restored immunologicsynapse formation and restored their ability to activate T cells.In conclusion, our data reveal LXR as a potent modulator ofDC maturation and function mediated in part by blocking theexpression of fascin. Due to the central position of DCs inimmunity, LXR ${alpha}$ could be a potential novel target for immunomodulation.

   Introduction

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Abstract
Introduction
Materials and methods
Results
Discussion
Authorship
References

Liver X receptors (LXR ${alpha}$ and LXRß) are nuclear receptorsthat are activated by oxidized cholesterols (oxysterols) orsynthetic agonists such as T0901317 or GW-3965. LXRs dimerizewith retinoid X receptors to bind to its response elements inthe promoters of target genes.^1–4 LXR ${alpha}$ is highly expressedin metabolic active organs such as liver, adipose tissue, andkidney, but also in immunocompetent cells such as macrophages,whereas LXRß occurs ubiquitously.⁵ LXRs have beenshown to be implicated in cholesterol, fatty acid, and glucosemetabolism.⁶ Moreover, LXR cross talk with inflammatory signalingpathways in macrophages particularly Toll-like receptor (TLR)signaling has been shown.^6–8 LXR agonists inhibit thelipopolysaccharide (LPS)/TLR4–induced expression of inflammatorygenes by interfering with nuclear factor- ${kappa}$ B signaling in macrophages.⁸
Dendritic cells (DCs) are the most potent antigen-presentingcells (APCs) that are crucial as a linker between innate andadaptive immune responses and play a key role in inflammatorydiseases such as atherosclerosis, rheumatoid arthritis, andallograft rejection.^9–12 After TLR activation, DCs transformfrom antigen-capturing immature DCs (iDCs) into mature DCs (mDCs),a process characterized by up-regulation of T-cell stimulatorycell surface molecules, secretion of inflammatory cytokines,and optimal T-cell stimulatory potency.^13,14 Activation of Tcells by APCs in vivo depends on formation of an immunologicsynapse (IS).¹⁵ This specialized contact zone between T cellsand the APC is dependent on reorganization of cytoskeletal proteinsin both participating cell types.^16,17 Active cytoskeletal changesresult in the dynamic clustering of T-cell surface receptorsand signaling molecules at the interface with the APCs.^15,18During IS formation, DCs actively polarize filamentous actin(F-actin) toward the interface with resting T cells. Fascinis a DC-specific actin-bundling protein expressed only in maturebut not in immature DCs¹⁹ that is required for actin polarizationin DCs during IS formation. Moreover, its expression is a prerequisitefor full T-cell activation.^16,19 In addition to initiation ofimmune responses, DCs are implicated in the induction of centraland peripheral tolerance under conditions of hampered DC maturation.^9,20–23Hence, interfering with DC maturation could be a promising optionfor immunosuppressive strategies in organ transplantation andtreatment of inflammatory diseases.²⁴
The biologic role of LXRs in DCs is unknown so far. We showhere that LXR ${alpha}$ is highly expressed in human DCs and that treatmentof DCs with LXR agonists affects DC phenotype and function particularlyfollowing LPS/TLR4-induced maturation. Thereby, LXR activationleads to impaired IS formation and markedly reduced capacityto promote T-cell activation in mDCs. Molecular studies revealedthat the inhibitory effects of LXRs on DC-mediated T-cell activationare caused by a failure of LPS-stimulated DCs to express fascin.Thus, LXRs not only exert inhibitory effects on the innate immunesystem, but also affect adaptive immunity by interfering withDC maturation and function. These findings indicate that LXR ${alpha}$ could be an interesting novel drug target for immunosuppressiveagents.

   Materials and methods

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Abstract
Introduction
Materials and methods
Results
Discussion
Authorship
References

Cell isolation and culture
Peripheral blood mononuclear cells (PBMCs) were isolated fromacid citrate dextrose (ACD) buffy coats of healthy (70% male;no sex-specific differences were observed; data not shown) donorsby density gradient centrifugation using Ficoll-Pacque (Pharmacia,Uppsala, Sweden). For isolation of myeloid DCs, PBMCs were depletedfrom monocytes by anti-CD14–conjugated magnetic MicroBeads(Miltenyi Biotec, Bergisch Gladbach, Germany). Peripheral bloodmyeloid DCs (purity > 80%) were magnetically isolated fromCD14^– cells using the CD1c (BDCA-1) Dendritic Cell IsolationKit (Miltenyi Biotec) according to the manufacturer's instructions.Myeloid DCs (2 x 10⁵ cells/mL) were directly analyzed or culturedfor 2 days in culture medium consisting of RPMI 1640 (Invitrogen,Groningen, the Netherlands) including 50 U/mL penicillin and50 µg/mL streptomycin, 2 mM glutamine (Invitrogen), and10% fetal bovine serum (Hyclone, Logan, UT).
For monocyte-derived DC differentiation, CD14⁺ monocytes wereisolated from PBMCs by magnetic cell sorting using anti-CD14–conjugatedmagnetic microbeads (Miltenyi Biotec) achieving a purity of95% to 99%. DCs were differentiated and matured as described²⁵in RPMI including supplements as described for myeloid DCs.LXR agonists T0901317 (Calbiochem, San Diego, CA) and GW-3965(generously provided by T. Willson and J. Collins; GlaxoSmithKline,Philadelphia, PA) were added at day 2 at 2 µM and didnot affect cell viability as assessed by propidium-iodide (Sigma,St Louis, MO) staining. Key experiments were repeated with additionof LXR agonists at day 5 yielding essentially the same results(not shown). For morphologic and immunofluorescence analysis,cells were embedded with mounting medium Vectashield (VectorLaboratories) and evaluated by light microscopy on an Aristoplan307 microscope (Leitz, Wetzlar, Germany) using a Pl FluotarPhaco 2 40x/0.70 objective lens. Images were captured with a300F camera (Leica Microsystems, Wetzlar, Germany) and analyzedby Leica IM500 software.
CD3⁺ T cells (purity > 95%) were isolated by magnetic depletionof non-T cells, as described.²⁶ For highly purified CD4⁺ andCD8⁺ T cells (purity > 98%), additional beads labeled withmAbs against CD19 (J4.119), CD56 (C218), CD34 (581), CD41 (P2),glycophorin A (11E4B7.6), and CD8 (B9.11) or CD4 [13B9.2] wereincluded.²⁷ All antibodies were purchased from Immunotech (Marseille,France). Naive CD4⁺CD45RA⁺ T-helper cells (purity > 85%)were isolated from PBMCs using the naive CD4⁺ T-cell isolationKit (Miltenyi Biotec) according to the manufacturer's instructions.
Gene expression analysis
Total RNA was isolated and reverse-transcribed as described,²⁵with the modification of adding Glycoblue (Ambion, Austin, TX)for coprecipitation. Expression of LXR ${alpha}$ , LXRß, andRXR ${alpha}$ mRNAs was quantitated by quantitative real-time reverse-transcription–polymerasechain reaction (QRT-PCR) using Taqman Assays-on-Demand (AppliedBiosystems, Foster City, CA) according to the manufacturer'sinstructions and normalized to 18S RNA using the comparativedCt-method.²⁸
Cytokine production and cell surface marker expression
Cytokines secreted by DCs (interleukin-12p40 [IL-12p40], IL-12p70,and IL-10) and T cells (IL-2, IFN- ${gamma}$ , IL-4, IL-5, IL-10, and IL-13)were analyzed by enzyme-linked immunosorbent assay (ELISA) asdescribed²⁹ or by commercially available kits (all R&D Systems,Minneapolis, MN). Surface molecule expression was analyzed byFITC-labeled anti-CD40 (Immunotech) and anti–human leukocyteantigen–DR (HLA-DR), and PE-labeled anti-CD80, anti-CD86,anti–HLA-ABC, and anti–mannose receptor (MR; allBD Biosciences, San Jose, CA). For analyzing T-cell activation,T cells were stained with FITC-labeled anti–T-cell receptor(TCR) or allophycocyanin-labeled anti-CD3, together with PE-labeledanti-CD25 or anti-CD69 (BD Biosciences), respectively. Cellswere analyzed on a FACSCalibur flow cytometer (Becton Dickinson,San Jose, CA).
Mixed leukocyte reaction (MLR)
DCs were irradiated (30 gray, ¹³⁷Cs source), washed, and subsequentlyadded at increasing cell numbers to 1 x 10⁵ allogeneic CD3⁺,CD4⁺, or CD8⁺ T cells in 96-well culture plates, and proliferationwas determined after pulsing with 1 µCi (0.037 MBq) [³H]-thymidine(ICN Pharmaceuticals, Irvine, CA) at day 4 of culture as described.²⁶To assess cytokine production and activation markers of T cellsin MLR, mature DCs (2 x 10⁵/well) were cocultured with 1.5 x10⁶ CD3⁺ T cells for 2 days in 12-well plates. For restimulationexperiments, T cells from day 4 of the MLR were washed and restedfor 24-hour culture medium including supplements as describedabove and restimulated with 10 ng/mL PMA (Sigma) and 1 µMionomycin (Sigma) for 96 hours. Subsequently, the cell-freesupernatant was analyzed for cytokine production.
Transfection of DCs
A pEGFP-C1-fascin-1 plasmid containing the full-length of humanfascin-1 coding sequence (1.5 kb, GenBank U09873 [GenBank] ) was generouslyprovided by Josephine C. Adams (Lerner Research Institute, Ohio)and used for transfection along with pEGFP-C1 empty vector plasmid(Clontech Laboratories, Palo Alto, CA). After 1-day maturationof DCs with LPS, the cells were harvested, washed with PBS,and resuspended in the specified electroporation buffer (Amaxa,Cologne, Germany) to a final concentration of 2 x 10⁶ cells/mL.Plasmid DNA (15 µg) was mixed with 0.1 mL cell suspension,transferred to a 2.0-mm electroporation cuvette, and transfectedwith an Amaxa Nucleofector apparatus (Amaxa). After electroporation,cells were immediately transferred to 2 mL culture medium andcultured for 24 hours in 6-well plates at 37°C. Optionally,transfected pEGFP-C1–positive and pEGFP-C1-fascin fusionprotein–positive cells were subjected to fluorescence-activatedcell sorting (FACS, FACSAria; BD Biosciences) and were usedfor further experiments. The viability of DCs directly and 24hours after transfection was 90% and 50%, respectively, whereas48 hours after transfection the viability was essentially lessthan 20%, which was not sufficient for activating peripheralT cells in our study. The purity of sorted cells was generallymore than 98%.
Analysis of IS formation
For superantigen stimulation, transfected or CellTracker Orange(CMTMR; Molecular Probes, Eugene, OR)–labeled untransfectedDCs were pulsed with 5 µg/mL staphylococcal enterotoxinE (SEE; Toxin Technology, Saratosa, FL) in Hank balanced saltsolution (HBSS) at 37°C for 30 minutes. After washing, DCswere incubated with Jurkat E6-1 T cells at a ratio of 1:1 at37°C for 30 minutes. Of note, Jurkat T cells spontaneouslyform conjugates with DCs even in unstimulated cells (data notshown). Relocalization of CD3 and PKC ${theta}$ toward the IS was analyzedas described.³⁰ The percentage of T cells forming conjugateswith DCs was determined by counting at least 100 T-cell/DC conjugatesper blinded sample by 2 individuals. No relocalization of CD3was seen without SEE stimulation (data not shown).
Intracellular fascin staining
For intracellular fascin staining, cells were permeabilizedwith methanol for 30 minutes at room temperature, and washedtwice with PBS/1% BSA (Sigma). Cells were stained with anti–humanfascin 1 mAb 55K-2 from Santa Cruz Biotechnology (Santa Cruz,CA) followed by staining with FITC-labeled goat anti–mouseF(ab')₂ Ab (DAKO, Glostrup, Denmark). All antibodies were incubatedfor 30 minutes at 4°C. After washing with PBS/1% BSA, fascinstaining of cells was analyzed on a FACSCalibur.
For immunofluorescence images, cells (1 x 10⁶) were mechanicallydetached from plates washed with PBS and allowed to settle onpoly-L-lysine–coated slides (Marienfeld, Lauda-Koenigshofen,Germany) for 30 minutes on ice. For fascin staining, cells werepermeabilized with methanol for 30 minutes at room temperatureand treated with the anti–human fascin Ab in PBS/1% BSAfollowed by Alexa Fluor 488–labeled F(ab')₂ fragment ofgoat antimouse (Molecular Probes). All antibodies were incubatedfor 30 minutes at 4°C. After washing with PBS, slides weredried by a piece of paper and embedded with mounting medium(Vector Laboratories, Burlingame, CA).
Statistics
Data are presented in means ± SEM. Comparisons were performedby 2-tail unpaired Student t test, and a P value less than .05was considered statistically significant.

   Results

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Abstract
Introduction
Materials and methods
Results
Discussion
Authorship
References

Human DCs highly express LXR ${alpha}$
To investigate whether human DCs express LXRs, we analyzed CD1c⁺myeloid DCs purified from peripheral blood. We found that freshlyisolated myeloid DCs expressed significantly more LXR ${alpha}$ mRNA comparedwith monocytes (+56%; P = .04). Notably, myeloid DCs stronglyup-regulated LXR ${alpha}$ expression (about 15-fold) after 2 days ofculture (Figure 1A), when they resemble fully differentiatedDCs as found in peripheral tissues.³¹ Since monocyte-derivedDCs are a useful model system for studying DCs in vitro, weexamined LXR ${alpha}$ expression in these cells. Immature DCs expressedabout 16 times more LXR ${alpha}$ mRNA than monocytes, and LXR ${alpha}$ expressionwas not significantly up-regulated after 2 days of LPS-inducedmaturation (Figure 1A). mRNA concentrations of LXR ${alpha}$ and LXRßat day 0 (d0) were very similar to each other as estimated bynearly identical dCt values (9.2 ± 0.4 vs 8.6 ±0).³ Taking into account the marked up-regulation of LXR ${alpha}$ duringDC differentiation, these data indicate that LXR ${alpha}$ is by far theprominent LXR isoform in DCs. In addition, RXR ${alpha}$ , the heterodimerpartner of LXRs, was uniformly expressed in monocytes and differenttypes of DCs (data not shown).

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Figure 1. LXR ${alpha}$ , LXRß, and RXR ${alpha}$ expression in human DCs. (A) mRNA expression of LXR ${alpha}$ was analyzed in human peripheral blood CD14⁺ monocytes (set to 100%), myeloid DCs (myDCs) directly after isolation and after 2 days in culture (2d-myDCs), as well as of monocyte-derived immature DCs (iDCs) and mature DCs (mDCs) by QRT-PCR. (B) LXR ${alpha}$ and LXRß induction during DC differentiation. LXR ${alpha}$ and LXRß mRNA expression were analyzed at different time points during DC differentiation from monocytes (d0 set to 100%). Data show means and SEM of 4 independent experiments.

LXR agonist treatment affects DC phenotype
The strong induction of LXR ${alpha}$ in DCs points to a possible functionalrole of LXR in these cells. First, we examined the impact ofLXR agonists (T0901317 and GW-3965) on the morphology of immatureand mature monocyte-derived DCs in culture. iDCs show unalteredmorphology when treated with LXR agonist (Figure 2A). AfterDC maturation by LPS, untreated mDCs become nonadherent to plasticand form large clusters (Figure 2A). However, LXR agonist–treatedDCs remained adherent to the culture plate after LPS-inducedmaturation, formed only few cell clusters, and exhibited a widespreadshape (Figure 2A).

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Figure 2. Effect of LXR agonist treatment on DC morphology, differentiation, and maturation. Immature DCs (iDCs) were differentiated for 7 days and left untreated (control) or treated from day 2 on with 2 µM of the LXR agonists T0901317 (T09) or GW-3965 (GW). Mature DCs were obtained from iDCs by incubation with LPS for the last 2 days. (A) The maturation-induced clustering of DCs and morphologic changes were analyzed by a phase-contrast microscopy. Bar represents 30 µm. Similar results were obtained in 4 different experiments. (B) Surface molecule expression as analyzed by immunofluorescence and flow cytometry. Histograms illustrate staining with isotype control mAb (open profile, fine line), and staining with mAb of the indicated specificity of untreated DCs (solid profiles) and of T0901317-treated (T09) DCs (open profiles, bold line). The logarithm of fluorescence intensities (FIs) is given in the abscissa spanning 4 orders of magnitude. One typical experiment of 10 is shown. Essentially identical results were obtained with GW-3965 (n = 4; data not shown).

Expression of a variety of cell surface molecules normally presenton iDCs (CD1b, CD1c, CD14, CD80, CD86, HLA-ABC, and HLA-DR)was essentially unaltered by LXR agonist treatment (P > .05),whereas expression of CD1a and CD40 was moderately but significantlydecreased (Figure 2B). In DCs that have been stimulated by LPSto induce maturation, the expected up-regulation of distinctsurface molecules CD40, CD80, and HLA-DR as well as their finalexpression in mDCs were essentially unaffected by both LXR agonistswith the exception of CD86 and HLA-ABC expression, whose expressionwas reduced to a moderate but statistically significant extent(Figure 2B). Thus, despite the gross alterations in mDC shape,LXR activation had only a minor impact on surface molecule expressionof immature and mature DCs.
LXR agonist treatment affects DC function
To investigate a potential functional role of LXRs in DCs, wefirst analyzed the impact of LXR agonists on DC cytokine production.Secretion of IL-12p40 and the functional form IL-12p70 was significantlydecreased in LXR agonist–treated compared with untreatedmDCs (Figure 3A). In contrast, production of IL-10 was increasedby more than 5-fold in LXR agonist–treated compared withuntreated mDCs.

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Figure 3. LXR agonist treatment of DCs leads to altered cytokine production and diminished ability to activate T cells. (A) Immature monocyte-derived DCs (iDCs) were differentiated for 7 days and left untreated (control) or treated from day 2 on with 2 µM of the LXR agonists T0901317 (T09). Mature DCs were obtained from iDCs by incubation with LPS for the last 2 days. After 2 days of LPS-induced DC maturation, cell-free supernatants were analyzed for IL-12p40, IL-12p70, and IL-10 secretion by ELISA in 7 different experiments. (B) Allogeneic T cells were cocultured with untreated or T0901317-treated (T09) iDCs and mDCs, respectively. CD25 and CD69 expression on CD3⁺ T cells was analyzed by flow cytometry after 2 days of coculture in 3 independent experiments. (C) Allogeneic T cells were cocultured for 2 days with DCs that have been treated or not with T09 as in panel B, and cell-free supernatants were analyzed for IL-2 and IFN- ${gamma}$ secretion (n = 3). (D) T-cell restimulaton. After 4 days of coculture, T cells were extensively washed, and restimulated with PMA/ionomycin. Cell-free supernatants of cocultures were analyzed for secretion of indicated cytokines. Significance versus untreated iDCs (*P $≤$ .05) or mDCs (***P < .001). Data show the means and SEM of 3 independent experiments.

The most important function of DCs is their ability to activateT cells. When stimulated with LXR agonist–treated comparedwith untreated mDCs, allogeneic T cells showed markedly reducedCD25 and CD69 surface expression as well as significantly reducedproduction of the T-helper cell type 1 (Th1) cytokines IL-2and IFN- ${gamma}$ (Figure 3B-C; also see Figure S1, available on theBlood website by clicking on the Supplemental Figure link atthe top of the online article). Since Th2 cytokine secretionwas not detectable in primary allogeneic MLR (data not shown),we restimulated these cells with PMA/ionomycin.³² The productionof Th2 cytokine IL-5 was increased in restimulated cells, whereasIL-4, IL-10, and IL-13 were not significantly altered (Figure 3D).The production of IFN- ${gamma}$ was also down-regulated in restimulatedcells. These data suggest that LXR activation in DCs not onlyinhibits Th1 responses but also promotes polarization towarda Th2 response. The final hallmark of T-cell activation is inductionof proliferation. Stimulation of CD4⁺ T cells by DCs is consideredto rely mainly on expression of major histocompatability complex(MHC) class II molecules.^13,33,34 However, although MHC II (HLA-DR)expression was unaltered in LXR agonist–treated mDCs (Figure 2B),their ability to induce proliferation of allogeneic CD4⁺, CD8⁺,as well as naive CD4⁺ CD45RA⁺ T cells was drastically reducedto a level comparable with that of iDCs (Figure 4A; and datanot shown). Notably, LXR agonists did not directly affect T-cellproliferation as assessed by stimulating T cells with CD3/28antibodies in presence and absence of LXR agonist (data notshown and Walcher et al³⁵).

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Figure 4. LPS- but not CD40L-matured LXR agonist–treated DCs fail to stimulate T cells. (A) Immature DCs (iDCs) were differentiated for 7 days and left untreated (control) or treated from day 2 on with 2 µM of the LXR agonist T0901317 (T09). Mature DCs were obtained from iDCs by incubation with LPS for the last 2 days. At day 7, immature and LPS-matured DCs were washed extensively, irradiated, and cocultured with 1 x 10⁵ allogeneic purified CD4⁺ T cells at the indicated ratios. After 4 days, proliferation was measured by [³H]-thymidine incorporation in 4 independent experiments. (B) Allogeneic MLRs were performed as described for panel A using LPS- and CD40-matured DCs, respectively. *P $≤$ .05 for difference between T09-treated versus untreated DCs. Data show the means and SEM of 4 independent experiments.

The block in T-cell stimulatory capacity of LXR agonist–treatedmDCs emphasized an interference of LXR with the process of DCmaturation. Since DC maturation can be accomplished by differentstimuli, we next tested whether the alterations found in LPS-inducedmDCs were also apparent when DC maturation was induced by CD40Ligand(CD40L). However, the inhibitory effect of LXR agonist on DC-inducedCD4⁺ T-cell proliferation did not occur with CD40L-induced mDCs(Figure 4B). Taken together, LXR agonist treatment stronglyimpaired critical mDC functions including T-cell activationselectively after LPS- but not CD40L-induced maturation.
LXR agonist treatment strongly impairs fascin expression and IS formation
Several findings of this study (eg, alterations in cell morphology,DC clustering, and impairment of CD4⁺ T-cell stimulation inMLR despite unaltered MHC II expression) pointed to a possibleinvolvement of LXRs in regulating cytoskeletal functions inTLR4-matured mDCs. Since the actin-bundling protein fascin isstrongly related to DC cytoskeletal functions such as dendriteformation and required for DC-mediated T-cell stimulation, weanalyzed its expression in DCs following LXR agonist treatment.¹⁹LPS-induced expression of fascin as assessed by flow cytometrywas essentially abolished by LXR agonists (Figure 5A). Alongwith unaltered induction of CD4⁺ T-cell proliferation (Figure 3C),the expression of fascin in LXR agonist–treated and CD40L-maturedDCs remained essentially unaffected (Figure 5A). In addition,the LXR agonist–induced inhibition of fascin expressionon LPS-matured DCs was further analyzed by immunofluorescencemicroscopy. Whereas untreated LPS-matured DCs showed numerousfascin-containing dendrites following mechanical detachmentfrom the plate for immunofluorescence analysis, LXR agonist–treatedmDCs almost completely lacked fascin expression and dendrites(Figure 5B lower panel). These findings emphasize a criticalrole of blocked fascin expression in the LXR-mediated DC maturationdefect.

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Figure 5. LPS- but not CD40L-matured LXR agonist–treated DCs fail to up-regulate fascin expression. (A) Immature DCs (iDCs) were differentiated for 7 days and left untreated (control) or treated from day 2 on with 2 µM of the LXR agonist T0901317 (T09). Mature DCs were obtained from iDCs by incubation with LPS or CD40L for the last 2 days. Histograms with open profiles (fine line) represent a staining pattern with an isotype control. T0901317-treated DCs (open profiles with bold line) and untreated DCs (solid profiles) show a staining pattern with the antifascin Ab. Typical histograms and diagrams showing mean of fluorescence intensities related to those obtained from untreated mDCs ± SEM of at least 4 independent experiments are given. Significance versus untreated mDCs: ***P $≤$ .001. (B) Typical light microscopy images and immunofluorescence staining of fascin of untreated and T09-treated LPS-matured DCs with different magnifications are shown. Bar represents 10 µm. Similar results were obtained in 4 different experiments.

Sustained TCR engagement by mDCs is important for full T-cellactivation and depends on the formation of the IS. Actin cytoskeletalpolarization in DCs that includes fascin was shown to be essentialfor IS formation.³⁵ As shown in Figure 6, IS formation (as assessedby the number of conjugates with relocalized CD3) was low withiDCs (18.5% ± 0.5%) and independent of LXR agonist treatment.IS formation was also not altered by LXR agonist treatment withmDCs that had been matured with CD40L (42.5% ± 1.5% vs41.5% ± 8.2% in LXR agonist–treated vs untreatedDCs). In contrast, the number of conjugates with relocalizedCD3 was markedly diminished in LXR agonist–treated comparedwith untreated mDCs (28.6% ± 4.4% vs 46.2% ± 4%)when DCs had been matured with LPS (Figure 6). Relocalizationof PKC ${theta}$ to the IS was not affected by LXR agonist treatment (Figure 6).Thus, the LXR-mediated blockage of fascin expression in LPSbut not CD40L-matured DCs strikingly correlates with the bluntedability of mDCs to present the T-cell receptor/CD3 complex withinthe context of an IS and subsequent T-cell activation.

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Figure 6. LPS- but not CD40L-matured LXR agonist–treated DCs fail to induce IS formation. Immature DCs (iDCs) were differentiated for 7 days and left untreated (control) or treated from day 2 on with 2 µM of the LXR agonist T0901317 (T09). Mature DCs were obtained from iDCs by incubation with LPS or CD40L for the last 2 days. Mature DCs were pulsed with superantigen for 30 minutes and incubated with Jurkat T cells for an additional 30 minutes. CD3 ${epsilon}$ and PKC ${theta}$ relocalization was visualized by indirect immunofluorescence. Typical examples of conjugates, negative (left) or positive (right) for relocalization of CD3 ${epsilon}$ and PKC ${theta}$ , are shown. Bar represents 10 µm. The diagram shows the percentage of conjugates counted positive for CD3 ${epsilon}$ and PKC ${theta}$ relocalization in means ± SEM of 4 independent experiments. Significance versus untreated mDCs: *P $≤$ .05.

Overexpression of fascin in LXR agonist–treated mDCs restores their ability to form an IS and activate T cells
In order to test whether blunted fascin expression underliesLXR-mediated inhibition of IS formation and DC-induced T-cellactivation, we transfected LXR agonist–treated and untreatediDCs and mDCs with either a plasmid encoding the GFP-linkedfull-length human fascin protein (fascin) or the empty GFP expressionvector (vector). The transfection efficiency of iDCs with eithervector or fascin plasmid was about 30% (data not shown). Transfectionof mDCs resulted in 24% positive cells when transfected withthe vector plasmid and about 14% when transfected with the fascinplasmid (data not shown). LXR agonist treatment reduced thetransfection efficiency of mDCs transfected with the vectorplasmid to 14% and fascin plasmid to 7% (data not shown). ISformation of DCs pulsed with superantigen SEE was assessed byCD3 relocalization to the T-cell/DC interface. Approximately16% of conjugates between plasmid-expressing iDCs and T cellsrelocalized CD3 to the IS independently of LXR agonist treatmentand the type of transfected plasmid (Figure 7A). As expectedfrom untransfected cells (Figure 6), LXR agonist treatment inhibitedCD3 relocalization of T cells to vector-transfected mDCs downto levels found in iDCs. However, CD3 relocalization to theIS was completely restored in LXR agonist–treated mDCsthat were transfected with fascin (Figure 7A). These data showthat fascin expression alone is sufficient to prevent the LXR-mediatedblock in IS formation of LPS/TLR4-stimulated DCs.

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Figure 7. Overexpression of fascin in LXR agonist–treated DCs leads to enhanced IS formation and further T-cell activation. Immature DCs were differentiated for 6 days and left untreated (untr) or treated from day 2 on with 2 µM LXR agonist T0901317 (T09). Mature DCs were obtained from iDCs by incubation with LPS for the last day. iDCs and mDCs were then transfected with pEGFP-C1-vector (vector) or pEGFP-C1-fascin (fascin) plasmid. (A) At 24 hours after transfection, DCs were pulsed with superantigen for 30 minutes and incubated with Jurkat T cells for an additional 30 minutes. CD3 ${epsilon}$ relocalization was visualized by indirect immunofluorescence. Typical examples of conjugates, negative (left) or positive (right) for relocalization of CD3 ${epsilon}$ , are shown. Bar represents 10 µm. The diagram shows the percentage of conjugates counted positive for CD3 ${epsilon}$ relocalization in means ± SEM of 4 independent experiments. Significance versus T09 + vector: *P $≤$ .05. (B) At 24 hours after transfection, GFP-positive DCs were FACS sorted to a purity of 98%. FACS-sorted pEGFP-C1–positive DCs were pulsed with superantigen for 30 minutes and incubated with Jurkat T cells at a DC/T-cell ratio of 1:8 and 1:16 for 24 hours. Expression of CD25 and CD69 was analyzed by 2-color flow cytometry. Diagram shows geometric mean fluorescence intensities (MFIs) ± SEM related to those obtained from T09-treated vector–transfected DCs (T09 + vector, set to 100%) of 3 independent experiments. Significance versus T09-vector: *P $≤$ .05.

To further evaluate the biologic importance of decreased fascinexpression for LXR-mediated inhibition of DC-induced T-cellactivation, we analyzed activation marker expression of T cellsstimulated with isolated vector- or fascin-transfected mDCs.Fascin transfection had no effect on induction of CD25 and CD69on T cells stimulated with untreated SEE-pulsed mDCs (Figure 7B).Induction of CD25 and CD69 expression was largely reduced byLXR agonist treatment in vector-transfected mDCs as expectedfrom data with allogeneic T cells (Figure 7B; cf Figure 3A-B).Strikingly, when cells were transfected with fascin, the inhibitoryeffect of LXR agonist treatment on mDC-induced T-cell activationmarker expression was significantly neutralized (Figure 7B).These data indicate that down-regulation of fascin expressionconstitutes one molecular mechanism by which LXR mediates itsinhibitory action in mDCs to reduce their T-cell stimulatoryability.

   Discussion

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Nuclear receptors regulate gene expression for a variety ofcellular functions including metabolic processes. From the so-calledorphan nuclear receptors that are mostly involved in metabolicregulation, only peroxisome proliferator-activated receptor ${gamma}$ (PPAR ${gamma}$ ) has been described to control DC function so far.^31,36,37Here we show that LXR ${alpha}$ , the LXR paralogue known to be primarilyinvolved in regulation of lipid metabolism, is highly expressedin peripheral myeloid as well as monocyte-derived DCs alongwith constitutive expression of LXRß and the heterodimerpartner RXR. The abundant expression of LXR ${alpha}$ compared with LXRßin DCs indicates that LXR ${alpha}$ is the predominant LXR in DCs, andeffects of unselective LXR ${alpha}$ /ß agonists as used hereare mediated primarily via LXR ${alpha}$ . Moreover, the strong inductionof LXR ${alpha}$ during DC differentiation suggests a physiological roleof this nuclear receptor in DCs.
Data on the impact of LXRs in immunity have essentially beenconfined to the innate part of the immune system, particularlyby controlling cholesterol efflux and inflammatory cytokineproduction in macrophages.^8,38 In contrast, few effects of LXRagonists have been reported on the adaptive immune system namelyon T-cell cytokine production without directly affecting T-cellproliferation.³⁵ The data presented here point to a criticalrole of LXR ${alpha}$ in DCs, which link innate and adaptive immunity.The functionally most significant finding in our study is thatDC-induced T-cell proliferation was abolished when LXR agonist–treatedDCs were used as stimulators. Since activation of primary Tcells depends on DCs, these data suggest a profound block inprimary T-cell responses upon LXR agonist treatment.
Our data on diminished T-cell stimulation despite essentiallyunaltered stimulatory molecule expression on the DC surfacesupport the notion that surface expression of these moleculesalone does not account for the exceptional ability of DCs toactivate antigen-dependent immune responses.^37,39 However, functionalactin cytoskeleton is required for full T-cell activation includingIS formation and DC-driven T-cell activation independent ofMHC II expression.¹⁹ Thus, our data on blocked IS formationand unaltered MHC II expression in LXR agonist–treatedDCs suggest that alterations in cytoskeletal function couldunderlie the observed defects in DC-mediated T-cell proliferation.
Induction of the actin-bundling protein fascin^40,41 followingLPS-induced DC maturation was almost completely abolished byLXR agonist treatment along with impaired T-cell stimulatorycapacity. Support for an involvement of fascin in LXR-mediatedeffects comes from our experiments with CD40L-matured DCs, inwhich LXR agonist treatment did not inhibit induction of fascinexpression along with only minimal impairment of their T cell-stimulatorycapacity. Based on these data, we hypothesized that lack offascin expression is a crucial mechanism of the inhibitory effectsof LXR in DCs. According to the function of cytoskeletal rearrangementsin IS formation, overexpression of fascin in LXR agonist–treatedDCs completely restored DC-induced CD3 relocalization to theIS, indicating that diminished fascin expression is a crucialmechanism by which LXR regulates IS formation. Moreover, thesedata illustrate the requirement of fascin in human DCs for ISformation. Unfortunately, the viability of human DCs rapidlydeclined within a few days following transfection thereby preventinginduction of significant T-cell proliferation by transfectedDCs and a direct test of restored DC fascin expression on thisreadout. Nonetheless, restoration of CD25 and CD69 expressionon T cells stimulated with LXR agonist–treated DCs byoverexpressing fascin strongly indicated the functional significanceof impaired IS formation due to LXR-mediated abolishment offascin expression in LPS-matured DCs. Since functional restorationby fascin overexpression was not complete, additional mechanismsof LXR action on DC ability to stimulate T cells cannot be excluded.Notably, neutralizing anti–IL-10 antibodies did not restorethe T-cell stimulatory ability of LXR agonist–treatedDCs in MLRs (data not shown). However, altered production offunctional IL-12p70 during the MLR as well as polarization ofT cells toward a Th2 response and secretion of cytokines otherthan those investigated here could contribute to LXR-mediatedeffects on DC stimulatory activity independently of abolishedfascin expression.
The selective inhibitory effect of LXR activation on LPS- butnot CD40L-induced DC maturation indicates that LXRs specificallyinterfere with LPS signaling. LXR-mediated inhibition of LPS/TLR4signaling has been shown in macrophages by antagonizing NF- ${kappa}$ Bsignaling thereby reducing proinflammatory cytokine expression.⁸TLR4 signals via myeloid differentiation primary response gene88 (MyD88) and Toll–IL-1 receptor domain-containing adaptor-inducinginterferon-ß (TRIF), which together activate nuclearfactor- ${kappa}$ B and mitogen-activated protein kinases (MAPKs), whereasCD40 activation implicates tumor necrosis factor (TNF) receptor–associatedfactor (TRAF) and Src family kinases,^42,43 giving rise to multiplepossibilities for selective interaction by LXR. However, theprecise mechanism how LXRs interfere with TLR4 signaling hasnot yet been resolved in any cell type.
DCs are critically involved in a variety of immune disorderssuch as rheumatoid arthritis, atherosclerosis, diabetes, andothers.^{12,13,44–48} Hence, alterations of DC phenotypeand function such as those induced by LXR agonists could bean option for immunosuppression and treatment of these diseases.In addition, DCs are capable of inducing central and peripheraltolerance,^9,20,22,23 and impaired DC maturation leading to inadequatelymatured DCs has repeatedly been shown to be an inducer of tolerance.^{10,26,49–51}Hence, LXR activation in DCs might be an attractive approachfor tolerance induction that is highly desirable in variousT-cell–mediated disorders such as autoimmune diseasesand allograft rejection.^9,20,22,23
In conclusion, the present study reveals a novel role of LXRsat the interface of innate and adaptive immune responses bycritically interfering with DC maturation and function. Althoughthe physiological role of LXRs and endogenous LXR agonists onDCs remains obscure, to date the marked impact of syntheticLXR agonists on DCs shown here bears novel possibilities forimmunosuppressive strategies and tolerance induction. Sinceunselective LXR agonists exert dramatic side effects such ashypertriglyceridemia, highly selective LXR modulators targetingLXR ${alpha}$ in distinct cell types are currently being developed.³⁸Such selective LXR modulators specifically acting on DCs couldbecome reasonable agents for novel immunosuppressive strategiesfor treatment of inflammatory and autoimmune diseases and preventionof allograft rejection.

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References

Contribution: All authors have contributed substantially tothe present publication. R.G., M.Z., and T.M.S. principallydesigned the study and largely wrote the paper; W.B. and E.K.performed significant experimental procedures; and M.D.S., G.J.Z.,and D.M. helped to analyze and interpret the data and helpedto write the paper.
Conflict-of-interest disclosure: The authors declare no competingfinancial interests.
Correspondence: Thomas M. Stulnig, Clin. Div. Endocrinologyand Metabolism, Dept. Internal Med. III, Medical Universityof Vienna, Währinger Gürtel 18-20, A-1090 Vienna,Austria; e-mail: thomas.stulnig{at}meduniwien.ac.at.

   Acknowledgments

This work was supported by grants from the Austrian ScienceFund (P16788 [GenBank] -B13 and P18776 [GenBank] -B11 [T.M.S.], and SFB2308 [D.M.]).
We thank T. Willson and J. Collins (GlaxoSmithKline) for providingthe synthetic LXR agonist GW-3965; J. T. Adams (Lerner ResearchInstitute, Cleveland, OH) for providing the pEGFP-C1–vectorand pEGFP-C1–fascin plasmids; and Bianca Weissenhorn,Margarete Mario, and Bärbel Reininger for excellent technicalassistance.

   Footnotes

Submitted August 31, 2006; accepted January 18, 2007.
Prepublished online as Blood First Edition Paper, January 25, 2007 DOI: 10.1182/blood-2006-08-043422

An Inside Blood analysis of this article appears at the frontof this issue.

The online version of this article contains a data supplement.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 USC section 1734.

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