Superantigen recognition by HLA class II on monocytes up-regulates toll-like receptor 4 and enhances proinflammatory responses to endotoxin

doi:10.1182/blood-2004-07-2523

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Blood, 1 May 2005, Vol. 105, No. 9, pp. 3655-3662.
Prepublished online as a Blood First Edition Paper on January 11, 2005; DOI 10.1182/blood-2004-07-2523.

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IMMUNOBIOLOGY
Superantigen recognition by HLA class II on monocytes up-regulates toll-like receptor 4 and enhances proinflammatory responses to endotoxin
Philip A. Hopkins, John D. Fraser, Alison C. Pridmore, Hugh H. Russell, Robert C. Read, and Shiranee Sriskandan
From the Department of Infectious Diseases, Imperial College, London, United Kingdom; the Division of Molecular Biology, University of Auckland, New Zealand; and the Department of Genomic Medicine, University of Sheffield, Sheffield, United Kingdom.

   Abstract

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Abstract
Introduction
Materials and methods
Results
Discussion
References

The devastating systemic effects of bacterial superantigensmay be explained by powerful proinflammatory synergy with lipopolysaccharide(LPS). However, the mechanism underlying this phenomenon remainsunclear and has never been investigated in humans. Specifically,there is no known link between superantigen-induced immune effectsand the pattern recognition of LPS at toll-like receptor 4 (TLR4).Here we show that bacterial superantigens induce rapid transcriptionand increased membrane expression of TLR4 in primary human monocytesby ligation of major histocompatibility complex (MHC) classII. We also demonstrate that superantigens are solely responsiblefor monocyte TLR4 up-regulation induced by products from Gram-positivebacteria. In parallel with enhanced TLR4 expression, primingof purified monocytes or mixed peripheral blood mononuclearcells with superantigens significantly enhanced the inductionof proinflammatory cytokines by known TLR4 ligands. Staphylococcalenterotoxin A constructs containing targeted mutations wereused to demonstrate a requirement for MHC class II ligationin both TLR4 up-regulation and enhanced responses to endotoxin.In contrast to results from animal models, superantigen-endotoxininteraction was not dependent on T-cell receptor ligation bysuperantigen or interferon gamma production. Pattern recognitionof bacterial superantigens by MHC class II receptors may exacerbatethe proinflammatory response of monocytes to Gram-negative infectionor endotoxin by up-regulation of TLR4.

   Introduction

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Abstract
Introduction
Materials and methods
Results
Discussion
References

The most potent microbial products implicated in the pathogenesisof septic shock are Gram-positive derived superantigenic exotoxinsand Gram-negative bacterial endotoxin.¹ Both types of toxininduce comparable proinflammatory cytokines from human mononuclearcells in vitro, cause lethal shock in vivo, and have been identifiedin the bloodstream of critically ill patients.^2-8 Despite thesestriking similarities, there appears to be a quite distinctimmunology underlying the shock states induced by these 2 bacterialproducts. Bacterial superantigens ligate both T-cell receptor(TCR) and major histocompatibility complex (MHC) class II withoutantigen processing.⁹ This leads to the activation of up to 20%of all peripheral circulating T cells, determined by TCR V betarepertoire and MHC haplotype, provoking massive cytokine production.^3,10,11In contrast, endotoxin is detected by a complex macromolecularcomplex dominated by CD14, toll-like receptor 4 (TLR4) and MD2,a key accessory molecule for TLR4.^12,13 The endotoxin pattern-recognitioncomplex is present on both epithelial and endothelial surfacesin addition to leukocytes such as monocytes/macrophages, mastcells, and granulocytes.¹⁴ Ligation of TLR4 leads to activationof transcriptional control elements such as nuclear factor ${kappa}$ B(NF- ${kappa}$ B), via a well-documented signal transduction cascade, andthe induction of cytokines.^1,14,15
Despite different proinflammatory pathways, there is a widearray of literature suggesting a major interaction between Gram-positivesuperantigenic exotoxins and Gram-negative endotoxin in animalshock models, where superantigens are reported to enhance thelethality of endotoxin by between 100- and 50 000-fold.^16-19The mechanism underlying this powerful in vivo effect has notbeen fully delineated. Although some workers have suggesteda predominant role for T cells and the lymphokine interferon ${gamma}$ (IFN- ${gamma}$ ), other cells and mediators may be involved.^18,20-26Surprisingly, biologically relevant concentrations of superantigenshave never been shown to produce a comparable effect in humancells. Moreover, to our knowledge, the mechanism underlyingsuperantigen-endotoxin synergy has never been investigated inany human system.
Here, we examine the effect of biologically relevant concentrationsof staphylococcal and streptococcal superantigens on TLR4 expressionin primary human monocytes. In addition, we describe the effectof superantigen exposure on subsequent responsiveness of humanmonocytes to TLR4 ligands. We also use staphylococcal enterotoxin(SE) A constructs with targeted mutations in key binding sitesto investigate the relative dependence of superantigen-endotoxininteraction on MHC class II and TCR ligation.

   Materials and methods

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

TLR agonists, heat-killed Staphylococcus aureus
Gel-filtered Pseudomonas aeruginosa lipopolysaccharide (LPS)(serotype 10) and Escherichia coli 0111.B4 LPS (purified onan ion-exchange column to protein/DNA content < 1%) wereobtained from Sigma (Poole, United Kingdom). E coli F515 hexa-bislipid A was kindly donated by U. Zahringer (Borstel, Germany)²⁷and endotoxin-free S aureus lipoteichoic acid (LTA) was kindlydonated by T. Hartung (Konstanz, Germany).²⁸ Heat-killed S aureus(HKSA) was generated from a single colony of S aureus H380,a clinical bacteremia isolate, which was cultured overnightin RPMI 1640 tissue-culture medium supplemented with 10% fetalcalf serum (FCS; Labtech, Ringmer, United Kingdom)/2 mM L-glutamine(Gibco, Paisley, United Kingdom). After centrifugation, bacterialpellets were washed, resuspended in saline, and quantified onblood agar prior to heat killing at 70°C for 1 hour.
Purified superantigens and mutant constructs
Native toxic shock syndrome toxin-1 (TSST-1), SEA (staphylococcalendotoxin A), and SEB (staphylococcal endotoxin B) were obtainedfrom Sigma (Poole, United Kingdom); streptococcal pyrogenicexotoxin A (SPEA) was from Toxin Technology (Sarasota, FL);and recombinant streptococcal mitogenic exotoxin Z–1 (rSMEZ-1)and rSMEZ-2 were kindly donated by T. Proft (Auckland, New Zealand).Wild-type (WT) and site-directed mutant constructs of rSEA weregenerated as described previously.²⁹ SEA F47S.L48A.Y92A wasdefective in MHC class II ${alpha}$ -chain binding; SEA-H225A in ${beta}$ -chainbinding; SEA-H225A.F47S in both ${alpha}$ and ${beta}$ -chain binding; and SEA-N25A.Y94Ain TCR binding. LPS content of superantigens was below 0.1 pg/ngof toxin by Limulus assay.
Bacterial supernatants
Overnight cultures of isogenic S pyogenes strains, grown inglutamine-supplemented RPMI 1640, were centrifuged and supernatantswere filter-sterilized. Aliquots were plated onto blood agarto ascertain equivalent growth. Strains used were parent strainH293, a clinical isolate (smez⁺), H377 (smez-mutant), and H432(complemented with smez as previously described).^30,31 Supernatantswere incubated with monocytes at a dilution of 1:10 and wereendotoxin-free by Limulus assay.
Reagents
Neutralizing anti–IFN- ${gamma}$ (R&D Systems, Abingdon, UnitedKingdom) was used in the range of 0.02 µg/mL to 2 µg/mLwith appropriate isotype-matched antibody controls. Genestein,cycloheximide, and phytohemagglutinin (PHA) were obtained fromSigma. Genestein (0.037 µM-37 µM) and cycloheximide(0.36 nM-360 nM) were dissolved in dimethyl sulfoxide (DMSO)and applied in parallel with appropriate vehicle-only controls.
Monocyte, nonmonocyte, T-cell, and PBMC cultures
Peripheral blood mononuclear cells (PBMCs) were extracted fromthe whole blood of healthy volunteers (Hammersmith Hospitalethics reference: 2002/6418) by differential gradient centrifugationover endotoxin-free Ficoll-Paque Plus (Amersham Biosciences,Amersham, United Kingdom). Monocytes and positively selected`nonmonocytes' were extracted from PBMCs using Monocyte IsolationKit II (Miltenyi Biotech, Bisley, United Kingdom), accordingto the manufacturer's instructions. Briefly, PBMCs were incubatedfor 10 minutes at 4°C with biotin-conjugated anti-CD3, CD7,CD19, CD45RA, CD56, and immunoglobulin E (IgE) in phosphate-bufferedsaline (PBS) supplemented with 10% autologous human serum andFcR blocking reagent (Miltenyi Biotec). Magnetic microbeadsconjugated to anti–biotin antibody were then added andcoincubated for an additional 15 minutes. Following a PBS serumwash, the sample was passed across an LS column within a magneticfield (Midi-Macs; Miltenyi Biotech). Cells were seeded in sterileflow cytometry tubes (Becton Dickinson, Oxford, United Kingdom)or 96-well plates at a concentration of 2 x 10⁵/well or tubein RPMI 1640/FCS supplemented with 50 U/mL penicillin G and50 µg/mL streptomycin sulfate. They were incubated at37°C in 5% CO₂ for 12 hours then washed and recovered withfresh medium. For monocyte preparation, nonadherent cells wereaspirated prior to washing to further increase purity. PureT cells were similarly prepared using a pan-T selection kit(Miltenyi Biotec) by selecting with hapten-conjugated CD11b,CD16, CD19, CD36, and CD56 antibodies prior to separation withhapten-conjugated microbeads. Cell populations were double-stainedwith phycoerythrin (PE)–CD3 and fluorescein isothiocyanate(FITC)–CD14 for flow cytometric analysis. Monocyte populationscontained less than 4% CD3⁺ cells and T-cell populations containedless than 0.5% CD14⁺ cells.
Flow cytometry
Monocyte populations were exposed to tissue-culture medium (TCM),superantigens, lipid A, LPS, LTA, or heat-killed whole bacteriafor various times at 37°C in 5% CO₂. They were then washedand resuspended in 50 µL ice-cold FACS buffer (PBS/1%bovine serum albumin [BSA]) prior to dark incubation for 30minutes on ice with PE anti-TLR4 and FITC anti-CD14 mouse, orIgG1-FITC, IgG2A-PE isotype-matched controls (ITMCs). Sampleswere washed and resuspended in 400 µL FACS buffer forflow cytometric analysis (FACSCalibur; Becton Dickinson) usingappropriately single-stained samples to set compensations. Themean fluorescence intensity generated from resting or stimulatedPE-TLR4–labeled cells in CD14-gated populations (n = 20000) was measured and the difference between these groups ( ${Delta}$ MFI)was calculated for each experimental condition.
Quantitative RT-PCR
Pure monocyte cultures from 5 different donors were exposedto 1 ng/mL SEB, or tissue-culture medium alone for 3 hours,7 hours, and 24 hours. In some cases, monocytes were also incubatedwith 1 ng/mL LPS 0111:B4. Cells were lysed with Trizol reagent(Invitrogen, Paisley, United Kingdom) and total RNA isolatedaccording to the manufacturer's instructions. cDNA was preparedby priming with oligo-dT primer, and then applying ImProm-IIreverse transcriptase (Promega, Southampton, United Kingdom).For reverse transcriptase–polymerase chain reaction (RT-PCR),TaqMan probe/primer sequences were determined using Primer Expresssoftware (Applied Biosystems, Warrington, United Kingdom) andsynthesized by Biosource (Nivelles, Belgium): TLR4 (forward:5'-CTGCAATGGATCAAGGACCAG'; reverse: 5'-TGC CCT GCT TAT CTG AAGGTG-3'; probe: 5'-FAM-CAGCTCTTGGTGGAAGTTGAACGAATG G-TAMRA-3');MD2 (forward: 5'-TGAATCTTCCAAAGCGCAAA-3'; reverse 5'-TGTATTCACAGTCTCTCCCTTCAGA-3';probe: 5'-FAM-TTATTTGCCGAGGATCTGATGACGATTACTCTT-TAMRA-3'); and ${beta}$ -actin (forward: 5'-TTGCCGACAGGATGCAGAA-3'; reverse: 5'-GCCGATCCACACGGAGTACT-3';probe: 5'-FAM-TCAAGATCATTGCTCCTCCTGAGAGC-TAMRA-3'). Standardcurves were constructed using dilutions of plasmids containingthe PCR products cloned into pCR2.1 (Invitrogen). PCR was performedusing qPCR mastermix (Eurogentec, Romsey, United Kingdom) andfluorescence measurement was conducted in the ABI Prism 7900HTsequence detection system (Applied Biosystems). Threshold cyclenumbers were used to calculate target gene copy number in thesamples by relating to the standard curves. Results were normalizedagainst ${beta}$ -actin transcripts.
Cytokine quantification by ELISA
Monocytes or PBMCs were exposed to superantigen and/or LPS undervarying conditions. Supernatants were stored at -80°C, priorto measurement of cytokines by enzyme-linked immunosorbent assay(ELISA; R&D Systems). Where PBMCs were primed with nonsuperantigenstimulants (LTA or heat-killed S aureus), the latter were usedat a concentration that individually produced the same magnitudeof cytokine production as solo superantigen stimulation.
T-cell proliferation
Two-day [³H] thymidine inclusion assay was used to assess themitogenic function of wild-type SEA in comparison with mutantSEA constructs. Superantigens were added to PBMC cultures andpulsed with 1 µCi (0.037 MBq) ³H-thymidine/well (AmershamBiosciences) at 24 hours. Cells were harvested 24 hours lateronto filter paper (Micro 96 harvester; Skatron Instruments,Lier, Norway) and tritium incorporation was measured using ascintillation counter (Wallac 1205 Betaplate, Turku, Finland).All samples were run in parallel with a PHA-only control.
Statistical analysis
Statistical analyses were provided by the Statistical AdvisoryService (Imperial College, London, United Kingdom). All errorbars shown represent standard deviations from the mean. Wherestatistical tests were applied to compare groups, significancewas defined at the 5% level (P < .05).
For flow cytometry data, individual gated populations of monocytes(20 000 events) were used for each measurement. Change in meanfluorescence intensity from resting levels ( ${Delta}$ MFI) was determinedfor cells stimulated with toxin and for cells exposed only toTCM. The paired t test was used to compare ${Delta}$ MFI values betweendifferent groups.
Analysis of RNA transcript changes in response to SEB over timewas performed by repeated measures analysis of variance followingBox-Cox transformation of RNA data; SEB-stimulated cells werecompared with control cells stimulated with TCM alone.
To analyze the effect of superantigen-endotoxin combinationson induction of cytokines, mean cytokine production and standarddeviations were calculated from triplicate repeats for eachindividual donor. All experiments were performed on at least5 occasions. Observed cytokine release was compared with expectedcytokine release (derived from the sum of cytokine productioninduced by single toxin stimulation). Where groups of 8 or moreindividuals were used, a 2-step nonparametric analysis was performedto demonstrate supra-additive effects. Median values for observedcytokine production were subtracted from expected values andthe results compared with 0 using the Wilcoxon signed rank test(Figure 4A, 6A-E).

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Figure 4.. Stimulation of primary human monocytes with superantigens enhances production of TNF- ${alpha}$ in response to subsequent LPS challenge. Monocytes were exposed to 1 ng/mL SEB for 3 hours with coincubation with 1 ng/mL E coli LPS 0111:B4 for an additional 4 hours. (A) Composite box-plot to illustrate magnitude of enhanced induction of TNF- ${alpha}$ by SEB-LPS (n = 10). ^*Denotes significant difference from "expected" cytokine production, derived from the sum of TNF- ${alpha}$ produced from individual toxin stimulations; P = .002. (B) Enhancement of LPS-induced TNF- ${alpha}$ production by SEB pre-exposure is restricted to the monocyte subset. Mean and SD of data from triplicate wells are shown. Data are representative of 3 separate experiments. (C) Enhanced production of TNF- ${alpha}$ is not inhibited by neutralizing concentrations of anti–IFN- ${gamma}$ . ITMC indicates isotype-matched control antibody. Mean and SD of data from triplicate wells are shown. Results are representative of 3 separate experiments.

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Figure 6.. The enhancement of proinflammatory responses to LPS by superantigens in PBMCs is a reproducible and specific cellular phenomenon. (A-B) TNF- ${alpha}$ production by PBMCs stimulated with superantigen-endotoxin in expanded donor population. Cells were pre-exposed to 1 ng/mL superantigen (A, TSST-1, n = 21; B, SEB, n = 15) for 3 hours, then coincubated with LPS (1 ng/mL) for an additional 4 hours. Median and 10th, 25th, 75th, and 90th centiles are shown. ^*Represents significant supra-additive superantigen-endotoxin interaction; P < .001 for both superantigens. (C) IL-1 ${beta}$ and (D) IL-6 cytokine induction by SEB-LPS compared with that expected from individual toxins was also supra-additive (P = .008). Results are shown for each individual donor (D1-D8). (E) IFN- ${gamma}$ production in response to SEB-LPS was not supra-additive from that predicted by levels induced by individual toxins. (F) In comparison with control PBMCs (incubated either alone or sequentially with SEB and LPS), SEB-exposed donor PBMCs retained hyperresponsiveness to LPS even when supernatants were removed and replaced with fresh medium (bars marked "D"). Supernatants from PBMCs pre-exposed to SEB did not directly transfer priming (ie, immediate enhanced LPS responsiveness) to naive recipient PBMCs (bars marked "R"). (G) Cycloheximide (cyclo) inhibited enhanced production of TNF- ${alpha}$ by superantigen-endotoxin. Error bars reflect standard deviation of triplicate wells.

   Results

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Purified superantigens induced up-regulation of monocyte membrane TLR4 expression via ligation of MHC class II
Reproducible increases in TLR4 membrane expression were foundfollowing exposure of monocytes to purified streptococcal andstaphylococcal superantigens, even in cultures where CD3⁺ cellswere undetectable by flow cytometry (Figure 1). Superantigen-inducedshifts in mean fluorescence intensity were not observed in isotype-matchedcontrol-stained cells or in experiments where monocytes werestained with a different isotype-matched antibody, anti–TLR-1-PE.The dose-response relationship between SEB and TLR4 expressionis shown in Figure 1B. SEB consistently produced maximal TLR4up-regulation at a concentration of 1 ng/mL. TLR4 up-regulationwas reproducibly observed from 3 hours after SEB exposure andwas maximal by 16 hours. All tested superantigens induced increasedmembrane expression of TLR4 at concentrations above 10 pg/mL,maximal in magnitude at superantigen concentrations between1 ng/mL and 100 ng/mL. Importantly, up-regulation of TLR4 thereforeoccurred at toxin concentrations compatible with those thoughtto occur in vivo in the context of severe sepsis.^6-8 The reproducibilityof this effect for both staphylococcal and streptococcal superantigenswas tested in multiple healthy subjects (Figure 1C). Up-regulationof TLR4 was specific to superantigens and was not seen withLTA (0.1 µg/mL-10 µg/mL), whole, heat-killed Gram-positivebacteria (S aureus 10-10⁵ CFU [colony-forming units]/mL), orany TLR4 agonist (purified LPS from E coli and Pseudomonas spp,hexa-bis lipid A). Indeed, 100 ng/mL lipid A significantly depressedTLR4 membrane expression relative to the low levels observedon resting monocytes. The latter observation is consistent withpublished observations in murine macrophages.³²

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Figure 1.. Surface TLR4 expression in monocytes is specifically up-regulated by superantigens via MHC class II ligation. (A) Membrane TLR4 expression following incubation of purified monocytes with medium alone (resting monocytes; dotted line) or with different microbial products (stimulated monocytes; solid line). Left panel, superantigens; right panel, other microbial products. Representative flow cytometry histograms are shown at the superantigen concentrations found to induce maximal TLR4 up-regulation. Cells stained with isotype-matched control (ITMC) antibody are shown in shaded region. Other microbial products, in particular LTA and E coli LPS 0111:B4, did not support TLR4 up-regulation at any concentration tested and in some cases down-regulated TLR4 expression. (B) Dose-dependence of SEB () and LPS (E coli 0111:B4; ${circ}$ ) effects on membrane TLR4 expression relative to unstimulated cells ( ${Delta}$ MFI): mean ± SD of 4 separate donor monocyte preparations. ^*Denotes difference from TCM-only controls. (C) Membrane expression of TLR4 in monocytes from expanded donor pool stimulated with 1 ng/mL SEB (n = 35), SEA (n = 16), SMEZ-1 (n = 9), LPS (n = 12), and lipid A (n = 9). Additional results are shown for cells stimulated with 10 ng/mL LPS, 10 ng/mL lipid A, 1 µg/mL LTA, and 10⁵ cfu/mL HKSA (n = 9) Median and 10th, 25th, 75th, and 90th centiles are shown: concentrations shown are those used in subsequent cytokine induction experiments. (D) In contrast to WT SEA, MHC nonbinding mutant constructs fail to support TLR4 up-regulation. Mean and SD of 3 experiments. ^*Denotes significant difference from TCM-only controls. (E) Genestein (37 µM) inhibits SEB-induced TLR4 up-regulation. Mean and SD of 3 experiments. ^**Denotes significant difference from SEB-only TLR4 up-regulation.

Importantly, up-regulation of TLR4 by superantigen was absolutelydependent on MHC class II ligation (Figure 1D). Up-regulationof TLR4 was not supported by mutant constructs of SEA designedto prevent binding to MHC class II, or by SEB in the presenceof genestein (37 µM), an inhibitor of protein tyrosinekinase known to be important in superantigen signaling via classII³³ (Figure 1E). This concentration of genestein did not inducecell death or changes in forward- or side-scatter characteristicsin monocytes.
The up-regulation of TLR4 on monocytes induced by streptococcal supernatants is solely due to superantigen production
The biologic relevance of the above findings was underlinedby the observation that dilute sterile supernatants from a clinicalS pyogenes isolate (H293), which expresses the superantigenSMEZ, also enhanced monocyte membrane TLR4 expression (Figure 2).Moreover, disruption of the smez gene in strain H377 preventedup-regulation of TLR4 by derived bacterial supernatant. Interestingly,reconstitution of smez by plasmid complementation (strain H432)increased the capacity of supernatant to enhance TLR4 expressionbeyond that seen for the parent strain. This is likely to bedue to the presence of 2 to 3 copies of smez in the complementedstrain.³¹

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Figure 2.. Up-regulation of TLR4 in monocytes by S pyogenes supernatants is solely due to superantigens. Dilute (1/10) supernatant from a superantigen-producing strain of S pyogenes (H293) up-regulates TLR4 on human monocytes. Disruption of smez gene (strain H377) abrogates TLR4 up-regulation. Complementation with smez (strain H432) restores TLR4 up-regulation beyond that of wild-type (WT). ^*Denotes significant difference from H293 parent strain. Mean and SD of triplicate monocyte cultures; results are representative of separate experiments in 3 different individuals.

TLR4 up-regulation was not observed using supernatant from nonsuperantigenproducing streptococci (S viridans, S pneumoniae) and, as withpurified TLR4 ligands, TLR4 expression was down-regulated bysupernatant from Gram-negative bacteria (P.A.H., unpublishedobservations, February 2004).
Superantigens induced up-regulation of TLR4 and MD2 mRNA in human monocytes
In comparison to control cells, primary human monocytes stimulatedwith 1 ng/mL SEB demonstrated significant up-regulation of TLR4transcription over the time course studied, which was maximalat 7 hours and diminished by 24 hours (Figure 3A). Interestingly,we found a parallel up-regulation of MD2 transcription by SEB(Figure 3B). Endotoxin had no apparent effect on TLR4 and MD2gene transcription relative to that seen in resting monocytes.

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Figure 3.. TLR4 and MD2 mRNA transcripts are up-regulated in purified primary human monocytes by SEB. Quantities of TLR4 (A) and MD2 (B) mRNA were corrected relative to the constitutively produced ${beta}$ -actin gene product. Individual results are shown for SEB-stimulated () or TCM-only exposed ( ${circ}$ ) monocytes from 5 donors at 3 hours, 7 hours, and 24 hours. The difference in TLR4 and MD2 expression in SEB- and TCM-stimulated cells was significant (repeated measures analysis of variance, P < .05). The result was representative of 2 independent experiments.

Superantigens enhance LPS-induced human monocyte TNF- ${alpha}$ production
The biologic consequence of TLR4 up-regulation at the levelof both transcription and membrane expression was tested bythe sequential stimulation of monocytes with SEB (1 ng/mL) followedby exposure to the TLR4 agonist E coli LPS 0111:B4 (1 ng/mL).Monocytes were exposed to SEB for 3 hours and then coincubatedwith LPS for an additional 4 hours (total superantigen exposure:7 hours). The amount of tumor necrosis factor (TNF)– ${alpha}$ producedfrom sequential stimulation of purified monocytes with superantigen-LPSgreatly exceeded any additive effects (Figure 4A). Enhancedproduction of TNF- ${alpha}$ was seen only from monocytes, and was notobserved from positively selected nonmonocytes or negativelyselected purified T cells, which were stimulated sequentiallywith SEB and LPS in parallel (Figure 4B). Neutralizing anti–IFN- ${gamma}$ (2.0 µg/mL) did not impair enhancement of TNF- ${alpha}$ productionfrom purified monocytes exposed sequentially to SEB and LPS(Figure 4C). This concentration of anti–IFN- ${gamma}$ is saturating(manufacturer's data) and blocked HLA class II up-regulationby exogenous IFN- ${gamma}$ (5 ng/mL). In contrast to murine shock models,the current data suggest that a proinflammatory interactionbetween superantigen and endotoxin can occur without the presenceof T cells or IFN- ${gamma}$ .
Pre-exposure to superantigens specifically enhances TLR4 ligand–induced human PBMC TNF- ${alpha}$ production
In order to further characterize the interaction of superantigenand LPS observed in primary monocytes in a more biologicallyrelevant setting and assess the interaction in more detail,experiments were performed using primary human PBMCs. Preliminarytitration experiments using superantigen-E coli LPS 0111:B4stimulation were used to define the optimal toxin concentrationsfor maximal induction of TNF- ${alpha}$ production by PBMCs stimulatedsequentially by both toxin types (Figure 5A). SEB concentrationsbetween 100 pg/mL and 1 ng/mL were optimal for enhancing subsequentresponses to LPS; the effect was not observed at SEB concentrationsbelow 10 pg/mL. To define the temporal relationship betweenthe 2 toxin types that was necessary for interaction, the durationof pre-exposure to superantigen was varied (Figure 5B). To determinethe rapidity of TNF- ${alpha}$ release following LPS exposure by superantigen-primedPBMCs, the duration of exposure to LPS was varied (Figure 5C).Superantigen priming of PBMCs for a minimum of 3 hours followedby coincubation with LPS for an additional 4 hours consistentlyenhanced TNF- ${alpha}$ production compared with either toxin alone. Furtherextension of superantigen priming interval or the period ofexposure to LPS did not further increase TNF- ${alpha}$ compared withthat resulting from stimulation with the individual toxins.Reversal of toxin addition led to complete loss of enhancedcytokine induction (Figure 5D). Proinflammatory priming wassupported by all other superantigens tested (TSST-1, SEA, SPEA,SMEZ-1, SMEZ-2) at similar optimal concentrations (not shown).HKSA and LTA were unable to prime PBMCs to respond to LPS tothe extent shown by superantigens. While proinflammatory superantigen-LPSinteractions were observed over a range of superantigen concentrations,any apparent interactions between LTA-LPS or HKSA-LPS were lowin magnitude and restricted to single priming stimulant concentrations.(Figure 5E-F). With regard to specificity of the secondary stimulus,other TLR4 ligands tested were able to act as secondary stimuli(LPS from Pseudomonas spp and lipid A) and produced enhancedlevels of TNF- ${alpha}$ in superantigen-primed PBMCs (Figure 5G-H). LTAand superantigens could not act as secondary stimuli and didnot induce enhanced levels of TNF- ${alpha}$ from superantigen-primedmonocytes (not shown). Hence, the priming effect of superantigensmay have specificity for TLR4 ligands.

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Figure 5.. Sequential PBMC stimulation by superantigen-LPS enhances TNF production. (A) Three-dimensional dose-response bar chart showing mean TNF- ${alpha}$ by SEB-LPS sequentially stimulated PBMCs from 3 different subjects. Means were derived from triplicate observations at each toxin concentration. Data were representative for those obtained for TSST-1 and SMEZ-1. (B) LPS-induced TNF- ${alpha}$ release by PBMCs: effect of duration of SEB pre-exposure. Enhanced TNF- ${alpha}$ production required a minimum period of 3 hours of pre-exposure to SEB. (C) LPS-induced TNF- ${alpha}$ release by PBMCs following 3 hours of pre-exposure to TSST-1: effect of duration of LPS exposure. Enhanced TNF- ${alpha}$ production was maximal 4 hours after LPS stimulation. (D) Reversal in order of exposure (LPS-SEB instead of SEB-LPS) did not produce enhanced observed levels of TNF- ${alpha}$ when compared with expected levels. (E-F) HKSA and LTA were unable to prime PBMCs for enhancement of LPS-induced TNF- ${alpha}$ production. (G) Enhanced TNF- ${alpha}$ production was also seen when TSST-1–primed PBMCs were exposed to lipid A as a secondary stimulant or (H) LPS from Pseudomonas aeruginosa (PSA LPS; threshold concentration one log higher than for E coli LPS or lipid A). All results are mean and SD of triplicate stimulations. Results are representative of 5 separate experiments and were repeated with both TSST-1 and SEB.

The enhancement of PBMC cytokine responses to TLR4 ligands by superantigens is reproducible and extends to IL-1 ${beta}$ and IL-6, though not IFN- ${gamma}$
Using a sequential stimulation approach (superantigen for 3hours followed by coincubation with LPS for an additional 4hours) the proinflammatory interaction between SEB or TSST-1and LPS was then examined in an expanded number of PBMC donors,to ascertain variablility. Data are shown for superantigen andLPS concentrations of 1 ng/mL although similar distributionwas also seen for both superantigens at 100 pg/mL (Figure 6A-B).
Interestingly, although significantly enhanced quantities ofIL-6 and IL-1 ${beta}$ were also produced by PBMCs exposed sequentiallyto superantigen-LPS, enhancement of IFN- ${gamma}$ production was notseen when the 2 types of toxin were added sequentially (Figure 6C-E).Removal of supernatant from superantigen-primed donorPBMCs and replacement with fresh medium did not impair subsequentenhancement of TNF- ${alpha}$ responses to LPS, showing that continuingpresence of superantigen or soluble factors, such as CD14, inmedium were not essential for the enhancement of TNF- ${alpha}$ productionby superantigen. This was further confirmed by the failure oftransferred primed supernatants to increase responsiveness ofnaive recipient PBMCs to LPS (Figure 6F). Taken together, thesedata suggested that the priming effect of superantigen was cell-associatedrather than secreted. The inhibition of superantigen primingeffects by cycloheximide confirmed a requirement for proteinsynthesis, and excluded effects due to the release of TNF- ${alpha}$ froma preformed pool of cytokine (Figure 6G).
Superantigens enhance the early TNF- ${alpha}$ response of human PBMCs to TLR4 ligands independent of TCR ligation or IFN- ${gamma}$ production
rSEA mutant constructs with impaired MHC class II receptor bindingcapacity were unable to support priming of PBMCs for LPS response,consistent with the data pertaining to TLR4 up-regulation. Incontrast, however, SEA-N25A.Y94A, with impaired TCR binding(and mitogenic potential), was shown to retain full primingpotential for subsequent LPS stimulation (Figure 7A-B). In addition,as in pure monocyte cultures, anti–IFN- ${gamma}$ failed to disruptsuperantigen-endotoxin proinflammatory cooperation (Figure 7C).

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Figure 7.. The enhancement of proinflammatory responses to LPS by superantigens in PBMCs is not dependent on superantigen ligation of TCR or IFN- ${gamma}$ production. (A) Enhancement of LPS-induced TNF- ${alpha}$ production was supported by TCR nonbinding but not MHC class II nonbinding SEA constructs. Cells were exposed to SEA constructs (1 ng/mL) for 3 hours, then coincubated with LPS (1 ng/mL) for an additional 4 hours. Mean and SD of triplicate stimulations are shown and data are representative of 5 experiments. (B) T-cell mitogenic potential of SEA WT versus mutant constructs was confirmed in 3 donors. (C) Anti–IFN- ${gamma}$ did not inhibit enhanced production of TNF- ${alpha}$ by PBMCs following superantigen-LPS exposure. ITMC indicates isotype-matched control antibody. Mean and SD of triplicate samples are shown; data are representative of 5 separate experiments.

   Discussion

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Abstract
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Materials and methods
Results
Discussion
References

Bacterial superantigenic exotoxins, derived predominantly fromS pyogenes or S aureus, can provoke severe hemodynamic shockand multiorgan failure.^1,3,11 The devastating pathophysiologyunderlying these conditions is thought to result from the abilityof these microbial products to cross-link T-cell receptors andMHC class II without undergoing conventional antigen processing.⁹This provokes a massive polyclonal T-cell expansion with theconsequent release of harmful proinflammatory cytokines.³ However,this immunologic phenomenon may not provide the sole explanationfor the potency of these toxins. First, superantigens can inducepowerful immune effects in the host without a requirement forT-cell proliferation.^22-26 Second, their capacity to induceproinflammatory injury can be greatly enhanced by Gram-negativebacterial endotoxin.^16-19,34 The interaction of endotoxin withsuperantigens has been shown to be highly significant in severalanimal models. However, the mechanism for this powerful effectremains uncertain and has not been studied in a human system.
Using primary human monocytes we have demonstrated that superantigenscan reproducibly enhance the membrane expression of TLR4, apivotal component in mammalian recognition of endotoxin. Weshowed that this effect is optimal at biologically relevantconcentrations of superantigen and that it is absolutely dependenton ligation of MHC class II. The up-regulation of TLR4 was specificto superantigens and did not occur with LTA, another immunologicallyactive Gram-positive product or whole, heat-killed bacteria.We used genetic disruption or complementation of the superantigengene smez to show that the ability of certain Gram-positivebacteria to induce increased expression of TLR4 was solely dueto the presence of superantigens. Although increased expressionof TLR4 has been reported in monocytes exposed to cytokines³⁵and in epithelial cells exposed to respiratory syncytial virus,³⁶this is the first demonstration of TLR4 up-regulation by anybacterial product.
In addition to increasing membrane expression of TLR4, superantigenswere also observed to induce significant and rapid TLR4 transcriptionin monocytes (in excess of 50-fold over resting levels in somesubjects). This finding is also novel. Although superantigensare known to induce important effects on transcription of cytokinessuch as TNF-alpha,^33,37,38 they have not previously been reportedto influence genes encoding toll-like receptors. Interestingly,we were also able to show a parallel increase in superantigen-inducedMD2 transcription. MD2 is now known to be a critical accessorymolecule for the function of TLR4 in endotoxin recognition.¹³
Critically, by describing superantigen-mediated amplificationof monocyte responses to TLR4 ligands, we were also able todemonstrate a clear proinflammatory phenotype for cells thatdemonstrate superantigen-mediated up-regulation of TLR4. Thisis the first report to describe proinflammatory superantigen-endotoxininteractions in human monocytes using concentrations of superantigenfound in sepsis. The presence of enhanced endotoxin responsivenessin monocytes primed with superantigen was unexpected, sinceanimal studies have delineated a key role for T cells in thisphenomenon.^18,20,21 Superantigen-endotoxin proinflammatory interactionswere therefore further investigated in human mixed PBMC cultureswhere SEA mutant constructs could be used to compare the relativecontribution of superantigen ligation by MHC class II or TCRto the priming effect. In addition, the larger sample sizesavailable in PBMC experiments also enabled better definitionand quantification of superantigen-endotoxin proinflammatorycooperation.
The sequential stimulation of PBMCs with superantigen-endotoxinagain induced early- and high-magnitude induction of proinflammatorycytokines when compared with that produced by stimulation withindividual toxins. This multiplicative effect was significantover a range of toxin concentrations. Interestingly, while greatlyenhanced levels of TNF- ${alpha}$ , IL-6, and IL-1 ${beta}$ were found followingsuperantigen-endotoxin addition, this was not true for IFN- ${gamma}$ .Although the optimal superantigen priming interval precededmaximal superantigen TLR4 membrane expression, it correlatedwell with the rapid rise in TLR4/MD2 transcription and the timepoint at which detectable up-regulation of TLR4 at the cellsurface occurred. There may also be important functional enhancementof the TLR4 signaling pathway ahead of maximal TLR4 membraneexpression as detectable by flow cytometry.
In addition to their failure to up-regulate TLR4, MHC classII nonbinding SEA constructs were also unable to enhance subsequentPBMC responses to endotoxin. It was therefore interesting tonote that superantigens known to cross-link MHC class II (suchas SEA)^29,38 were not the most potent with respect to eitherTLR4 up-regulation or amplification of cytokine induction. Importantly,not only was proinflammatory priming invoked in full by theTCR nonbinding SEA construct, but it also could not be disruptedby saturating concentrations of anti–IFN- ${gamma}$ . Taken together,these data confirmed that superantigen-endotoxin proinflammatorycooperation in this system occurs independent of any interactionwith T cells, and raises the possibility that monocytes mayconstitute a major early host responder cell in Gram-positivetoxic shock.
We considered the possibility that trace amounts of endotoxinpresent in superantigen preparations might account for TLR4up-regulation or for interactions with secondary LPS challenge.However, this possibility was discounted because exogenous endotoxinand mutant constructs of superantigens were unable to reproduceTLR4 up-regulation or priming of mononuclear cells. Furthermore,superantigen-containing bacterial supernatants were able tosupport TLR4 up-regulation despite being LPS-free.
The induction of significant TLR4 up-regulation and proinflammatorypriming in monocytes by low concentrations of superantigen (100pg/mL), raises the possibility that reported synergy betweenother Gram-positive microbial products and endotoxin could bemediated by contaminating superantigens. The suggestion thatendotoxin may be important in the pathogenesis of Gram-positivetoxic shock may also have important clinical relevance. Thisis because the systemic circulation of critically ill patientsmay be vulnerable to concurrent assault from both endotoxinand superantigens. Not only may both toxins be released duringepisodes of polymicrobial sepsis,⁷ but translocation of endotoxinmay occur during Gram-positive sepsis where there is injuryto the gastrointestinal tract or ventilated lung.^5,39-41 Conversely,acquisition of nosocomial infection with superantigen-producingbacteria (such as S aureus) could adversely affect outcomesin patients with severe sepsis due to Gram-negative organisms,particularly if plasma levels of superantigen in excess of theapparent threshold (10 pg/mL-100 pg/mL) are reached. Intriguingly,the results from our study may offer an explanation for theobservation that TLR4 is up-regulated in critically ill patientswith Gram-positive sepsis (predominantly S aureus).⁴² Our observationsmay also explain apparent discrepancies between the presenceof circulating superantigens and severity of illness.^6,7 Anabsence of systemic endotoxin in some patients may blunt hostinjury due to superantigens.
In summary, we have demonstrated that by signaling through MHCclass II, Gram-positive bacterial superantigenic exotoxins canup-regulate the transcription and membrane expression of TLR4in human monocytes. These events are associated with a markedenhancement of proinflammatory cytokine production when superantigen-primedmonocytes are stimulated with TLR4 ligands. Importantly, T cellswere not necessary for the superantigen-endotoxin interactionsobserved in this system. Taken together, our observations suggestthat general pattern recognition of superantigens from S aureusand S pyogenes by monocyte MHC class II can enhance endotoxinsensing and signal transduction and offer a novel and mechanisticexplanation for the rapid and devastating effects that smallquantities of bacterial superantigens provoke when releasedinto the systemic circulation. This provides a further exampleof important cross-talk between Gram-positive and Gram-negativebacterial products and raises the possibility that endotoxintranslocation in critically ill patients may be highly detrimentalin the context of concurrent Gram-positive infection.

   Acknowledgements

We thank Dr Lee Faulkner (Gram Positive Molecular PathogenesisGroup, Imperial College, London) for advice and technical assistance.We also thank Dr Elena Kulinskaya and Dr Fabiana Gordon (StatisticalAdvisory Service, Imperial College, London) for advice regardingdata analysis.

   Footnotes

Submitted June 2, 2004; accepted January 5, 2005.
Prepublished online as Blood First Edition Paper, January 11,2005; DOI 10.1182/blood-2004-07-2523.

Supported by an MRC Clinical Training Fellowship (P.A.H.), agrant from the Intensive Care Society (P.A.H.), and the SheffieldTeaching Hospitals Charitable Trust (A.C.P.).

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 U.S.C. section 1734.

Reprints: Shiranee Sriskandan, Department of Infectious Diseases, Imperial College, Du Cane Rd, London W12 0NN; e-mail: s.sriskandan{at}imperial.ac.uk.

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