Epstein-Barr virus nuclear antigen 2 induces interleukin-18 receptor expression in B cells

doi:10.1182/blood-2004-08-3196

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Blood, 15 February 2005, Vol. 105, No. 4, pp. 1632-1639.
Prepublished online as a Blood First Edition Paper on October 21, 2004; DOI 10.1182/blood-2004-08-3196.

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IMMUNOBIOLOGY
Epstein-Barr virus nuclear antigen 2 induces interleukin-18 receptor expression in B cells
Franck Pagès, Jérôme Galon, Galina Karaschuk, Diana Dudziak, Mathieu Camus, Vladimir Lazar, Sophie Camilleri-Broët, Christine Lagorce-Pagès, Sophie Lebel-Binay, Gerhard Laux, Wolf-Herman Fridman, and Berthold Henglein
From Institut National de la Santé et de la Recherche Médicale (INSERM) U 255, Centre de Recherches Biomédicales des Cordeliers, Paris, France; Hôpital Européen Georges Pompidou, AP-HP, Service d'Immunologie Biologique, Paris, France; GSF-Forschungszentrum für Umwelt und Gesundheit, Institut für Klinische Molekularbiologie und Tumorgenetik, München, Germany; Institut Gustave Roussy, Unité de Génomique Fonctionnelle, Villejuif, France; Hôpital Hôtel-Dieu, AP-HP, Service d'Anatomie Pathologique, Paris, France; Hôpital Avicenne, AP-HP, Service d'Anatomie Pathologique, Bobigny, France; and Centre National de la Recherche Scientifique (CNRS) Unité Mixté de Recherche (UMR) 7098, Université Pierre et Marie Curie, Paris, France

   Abstract

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Epstein-Barr virus (EBV) latently infects and immortalizes Blymphocytes and causes lymphoproliferative malignancies. Weshow here that the EBV nuclear antigen EBNA2 induces expressionof the 2 chains of the interleukin-18 receptor (IL-18R) in Burkittlymphoma (BL) cell lines and in nontransformed B cells. Activationof IL-18R expression by EBNA2 is independent of its interactionwith the transcriptional repressor RBPJ ${kappa}$ . It occurs in the absenceof any other viral protein but requires de novo synthesis ofcellular proteins. IL-18R induction is a highly specific functionof EBNA2, because neither other EBV latent proteins nor thecellular proteins c-myc or Notch can exert this effect. UsingcDNA microarray expression profiling, we find that the IL-18receptor expressed in EBV-infected BL cells has signaling capacity,because IL-18 significantly modified gene expression. We reportthat EBNA2 expression is associated with IL-18R expression invivo in EBV-positive B-lymphomas from AIDS patients. (Blood.2005;105:1632-1639)

   Introduction

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Epstein-Barr virus (EBV) is a ubiquitous human lymphotropic ${gamma}$ herpesvirus that latently infects and immortalizes B cellsand persists lifelong in resting memory B cells. Ultimately,latent EBV infection can lead to the development of Burkittlymphoma (BL), nasopharyngeal carcinoma, Hodgkin disease, posttransplantationlymphoproliferative disease, and immunoblastic lymphoma in immunocompromisedpatients (reviewed by Young and Murray¹).
B cells latently infected with EBV express variable subsetsof the EBV latency genes, which code for the nuclear antigensEBNA1, EBNA2, EBNA3A, EBNA3B, EBNA3C, and EBNA-LP and the membraneproteins LMP1 (latent membrane protein-1), LMP2A (or TP1), andLMP2B (or TP2). Freshly infected naive B cells and in vitro-transformedlymphoblastoid cell lines express the full set of latency genes,while their expression may be restricted to EBNA1 alone in BL(reviewed by Young et al²). Uncontrolled proliferation of EBV-immortalizedB cells in vivo is prevented by strong primary and memory CD8⁺cytotoxic T lymphocyte (CTL) responses directed essentiallytoward HLA allele-specific epitopes from the latent proteinsEBNA3A, EBNA3B, and EBNA3C.^3,4 Virus-bearing memory B cellsor B-cell tumors escape immune surveillance by down-regulationof immunogenic latent proteins, particularly EBNA2, which activatestranscription of the EBNA3 genes.
EBV latent proteins induce the synthesis of surface and solubleproteins, which can interfere with the host's immune response.Thus, EBV infection activates expression of the receptors CD21,⁵CD23,⁶ CD25,⁷ Fas ligand,⁸ and BLR2/CCR7⁹ and the cytokinestumor necrosis factor- ${alpha}$ (TNF- ${alpha}$ ),¹⁰ lymphotoxin ${alpha}$ (LT- ${alpha}$ ),¹¹ granulocytecolony-stimulating factor (G-CSF),¹⁰ interferon- ${beta}$ (IFN- ${beta}$ ),¹² interleukin-6(IL-6),¹³ IL-8,¹⁴ IL-10,¹⁵ and IL-12.¹⁶ The cytokine IL-18 ismainly produced by activated macrophages and dendritic cells;it has multiple functions in the regulation of innate and adaptiveimmune responses¹⁷ and has antitumoral^18,19 and antiviral²⁰properties.
IL-18 binds to the cell through a specific receptor, IL-18R,belonging to the Toll-like receptor family.²¹ It is composedof IL-18R ${alpha}$ ,²² which binds IL-18 with low affinity,²³ and IL-18R ${beta}$ ,which does not bind IL-18 but together with IL-18R ${alpha}$ forms thehigh-affinity IL-18 receptor and mediates signaling²⁴ throughpathways shared with the IL-1 receptor. IL-18R is expressedon a variety of cell types, including T cells, natural killer(NK) cells, and peripheral CD19⁺ B cells.²⁵ Freshly isolatedhuman tonsillar B cells, however, do not express IL-18R.^26,27
IL-18 was found to participate in host reactions to EBV-infectedcells. Significant amounts of IL-18 are detected in lymphoidtissues during EBV-induced infectious mononucleosis.²⁸ In athymicmice, murine IL-18 accumulates in experimental tumors of EBV-positiveBL cells and may contribute to their rejection.²⁹ The availabilityof IL-18 in the environment of EBV-infected cells raised thequestion of whether these cells express the IL-18 receptor andmight thus respond to IL-18. It has indeed been found recentlythat IL-18R ${alpha}$ was strongly expressed in some EBV-transformed celllines but absent in a series of EBV-negative B-cell tumors.²⁵These observations prompted us to investigate whether EBV infectioncould lead to expression of a functional IL-18R in B cells.We report that the latent EBV protein, EBNA2, drives IL-18Rexpression, allowing the infected cell to respond to IL-18.

   Materials and methods

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Cell lines
The EBV-negative BL cell lines DG75, BL2, BL30, BL31, BL41,and BL70 and their in vitro-infected counterparts with the EBVstrains P3HR-1 (P3) or B95-8 (B95), BL2-P3, BL41-P3, BL2-B95,BL30-B95, BL31-B95, BL41-B95, and BL70-B95 were a gift fromG. Lenoir and have been described previously.^30-33 Conditionallyimmortalized EREB2-5 cells, which proliferate as a lymphoblastoidcell line in the presence of estrogen, were obtained from B.Kempkes.³⁴ The cell lines P493-6,³³ LMPtet EREB,³⁵ and 1414³⁶were established by stable transfection of EREB2-5 cells withtetracycline-controlled expression plasmids for c-myc, LMP1,and the intracellular domain of Notch1, respectively. The myelomonocyticcell line KG-1 was purchased from the American Type CultureCollection (Manassas, VA).
Cells were cultured in RPMI 1640 medium (Gibco, Gaithersburg,MD) supplemented with 10% fetal calf serum (Gibco), 2 mM L-glutamine,100 U/mL penicillin, and 100 mg/mL streptomycin. For inductionof estrogen receptor (ER) chimeras, ${beta}$ -estradiol (estrogen) wasadded to the culture medium at 1 µM. For repression oftetracycline-controlled transgenes, the medium was supplementedwith 0.1 µg/mL tetracycline.
Transfection and plasmids
Cells were transfected by electroporation (240 to 280 V, 975µF). Expression plasmids coding for the EBV latent proteinsEBNA2 and LMP1 were obtained from A. Sergeant and W. Hammerschmidt,respectively. pPDL152, an expression plasmid coding for theRBPJ ${kappa}$ -binding deficient mutant WW323SR of EBNA2,³⁷ was obtainedfrom S. D. Hayward.
Luciferase assays were performed as described.³⁸ The nuclearfactor- ${kappa}$ B (NF- ${kappa}$ B) reporter plasmids Ig ${kappa}$ 3-ConA-Luc³⁹ and p(IL6 ${kappa}$ B)3-50hu.luc⁴⁰were obtained from A. Israel and G. Haegeman, respectively.A luciferase reporter construct for the human IFN- ${gamma}$ promoter⁴¹was obtained from K. Barbulescu. The previously described reporterplasmid Ga981-16 contains 12 tandemly repeated RBPJ ${kappa}$ bindingsites from the viral TP1 promoter.⁴² Complementary DNA (cDNA)coding for the human IL-18 receptor alpha chain (IL-18R ${alpha}$ ) wasobtained from J. E. Sims.²²
Immunofluorescence and flow cytometry
For detection of IL-18R ${alpha}$ , cells were reacted with mouse monoclonalantibody MAB840 (R&D Systems, Minneapolis, MN), followedby a secondary fluorescein isothiocyanate (FITC)-labeled antibodyor by the phycoerythrin (PE)-labeled mouse monoclonal antibodyFAB840P (R&D Systems), according to the manufacturer's recommendations.IL-18R ${beta}$ was detected by incubation with goat polyclonal antibodyAF118 (R&D Systems), followed by biotinylated antibodiesto goat immunoglobulin G (IgG) and streptavidin coupled to FITC.Staining was visualized by fluorescence microscopy using a ZeissAxiovert 405 microscope equipped with an Achroplan 20 x/0.45objective lens (Carl Zeiss, Oberkochen, Germany) and a HamamatsuC5810 camera (Hamamatsu, Hamamatsu City, Japan). Images wereprocessed with Adobe Photoshop 4.0 software (Adobe, San Jose,CA). For Figure 4 acquisition, we used a Leica DMR microscopeequipped with HCPL Fluotar 20 x/0.5 and Apo oil 63 x/1.32 objectivelenses (Leica, Heidelberg, Germany) and a KAPPA PS30C camera;images were processed with KAPPA ImageBase Control 2.5 software(KAPPA, Gleichen, Germany). Flow cytometry was performed usinga FACScan instrument (Becton Dickinson, San Jose, CA) with CellQuestacquisition software.
Northern blots and polymerase chain reaction
Northern blotting was performed according to standard procedures.The radiolabeled cDNA for human IL-18R ${alpha}$ was used as a probe.
RT-PCR for IL-18R ${alpha}$ , IL-18R ${beta}$ , and HPRT was as follows: RNA wasisolated using the RNeasy Kit (Qiagen, Valencia, CA) and treatedwith RNAse-free DNase I. Reverse transcriptase-polymerase chainreaction (RT-PCR) was performed using 1 µg total cellularRNA incubated with avian myeloblastosis virus (AMV) reversetranscriptase, primer oligo(dT), deoxyribonucleoside triphosphate(dNTP), and RNase inhibitor for 1 hour at 42°C (cDNA synthesiskit; Boehringer Mannheim Biochemica, Indianapolis, IN). PCRamplification was performed as previously described.¹⁹ The senseand antisense primers, respectively, and the size of the PCRproducts were as follows: IL-18R ${alpha}$ , 5'-TTGGAGTGATGACAGGAACAC-3',5'-CATCAGATAGGTCGTTACTACTACC-3', 223 bp; IL-18R ${beta}$ , 5'-GGTTATTACTCCTGCGTGC-3',5'-CCATTTTCTTCCCCGAACATCC-3', 273 bp; and hypoxanthine phosphoribosyltransferase(HPRT), 5'-TTCAAATCCAACAAAGTCTG-3', 5'-AGCACTGAATAGAAATAGTGATAGA-3',278 bp.
Immunohistochemistry: case selection
Tissue specimens from patients with cerebral diffuse large B-celllymphomas (n = 6) were obtained from J. J. Hauw, Departmentof Neuropathology, CHU Pitie-Salpetrière, Paris, France,and 7 cases of systemic large B-cell lymphoma from the Departmentof Pathology, Hôtel-Dieu, Paris. Patient samples wereobtained from the pathologists after completion of the diagnosticprocedures. Large B-cell lymphomas were diagnosed on the basisof clinical and characteristic histologic features and wereclassified according to the Revised European-American Lymphomaclassification.⁴³ Pertinent selected information on each tissuesample is given in Figure 4.
The avidin-biotin-peroxidase method was performed on frozensections using the LSAB⁺ peroxidase kit (Dako, Glostrup, Denmark).Briefly, tissue sections were deparaffinized, subjected to microwavetreatment (3 times for 5 minutes), and then incubated in hydrogenperoxide for 15 minutes and blocked with bovine serum albuminfor 30 minutes before incubation with the primary antibodies.The complex was visualized with diaminobenzidine, and the nucleiwere counterstained with hematoxylin. Anti-IL-18R monoclonalIgG1 (R&D Systems) was used at a final concentration of0.25 µg/mL, and anti-EBNA2 monoclonal IgG1 (Dako) wasused at a final concentration of 32 µg/mL. Irrelevantmurine IgG1 was used at the same final concentrations as negativecontrols. EBV was detected by in situ hybridization of paraffinsections using an FITC-labeled oligonucleotide complementaryto EBV-encoded RNA1 (EBER1) (Dakopatts, Glostrup, Denmark).⁴⁴
Complementary DNA microarrays
BL2-B95 cells (1 x 10⁷) were kept in serum-free medium for 24hours. Incubation was continued for 24 hours in the presenceof 100 ng/mL IL-18 or bovine serum albumin (BSA). RNA was extractedusing RNAgents (Promega, Madison, WI). Complemenatary DNA madefrom 10 µg RNA from each sample and from reference RNA(R) (Clontech, Palo Alto, CA) was labeled with deoxycytidinetriphosphate (dCTP) dyes cyanine-3 and cyanine-5 (Perkin Elmer,Norwalk, CT), respectively, according to the instructions ofAgilent Technologies (Palo Alto, CA). Sample cDNAs were mixedwith reference cDNA and hybridized for 16 hours to the Human1 cDNA Microarray (Agilent Technologies) containing 12814 uniqueclones from the clone sets Incyte Unigen 1 and Human Drug TargetDNA (Incyte Genomics, St Louis, MO). The reproducibility hasbeen evaluated for these microarrays by the manufacturer (interarraystandard deviation of log ratios less than 0.1 for 24 arrays).All microarray hybridizations are assessed for labeling, hybridizationefficiency, and sensitivity using specially designed controlelements that are added to each labeling reaction (for details,see Galon et al⁴⁵). The detection limit (sensitivity) of themicroarrays is such that control targets added to the hybridizationreaction are easily detected over background at a concentrationof 3.0 copies per cell per million cells. The microarrays werescanned on a dynamic autofocus microarray scanner (Agilent Technologies).Feature Extraction Software (Agilent Technologies) was usedto extract data information and to perform statistical analysisof signals. The intensity of the fluorescence at each arrayelement was proportional to the expression level of that genein the sample. The ratio of the 2 fluorescence intensities provideda quantitative measurement of the relative gene expression levelin the 2 samples. The statistical significance of the correlationbetween 2 DNA microarray experiments was determined using correlationmatrix algorithm, Kendall correlation algorithm, and Spearmancorrelation algorithm. Similar results were found with all algorithms.When no fluorescent signal was detected (signal intensity =intensity of local background + SD local background) in oneor both experiments, the corresponding gene was removed fromthe statistical analysis. Correlation analyses were performedby plotting differential gene expression of one experiment againstthe value from the other experiment. The correlation coefficient(r) and the statistical significance (P) were determined. Levelsof expression after IL-18 treatment were compared with thoseof BSA-treated cells. Data are presented as mean ± SDand were analyzed by analysis of variance (ANOVA) t test foreach gene.

   Results

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Abstract
Introduction
Materials and methods
Results
Discussion
References

EBNA2 induces expression of IL-18R ${alpha}$ in the absence of other EBV genes
To study whether latent infection of BL cells by EBV could leadto IL-18R ${alpha}$ expression, we analyzed a series of EBV-negative BLcell lines and their in vitro EBV-converted counterparts. RT-PCRusing total RNA from the EBV-negative BL cell lines DG75, BL2,BL30, BL31, BL41, and BL70 demonstrated the absence of transcriptsspecific for IL-18R ${alpha}$ . In contrast, the cell lines BL2, BL30,BL31, BL41, and BL70 accumulated IL-18R ${alpha}$ RNA after conversionwith the wild-type EBV-strain B95-8 (Figure 1A and data notshown). Surface expression of the receptor was readily detectedin these cells by flow cytometry (Figure 1B). The mean fluorescenceintensity was comparable to that observed with the KG-1 cellline derived from an acute myeloblastic leukemia, which hasbeen shown to strongly express IL-18R ${alpha}$ .⁴⁶ Conversion with theEBNA2-deficient, nontransforming EBV strain P3HR1, however,did not induce IL-18R ${alpha}$ expression (Figure 1A). These resultsindicate that in vitro infection of BL cells with wild-typeEBV leads to expression of IL-18R ${alpha}$ and suggest that this processdepends on EBNA2 expression. To identify the EBV latent proteinsinvolved in induction of IL-18R ${alpha}$ expression, we transfected theEBV-negative BL cell lines BL2 and BL41 and their P3HR1 convertantswith expression plasmids for EBNA2 or LMP1 or an empty controlvector. Proper expression from the EBNA2 and LMP1 coding plasmidswas monitored by transactivation of the cotransfected reportergenes Ga981-16 and Ig ${kappa}$ 3-ConA-Luc, respectively ("Materials andmethods" and data not shown). Forty-eight hours after transfection,we analyzed the cells for the presence of IL-18R ${alpha}$ mRNA (Figure 1C)and protein (Figure 1D and data not shown). While EBNA2transfectants expressed IL-18R ${alpha}$ , IL-18R ${alpha}$ expression was undetectablein LMP1 and control transfectants. These observations implythat EBNA2 can induce IL-18R ${alpha}$ in the absence of other viral proteinsand that overexpression of LMP1, even in combination with thelatent proteins EBNA1, EBNA3A, EBNA3B, and EBNA3C, which areexpressed in P3HR1 convertants,⁴⁷ cannot substitute for thisfunction of EBNA2. EBNA2 can transactivate viral and cellulargenes by binding to and converting the site-specific transcriptionalrepressor RBPJ ${kappa}$ (or CBF1) into a transcriptional activator.⁴⁸The expression plasmid pPDL152 codes for the point mutant WW323SRin conserved region 6 (CR6) of EBNA2. The mutation specificallyabrogates binding of RBPJ ${kappa}$ and derepression of RBPJ ${kappa}$ -repressedgenes.³⁷ We cotransfected EBV-negative BL cells with plasmidpPDL152 and the Ga981-16 reporter gene. As shown in Figure 1C,IL-18R ${alpha}$ mRNA is efficiently induced by this mutant, which onlymarginally enhanced transcription of the reporter (data notshown).

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Figure 1.. EBNA2 induces IL-18R ${alpha}$ expression in BL cells. (A) RT-PCR for IL-18R ${alpha}$ and the housekeeping gene, HPRT, in BL2, BL2-B95, BL2-P3, BL41, BL41-B95, BL41-P3, and KG-1 cells. (B) Flow cytometric analysis of IL-18R ${alpha}$ expression in BL2, BL2-B95, BL41, BL41-B95, and KG-1 cells. Cells were reacted with a mouse monoclonal antibody to IL-18R ${alpha}$ (filled histogram) or an isotype-matched control antibody (open histogram), followed by an FITC-labeled secondary antibody. (C) RT-PCR for IL-18R ${alpha}$ and HPRT in BL41 and BL41-P3 cells transfected with expression plasmids for EBNA2, LMP1, or the EBNA2-mutant WW323SR, as indicated. (D) BL2 cells, transiently transfected with an expression plasmid for EBNA2, were reacted 48 hours after transfection with a phycoerythrin-labeled mouse monoclonal antibody to IL-18R ${alpha}$ . Micrograph shows phase contrast and red fluorescence.

We conclude that IL-18R ${alpha}$ induction by EBNA2 is independent ofits capacity to bind RBPJ ${kappa}$ and does not require other EBV proteins.
Induction of IL-18R ${alpha}$ is highly specific to EBNA2
To further examine the role of EBNA2 in IL-18R ${alpha}$ expression, weused conditionally immortalized EREB2-5 cells. These cells harborthe EBNA2-deficient nontransforming EBV strain P3HR1 and constitutivelyexpress EBNA2 fused to the estrogen receptor (ER), which translocatesto the nucleus upon estrogen addition and drives proliferation.³⁴Incubation of EREB2-5 cells in the presence of estrogen rapidlyled to IL-18R ${alpha}$ protein expression on the cell surface (Figure 2A).To assess whether induction of IL-18R ${alpha}$ by EBNA2 requiredde novo protein synthesis, we recorded the accumulation of IL-18R ${alpha}$ mRNA in estrogen-treated EREB2-5 cells in the presence and inthe absence of the protein synthesis inhibitor, cycloheximide.Figure 2B shows that IL-18R ${alpha}$ mRNA was detectable already 6 hoursafter estrogen addition. While cycloheximide alone also ledto accumulation of a small amount of IL-18R ${alpha}$ transcripts, italmost completely abrogated their induction by EBNA2. Giventhat other viral proteins are not required (Figure 1), thesedata indicate that activation of IL-18R ${alpha}$ expression by EBNA2depends on de novo synthesis of a cellular protein(s). LMP1and EBNA2 have overlapping functions as transactivators of cellulargenes. We asked whether LMP1, together with the P3HR1-encodedlatent proteins, could replace EBNA2 in induction of IL-18R ${alpha}$ expression. We made use of the cell line LMPtet-EREB (ie, EREB2-5cells stably transfected with a tetracycline-controlled expressionplasmid for LMP1). We induced LMP1 expression and/or EBNA2 expressionin these cells and monitored the appearance of IL-18R ${alpha}$ on thecell surface. Figure 2C shows that LMP1 expression in the absenceof EBNA2 is not sufficient to induce IL-18R ${alpha}$ expression in EREB2-5cells and that it does not interfere with induction of IL-18R ${alpha}$ by EBNA2. These data confirm again that the IL-18R ${alpha}$ gene is nota target of LMP1.Acandidate cellular gene to mediate inductionof IL-18R ${alpha}$ expression by EBNA2 is the transcription regulatorc-myc, because the c-myc gene is activated by EBNA2⁴⁹ throughan RBPJ ${kappa}$ -independent mechanism. In addition, constitutive expressionof c-myc can substitute for EBNA2 in maintenance of proliferationin EREB2-5 cells.³³ We therefore asked whether it was also sufficientto drive IL-18R ${alpha}$ expression. The cell line P493-6 was establishedby stable transfection of EREB2-5 cells with a tetracycline-controlledexpression plasmid for c-myc. We induced c-myc expression and/orEBNA2 expression in these cells and analyzed IL-18R ${alpha}$ RNA andprotein expression by Northern blotting and flow cytometry.Figure 2D shows that c-myc cannot activate IL-18R ${alpha}$ in P493-6cells in the absence of EBNA2. Rather, IL-18R ${alpha}$ induction by EBNA2appears reduced on the protein and RNA levels when c-myc isoverexpressed. We conclude that, even in the P3HR1 background,c-myc cannot replace EBNA2 in IL-18R ${alpha}$ induction and that thelatter does not result from activation of the proliferativeprogram that is triggered by c-myc. EBNA2 and the cellular receptor,Notch, have overlapping functions beyond their capacity to interactwith RBPJ ${kappa}$ . Thus, the activated form of Notch, Notch-IC, caninduce the EBNA2 target genes CD21 and CD23 in EREB2-5 cells,⁵⁰and it can partially substitute for the growth-promoting functionsof EBNA2 in the presence of LMP1.³⁶ To investigate whether Notchcould activate IL-18R ${alpha}$ expression, we used the cell line 1414,derived from EREB2-5 by stable transfection of a tetracycline-controlledexpression plasmid for Notch-IC. Figure 2E shows that inductionof Notch-IC is unable to trigger IL-18R ${alpha}$ expression in the absenceof EBNA2.

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Figure 2.. EBNA2 but not LMP1, c-myc, or Notch induces IL-18R ${alpha}$ expression in nontransformed B cells. (A) Flow cytometric analysis of IL-18R ${alpha}$ expression (Figure 1B) in EREB2-5 cells treated with estrogen for the indicated times. (B) EREB2-5 cells were treated with estrogen (abbreviated E) and/or cycloheximide (CHX). Total RNA was prepared at the indicated time points, blotted, and probed with IL-18R ${alpha}$ cDNA. (C) Flow cytometric analysis of IL-18R ${alpha}$ expression in LMPtet-EREB cells treated with estrogen and/or tetracycline for 24 hours, as indicated. (D) Flow cytometric analysis of IL-18R ${alpha}$ expression in P493-6 cells treated with estrogen (EBNA2 on) and/or tetracycline (c-myc off) for 24 hours, as indicated. (E) Flow cytometric analysis of IL-18R ${alpha}$ expression in 1414 cells treated with estrogen (EBNA2 on) and/or tetracycline (Notch-IC off) for 24 or 96 hours, as indicated.

Taken together, these results show that activation of the IL-18R ${alpha}$ gene is an activity highly specific to EBNA2 that is not sharedby the known viral or cellular proteins with similar functions.
EBNA2 activates IL-18R ${beta}$ in a manner very similar to IL-18R ${alpha}$
The high-affinity IL-18 receptor is composed of IL-18R ${alpha}$ , whichbinds IL-18, and IL-18R ${beta}$ , which mediates signaling.²⁴ Hence,the biologic consequences of induction of IL-18R ${alpha}$ expressionby EBNA2 depend on the presence of IL-18R ${beta}$ in the EBV-infectedcells. We therefore analyzed the expression of IL-18R ${beta}$ in thesame cellular settings used for the analysis of IL-18R ${alpha}$ . RT-PCRfrom total RNA of the EBV-negative BL cell lines DG75, BL2,BL30, BL31, BL41, and BL70 demonstrated the absence of transcriptsspecific for IL-18R ${beta}$ . The B95-8 convertants, however, clearlyexpressed IL-18R ${beta}$ mRNA and surface protein, while P3HR1 convertantsdid not (Figure 3A and data not shown). This expression profilewas strikingly similar to that observed for IL-18R ${alpha}$ . Upon transfectioninto the EBV-negative BL cell lines BL2 and BL41, EBNA2 inducedIL-18R ${beta}$ mRNA in the absence of other viral proteins and independentlyof its capacity to bind RBPJ ${kappa}$ . LMP1, even in the P3HR1 background,could not substitute for EBNA2 (Figure 3B and data not shown).Induction of EBNA2 expression in EREB2-5 cells led to accumulationof IL-18R ${beta}$ RNA with similar kinetics as for IL-18R ${alpha}$ ; this effectwas inhibited by cycloheximide (Figure 3C and data not shown).Using the cell lines P493-6 and 1414, we found that the IL-18R ${beta}$ gene is neither inducible by c-myc nor by Notch in the presenceof P3HR1 (data not shown). These data demonstrate that the genescoding for the 2 chains of the IL-18 receptor are both specificallytargeted by EBNA2.

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Figure 3.. EBNA2 induces IL-18R ${beta}$ expression. (A) (Left) RT-PCR for IL-18R ${beta}$ and the housekeeping gene, HPRT, in BL2, BL2-B95, BL2-P3, BL41, BL41-B95, and BL41-P3HR1 cells. (Right) Green fluorescence micrograph of BL41-B95 cells, reacted with a goat polyclonal antibody to IL-18R ${beta}$ , followed by biotinylated antibodies to goat IgG and FITC-coupled streptavidin. (B) RT-PCR for IL-18R ${beta}$ and HPRT in BL2, BL41, and BL41-P3 cells transfected with expression plasmids for EBNA2 or LMP1, as indicated. (C) RT-PCR for IL-18R ${beta}$ in EREB2-5 cells treated with estrogen (E) for the indicated times.

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Figure 4.. A section from patient 4. (Left) Nuclear staining for EBNA2. (Middle) Positive staining for IL-18R ${alpha}$ in a subset of immunoblastic cells. (Right) Highermagnification micrograph showing membrane staining for IL-18R ${alpha}$ .

IL-18 receptor expression is linked to EBNA2 expression in vivo
In vivo, EBNA2 is expressed mainly in freshly infected B cells,⁵¹in posttransplantation EBV-associated lymphoproliferative disease,and in EBV-positive lymphomas in AIDS patients, with particularlyhigh incidence in primary central nervous system lymphomas.⁵²To assess whether EBNA2 expression was linked to IL-18R ${alpha}$ expressionin vivo, we examined 13 cases of diffuse large B-cell lymphoma(6 cases of primary central nervous system lymphoma from AIDSpatients and 7 cases from other anatomic sites) for the presenceof EBV and for the expression of EBNA2 and IL-18R ${alpha}$ . The resultsare listed in Table 1. Eight of 13 cases were EBV positive asjudged by in situ hybridization with a probe specific for EBER1RNA, as previously published.⁴⁴ The typical nuclear stainingfor EBNA2 was seen in 5 cases (4 cerebral and 1 peripheral lymphoma),with a range of EBNA2-positive cells among neoplastic cellsfrom 35% to 70%. A representative example of EBNA2 staining(patient 4) is shown in Figure 4. IL-18R ${alpha}$ expression was observedin 5 of 13 lymphomas tested, where 10% to 65% of the tumor cellsstained positive for IL-18R ${alpha}$ (Figure 4). Four of 5 immunoblasticlymphomas expressing EBNA2 stained positive for IL-18R ${alpha}$ . Sevenof 8 EBNA2-negative cases stained negative for IL-18R ${alpha}$ . The significantcorrelation between EBNA2 and IL-18R ${alpha}$ staining (P < .01; ${chi}$ ²test) supports the notion that EBNA2 is linked to IL-18R ${alpha}$ expressionin vivo.

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Table 1.. Immunohistochemical staining for EBNA2 and IL-18R ${alpha}$ in a series of immunoblastic lymphomas

IL-18 modifies gene expression in EBV-infected BL cells
Little is known about the signaling capacity of IL-18R in Bcells. In primary human B cells, IL-18 signals to NF- ${kappa}$ B and synergizeswith IL-12 in IFN- ${gamma}$ production only after preactivation by IL-12.²⁶We treated the EBV-positive BL cells BL2-B95, which expressIL-18R (Figure 1) with various amounts of IL-18. We did notobserve enhanced activity of the NF- ${kappa}$ B reporter genes Ig ${kappa}$ 3-ConA-Lucand p(IL6 ${kappa}$ B)3-50hu.luc, or of the human IFN- ${gamma}$ promoter, or enhancedIFN- ${gamma}$ production, even after pretreatment with IL-12 (data notshown).
To assess the capacity of EBV-infected BL cells to react toIL-18 alone, we compared the gene expression profile of IL-18-treatedBL2-B95 cells with that of BSA-treated cells using cDNA microarrays(Figure 5). To measure the reproducibility of the results andto exclude false positive and false negative results, we replicatedthe experiment (ie, we performed 4 microarray hybridizationsusing probes from separate duplicates of RNA prepared from BSA-treated[experiments BSA(1), BSA(2)] and IL-18-treated [experimentsIL-18(1), IL-18(2)] cells compared with the reference [R]).Statistical significance of the correlation between experimentsIL-18(1) and IL-18(2) was determined (Figure 5A) by plottingdifferential gene expression of one experiment against the valuefrom the other experiment.⁴⁵ An excellent correlation betweenexperiments was observed (r = 0.967), which was statisticallysignificant (P < .0001), showing the homogeneity and theconsistency of the cyanine-3 (Cy3) and and cyanine-5 (Cy5) signalsover different experiments. The frequency of genes for a givenlog ratio is shown in the histograms (Figure 5A). The sensitivityand reproducibility of the DNA microarrays is highlighted bythe fact that common regulated genes were detected in separateDNA microarray experiments. In the whole data set we could notfind a single major difference (genes regulated in oppositedirections) between the experiments, showing a very low variancebetween microarrays. Good intramicroarray reproducibility ondifferent cDNAs from the same gene was also found (eg, coregulationof major histocompatibility complex [MHC] class II DQ, cloneM24364 [GenBank] , clone U83582 [GenBank] , and clone M60028 [GenBank] ).

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Figure 5.. IL-18 modifies gene expression in EBV-infected BL cells. Differential gene expression in IL-18-treated versus BSA-treated BL2-B95-8 cells was analyzed using DNA microarrays. (A) Correlation analysis was performed by plotting differential gene expression (log ratio) from experiment IL-18(1) against that of experiment IL-18(2) (see "Results"). Negative values represent down-regulated genes, and positive values represent up-regulated genes. Histograms represent the frequency of genes with differential expression (log ratio). Correlation coefficient between experiments (r = 0.967) and statistical significance (P < .0001) was determined. (B) Hierarchical clustering analysis of genes differentially regulated between IL-18- and BSA-treated cells. Values a to d (see "Results") are plotted for genes having a significant (P < .05) difference of expression. (C) Genes having a significant (P < .05) difference of expression between BSA- and IL-18-treated cells were grouped in functional categories according to the Gene Ontology Database (GO; http://www.godatabase.org). Bars represent the number of IL-18-regulated genes in the indicated functional clusters and subcategories.

The gene expression differences between IL-18- and BSA-treatedcells (log ratio, log2(IL-18/BSA)) were calculated from thedifferences log2(IL-18(1)/R(1) - log2(BSA(1)/R), log2(IL-18(2)/R(1)- log2(BSA(1)/R), log2(IL-18(1)/R - log2(BSA(2)/R), and log2(IL-18(2)/R(1)- log2(BSA(2)/R) (values a to d), the variance being 2 ${sigma}$ .² Themean and SD were calculated, and genes having a significant(P < .05) difference of expression between IL-18- and BSA-treatedcells were plotted using hierarchical clustering (Figure 5B).Of the 12 814 unique human expressed genes of the DNA microarray,0.57% were down-regulated (73 genes) and 0.71% up-regulated(91 genes) using a P < .05 across all experiments, whereas32 genes and 26 genes were respectively up-regulated and down-regulatedusing a P < .01. Up-regulated genes include CD83, CD86, RANTES(regulated on activation normal T cells expressed and secreted),and the MHC alleles DQ ${alpha}$ 1, DQ ${beta}$ 1, and DN ${alpha}$ . Down-regulated genes includeHLA-DR.
Using the Gene Ontology database (GO, http://www.godatabase.org),IL-18-regulated genes were clustered into functional categories(Figure 5C). Expression of genes from 7 families having a frequencyof regulated genes above 6 was altered by IL-18. These includemetabolism, cell growth, signal transduction, transferase andhydrolase activities, immune response, and MHC class II receptoractivity-regulated genes.
These data imply that EBV infection leads to expression of afunctional IL-18 receptor that signals in response to IL-18.

   Discussion

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Abstract
Introduction
Materials and methods
Results
Discussion
References

The transcription factor EBNA2 activates, on one hand, cellulargenes that are involved in intrinsic growth and survival control,like cyclinD2,⁵³ c-myc,⁴⁹ and c-fgr.⁵⁴ On the other hand, itinduces expression of cell surface and soluble proteins thatmodulate the cell's interaction with the environment, like thereceptors CD21,⁵ CD23,⁶ and BLR2/CCR7⁹ and the cytokines TNF- ${alpha}$ and LT- ${alpha}$ .¹⁰
EBNA2 cannot bind DNA directly but contacts responsive promotersthrough interactions with cellular factors that include thesequence-specific repressor RBPJ ${kappa}$ (CBF1),^42,55 Spi-1/PU.1,^56,57and activating transcription factor (ATF).⁵⁸ It also can modulatetranscription through interactions with components of the basaltranscription machinery^59-61 and probably through chromatinmodification, because it binds the SWI/SNF chromatin-remodelingcomplex^62,63 and can form complexes with the histone deacetylaseHDAC2 independently of its ability to bind RBPJ ${kappa}$ .⁶⁴
We have shown here that EBNA2 induces expression of the 2 chainsof the IL-18 receptor in B cells. This activity is independentof its capacity to bind to RBPJ ${kappa}$ . No other EBV proteins but denovo synthesis of a cellular protein(s) are required for thiseffect.
The EBV latent membrane protein LMP1 and the cellular proteinsc-myc and Notch have overlapping functions with EBNA2, particularlyas transcriptional activators. LMP1 can partially substitutefor EBNA2 in cell survival³⁵ and in induction of the surfacemarkers CD21, CD23, intercellular adhesion molecule 1 (ICAM-1),and lymphocyte function antigen-1 (LFA-1).^65,66 Notch can partially³⁶and c-myc fully³³ replace EBNA2 in growth promotion in the presenceof the P3HR1 genome. We report here that neither LMP1, c-myc,nor Notch can induce expression of IL-18R even if the full setof EBV latent proteins (except EBNA2) is coexpressed. The IL-18Rgenes hence belong to the hitherto relatively small group ofgenes identified as specific targets of EBNA2, which includesTNF- ${alpha}$ , LT- ${alpha}$ ,¹⁰ and BLR2/CCR7.⁹
The c-myc gene is transcriptionally activated by EBNA2 in anRBPJ ${kappa}$ -independent fashion¹⁰ and hence was a good candidate tomediate IL-18 activation by EBNA2. However, its overexpressionin P493-6 cells was not sufficient to drive IL-18R expressionin the absence of EBNA2 (Figure 2D). Rather, c-myc overexpressionreduced IL-18R induction by EBNA2 in P493-6 cells, in keepingwith the previous observation that c-myc down-regulates severalB-cell activation markers in this cell line.⁶⁷
Taken together, our data demonstrate that the IL-18R genes areactivated through a mechanism that is highly specific to EBNA2among the EBV latent genes and among the known cellular geneswith similar functions as EBNA2.
Presence of the 2 chains of the IL-18 receptor has been shownto be sufficient for high-affinity binding of IL-18.²⁴ However,signaling capacity of IL-18 in B cells has been demonstratedonly after pretreatment with IL-12.^26,68 In our hands, IL-18neither enhanced the activity of NF- ${kappa}$ B reporter genes nor ofthe IFN- ${gamma}$ promoter and did not lead to enhanced IFN- ${gamma}$ secretionin BL2-B95 cells even after pretreatment with IL-12, in keepingwith previous reports showing that EBV-transformed B-cell lineslack a functional IL-12 receptor.^69,70 However, using microarrayexpression profiling, we could show here that IL-18 significantlymodifies gene expression in BL2-B95-8 cells (Figure 5). In atotal of 12 800 genes analyzed in 4 DNA microarray experiments,we found that IL-18 treatment significantly and reproduciblyalters the expression of at least 58 genes (P < .01). Thisresult implies a signaling capacity of the EBNA2-induced IL-18receptor, because IL-18 does not bind to other surface molecules.⁷¹Analysis of the regulatory elements of the IL-18-regulated geneswill contribute to elucidate the signal transduction pathwaysof IL-18R in B cells.
While we could not find IL-18 to be secreted by the BL cellsthemselves in vitro (data not shown), IL-18 may be availableto EBV-infected cells in vivo as part of T-cell-dependent and-independent immune reactions to EBV. Thus, elevated levelsof IL-18 are found in lymphoid tissues during infectious mononucleosis,²⁸and substantial amounts of murine IL-18 accumulate in experimentaltumors of LMP1-expressing BL cells in athymic mice.²⁹ In patients,EBNA2 is mainly expressed in newly EBV-infected B cells^51,72and in EBV-positive lymphomas of immunocompromised patients,particularly of the central nervous system.⁵² We examined herea series of cerebral immunoblastic lymphomas from AIDS patientsand report a correlation between EBNA2 expression and IL-18R ${alpha}$ receptor expression (Figure 4). This supports the notion thatEBNA2 can induce IL-18R ${alpha}$ expression in vivo. Our observationsprompt us to investigate whether IL-18R expression has a rolein the establishment and maintenance of EBV-infected B cells,in their EBNA2-dependent immunogenicity, and in their immunesurveillance.

   Acknowledgements

We thank G. Lenoir, J. Feuillard, F. Baran-Marszak, M. Rowe,B. Kempkes, and U. Zimber-Strobl for cell lines; J. E. Sims,A. Israel, H. Gruffat, A. Sergeant, G. Haegeman, K. Barbulescu,and W. Hammerschmidt for plasmids; and J. J. Hauw for providingtissue specimens from patients with DLBL.

   Footnotes

Submitted August 19, 2004; accepted October 13, 2004.
Prepublished online as Blood First Edition Paper, October 21,2004; DOI 10.1182/blood-2004-08-3196.

Supported by Association pour la Recherche sur le Cancer (G.K.,B.H.), and by the Alliance des Recherches sur le Cancer (ARECA)network.

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: Berthold Henglein, CNRS UMR 7098, Université Pierre et Marie Curie, Bat.C, 5e étage, 9 quai Saint Bernard, F-75005 Paris, France; e-mail: berthold.henglein{at}snv.jussieu.fr.

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Results
Discussion
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