Requirements for the Induction of Interleukin-6 by Herpes Simplex Virus-Infected Leukocytes

doi:10.1128/JVI.75.17.8008-8015.2001

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Journal of Virology, September 2001, p. 8008-8015, Vol. 75, No. 17
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.17.8008-8015.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Requirements for the Induction of Interleukin-6 by Herpes Simplex Virus-Infected Leukocytes

Søren R. Paludan^*

Department of Medical Microbiology and Immunology, University of Aarhus, Aarhus, Denmark

Received 2 March 2001/Accepted 29 May 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Cytokines play important roles in the clearance of herpes simplex virus (HSV) infections and in virus-induced immunopathology.One cytokine known to contribute to resistance against HSV isinterleukin-6 (IL-6). Here we have investigated virus-cell interactionsresponsible for IL-6 induction by HSV in leukocytes. Both HSVtype 1 and type 2 are potent inducers of IL-6, and this phenomenonis augmented in the presence of gamma interferon. The abilityto induce IL-6 is dependent on de novo protein synthesis and issensitive to UV irradiation of the virus. Virus mutants lackingthe virion-transactivating protein VP16 or any of the immediate-earlyproteins ICP0, ICP4, or ICP27 displayed unaltered capacities toinduce IL-6. However, wild-type virus was unable to induce IL-6in a macrophage cell line overexpressing a mutant of double-strandedRNA-activated protein kinase (PKR). This suggests a role for PKRin HSV-induced IL-6 expression. HSV infection led to enhancedbinding to the $kappa$ B, CRE, and AP-1 sites of the IL-6 promoter, andinhibitors against NF- $kappa$ B and the p38 kinase strongly reduced accumulationof IL-6 mRNA in infected cells. Moreover, macrophage cell linesexpressing dominant negative mutants of I $kappa$ B $alpha$ and p38 respondedto HSV-1 infection with reduced IL-6 expression compared to thecontrol-vector-transfected cell line. The results show that inductionof IL-6 by HSV in leukocytes is dependent on PKR and cellularsignaling through NF- $kappa$ B and a p38-dependentpathway.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Efficient elimination of virus infections occurs through a highly controlled host response relying on both the innate andacquired immune defense systems. For instance, mice infected inthe eye with herpes simplex virus type 1 (HSV-1) require bothmacrophages and T lymphocytes to resolve the infection (19).It is believed that the cross talk between different cell typesof the immune system is highly dependent oncytokines.

Interleukin-6 (IL-6) is a pleiotropic cytokine supporting a range of functions in the host response to infection and variousforms of stress. These include differentiation and proliferationof B cells and T cells, multipotent colony formation by hematopoieticstem cells and the acute-phase response (3). Recently it wasshown that IL-6 switches the differentiation of monocytes fromdendritic cells to macrophages (8). The role of IL-6 in clearanceof infections with intracellular bacteria and viruses has beendemonstrated through studies with IL-6-deficient mice (20).Specifically, it was shown that such mice are unable to controlinfections with Listeria monocytogenes and vaccinia virus. Moreover,the mice mount an impaired T-cell-dependent antibody responseagainst vesicular stomatitis virus. Recently, it has been demonstratedthat IL-6 is also required for an optimal immune response afterocular HSV-1 infection (23). Despite similar viral titers inthe eye, the knockout mice were less able than their wild-typelittermates to survive theinfection.

As to the cell types responsible for IL-6 production, many cell populations have been reported to produce this cytokine, withmonocytes and macrophages representing an important source (3).The molecular mechanism of IL-6 induction has been studied ingreat detail for a number of nonviral proinflammatory agents (11,15, 27, 30, 37), whereas the regulation by viral infectionsis less well understood. The IL-6 promoter contains a region withadjacent binding sites for nuclear factor $kappa$ B (NF- $kappa$ B) and NF-IL6,and the participation of these two factors in IL-6 expressionin response to many stimuli is well documented (27). Moreover,binding sites for activator protein 1 (AP-1), cAMP responsiveelement binding protein, and activating transcription factor 2(ATF2/Jun) are present, and potential roles for these in IL-6gene transcription have been suggested (11, 21).

A number of studies have addressed which viral entities elicit cytokine expression (reviewed in reference 28). For instance,it has been shown that cytomegalovirus induces IL-6 productionthrough interaction between the viral glycoprotein gB and a cellularreceptor (6), while hepatitis B virus triggers the responseby a mechanism dependent on the viral X protein (24). Humanimmunodeficiency virus is particularly interesting in this respectsince it induces IL-6 by no fewer than four distinct mechanismsinvolving the viral proteins gp120, Tat, Nef, and Vpr (4, 10,35, 38).

In this study we have investigated the ability of leukocytes to produce IL-6 in response to HSV infection and have studiedviral components responsible for the induction. In addition, ourwork addresses the cellular signaling pathways leading to IL-6expression in HSV-infectedleukocytes.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Reagents. The recombinant cytokines used were murine IL-6 (Genzyme), murine gamma interferon (IFN- $gamma$ ) (Pharmingen), and human IFN- $gamma$ (Genzyme).Antibodies used were neutralizing polyclonal rabbit anti-tumornecrosis factor alpha (TNF- $alpha$ ) (Genzyme), mouse monoclonal anti-gD(Virusys), rat monoclonal anti-mouse IL-6 (Genzyme), biotinylatedmonoclonal rat anti-mouse IL-6 (Pharmingen), and horseradish peroxidase-conjugatedrabbit polyclonal anti-mouse immunoglobulin (Transduction Laboratories).RNA was purified with Trizol (Life Technologies) and reverse transcribedusing Expand Reverse Transcriptase (Roche). For PCR amplification,Taq2000 DNA polymerase (Stratagene) was used. The chemical inhibitorsof diverse cellular functions were cyclosporine (CsA; Sigma),1 µM; SB203580 (Calbiochem), 10 µM; pyrollidine dithiocarbamate(PDTC; Sigma), 10 µM; N-tosyl-L-phenylalanine chloromethyl ketone(TPCK; Sigma), 3 µM; H89 (Biomol), 5 µM; GF109203X (Biomol) andcycloheximide (CHX; Sigma), 10 µg of each/ml. DNA primers andprobes were obtained from DNA Technology. LumiGLO was purchasedfrom New England BioLabs, and the polyvinylidene difluoride membraneswere from Novex. Heparin was from Leo Pharmacies and G418 wasobtained from Roche. Cells were transfected with LipofectAMINE(LifeTechnologies).

Cell culture. Peripheral blood mononuclear cells (PBMCs) were isolated from blood obtained from a healthy 28-year-old male donor by Isopaque-Ficollseparation. Briefly, the blood was laid on top of Ficoll and centrifugedat 600 × g for 30 min at 20°C. The PBMC-containing interphasewas isolated, and the cells were washed in phosphate-bufferedsaline (PBS) containing 100 µg of heparin per ml. Subsequently,the cells were centrifuged at 200 × g for 15 min at 20°C and resuspendedin RPMI 1640 medium containing 5% fetal calf serum (FCS) and antibiotics(200 IU of penicillin per ml and 200 µg of streptomycin per ml).The cells were seeded in 10-cm² tissue culture wells at a density of 7 × 10⁶ cells/well and left overnight before stimulation andinfection.

Resting peritoneal cells (PC) were harvested from C57BL/6 mice by lavage of the peritoneal cavities with cold PBS supplementedwith 2% FCS and 20 IU of heparin per ml. Inflammatory macrophageswere induced by injection of 2 ml of 10% thioglycolate into theperitoneal cavities of C57BL/6 mice, and five days later the cellswere harvested as described above. The cells were washed oncein RPMI 1640 medium plus 5% FCS and seeded at a density of 7 ×10⁶ cells/10 cm² and left overnight before stimulation andinfection.

The cell lines RAW 264.7 and J774A.1 were maintained in Dulbecco's minimal essential medium with 1% Glutamax I (Life Technologies),antibiotics, and 5% FCS. For experiments, the cells were seededin 10-cm² tissue culture wells at a density of 2 × 10⁶ cells/well and left 16 to 20 h before further treatment. THP-1cells were grown in RPMI 1640 containing 2 mM glutamine, 10% FCS,and antibiotics. For experiments the cells were seeded in 10-cm² tissue culture wells at a density of 5 × 10⁶ cells per well. Vero cells were maintained in minimal essentialmedium supplemented with 200 IU of penicillin per ml, 200 µg ofstreptomycin per ml, and 5% FCS. For virus amplification the cellswere seeded at a density of 2 × 10⁷ cells per 175-cm² tissue culture flask 5 h prior to infection. For plaque assays,the cells were seeded at a density of 2 × 10⁶ cells per 22.5-cm² tissue cultureplate.

The RAW 264.7-derived cell lines were grown in the same manner as the parental cell line, with the addition of 300 µg of G418per ml. The protein kinase (PKR)-mutant cell line RAW-PKR-M7 andempty vector control cell line RAW-pBK-CMV, kindly donated byJ. A. Corbett, Washington University (25), were grown in thepresence of 200 µg of G418 perml.

Viruses The wild-type viruses used in this study were the MS strain of HSV-2 and the KOS and 17+ strains of HSV-1. The ICP0 mutantdl1403, the VP16 mutant in1814, and the rescued virus in1814Rare on a 17+ genetic background (1, 41). The mutants lackingICP4 or ICP27 or gL are on a KOS genetic background (29, 34,39). The viruses were produced essentially as previously described(12). Just before usage, virus was thawed and used as infectiousvirus, subjected to heat inactivation at 56°C for 30 min, or inactivatedby UV light for 15min.

Isolation of RNA and RT-PCR. RNA was isolated using Trizol according to the manufacturer's recommendations. Two micrograms of RNA was subjected to reversetranscription (RT) using oligo(dT)₁₅ and Expand Reverse Transcriptase.The cDNA was amplified by PCR with the following primers: humanIL-6, 5'-ACA AAT TCG GTA CAT CCT C-3' (sense) and 5'-GCA GAA TGAGAT GAG TTG T-3' (antisense); murine IL-6, 5'-TTC TGG AGT ACCATA GCT AC-3' (sense) and 5'-AGT TCT TCG TAG AGA ACA AC-3' (antisense); $beta$ -actin, 5'-CCA ACC GTG AAA AGA TGA CC-3' (sense) and 5'-GCA GTAATC TCC TTC TGC ATC C-3' (antisense). The products spanned 421bp (human IL-6), 370 bp (murine IL-6), and 616 bp ( $beta$ -actin). TheRT-PCR protocol was tested with serial twofold dilutions of RNAprepared from RAW 264.7 cells treated with HSV-1 and IFN- $gamma$ for4 h. Twenty cycles of PCR were found to be required to detectIL-6 mRNA, and a twofold difference in input material could bedetected on the final agarose gel when performing 25 PCR cycles(data notshown).

ELISA. Murine IL-6 was detected by enzyme-linked immunosorbent assay (ELISA). Maxisorp plates were coated overnight at 4°C with 2µg of anti-IL-6 per ml in coating buffer (15 mM Na₂CO₃, 35 mMNaHCO₃, 0.2% sodium azide [pH 9.6]). After blocking for 2 h at37°C with PBS (pH 7.4) containing 1% (wt/vol) bovine serum albumin,samples and standard dilutions of IL-6 (3.9 to 2,000 pg/ml) wereadded to the wells and the plates were incubated at 37°C for 1h. Subsequently the wells were incubated for 1 h at 37°C witha biotin-labeled IL-6 detection antibody at a concentration of1 µg/ml in blocking buffer. Finally, horseradish peroxidase-conjugatedstreptavidin, diluted in blocking buffer, was added and incubatedfor 20 min at 20°C, and the result was visualized by the TMB system.After 10 min the color reaction was stopped with 5% H₂SO₄. Betweeneach step the plates were washed three times with PBS containing0.05% (vol/vol) Tween 20. The results were quantified by readingthe absorbance at 450nm.

Isolation of nuclear extracts. To isolate nuclear proteins, the cell monolayer was washed twice with ice-cold PBS, scraped off the plate, and spun down (2,000× g for 1 min). The cells were resuspended in a hypotonic buffer(20 mM HEPES [pH 7.9], 1.5 mM MgCl₂, 10 mM KCl, 0.5 mM dithiothreitol[DTT], 0.2 mM EDTA, 0.2 mM phenylmethylsulfonyl fluoride [PMSF],0.2 mM leupeptin, 0.2 mM pepstatin A, 0.1 mM Na₃VO₄) and lefton ice for 15 min. NP-40 was added to 0.6%, and the mixture wasvortexed 15 s and centrifuged at 10,000 × g for 1 min. Extractionbuffer (20 mM HEPES [pH 7.9], 20% glycerol, 1.5 mM MgCl₂, 420mM NaCl, 0.5 mM DTT, 0.2 mM EDTA, 0.2 mM PMSF, 0.2 mM leupeptin,0.2 mM pepstatin A, 0.1 mM Na₃VO₄, 0.2% NP-40) was added to thenuclei, and incubated 30 min at 4°C with rocking. The sampleswere centrifuged at 10,000 × g for 15 min at 4°C and the supernatantswere harvested as nuclearextracts.

Electrophoretic mobility shift assay. To assay for DNA-binding activity, 5 µg of protein in 3 µl of nuclear extraction buffer was mixed with 4 µg of poly(dI-dC)and 20,000 cpm of ³²P-labeled probe in 18 µl. The final concentrations were 4 mM Tris-HCl,23 mM HEPES (pH 7.9), 66 mM NaCl, 5 mM MgCl₂, 0.7 mM EDTA, 1 mMDTT, and 14% glycerol. After 25 min of incubation at room temperature,the reaction mixture was subjected to electrophoresis on a nondenaturing5% polyacrylamide gel in 0.5× TBE buffer (45 mM Tris base, 45mM boric acid, 1 mM EDTA). The gel was dried and analyzed by autoradiography.For competition assays 100-fold excess of cold probe was addedtogether with the labeled probe. The probes corresponding to sitesin the murine IL-6 promoter are as follows: $kappa$ B, 5'-ATG TGG GATTTC CCA TG-3'; AP-1, 5'-AGT GCT GAG TCA CTT TT-3'; CRE, 5'-CTAAAC GAC GTC ACA TTG-3'; C/EBP, 5'-CGT CAC ATT GTG CAA TCT TAAT-3'.

Stable transfections. The DNA plasmids used for transfections encoded dominant negative versions of p38 and I $kappa$ B $alpha$ . The p38 construct was a kind giftfrom Helmut Holtmann (43). To generate the dominant negativeI $kappa$ B $alpha$ expression construct, mutant I $kappa$ B $alpha$ , generously donated byJohn Hiscott (22), was amplified by PCR with the high-fidelitypolymerase Pfu using the following primers: 5'-GAA TTC ATG TTCCAG GCG GCC GAG-3' (sense), 5'-GTC GAC TTA GAA CTC TGA CTC TGTGTC-3' (antisense) (restriction sites used for subcloning areunderlined). The PCR fragment was cloned into the EcoRV site ofpBluescript KS and subcloned into the appropriate sites in pcDNA3.For the empty vector, control pcDNA3 was used. For transfectionsthe cells were seeded at a density of 5 × 10⁶ cells/25-cm² plate and left for 24 h. The cells were transfected using LipofectAMINE(7.5 µg of DNA and 20 µl of LipofectAMINE) and serum-free medium.Four hours after transfection, FCS was added to 10%, and the cellswere incubated 24 h before application of selection with 300 µgof G418 per ml. Surviving colonies were pooled in order to avoidsingle-clone abnormalities, and cells were grown through fiveto eight passages in Dulbecco's modified Eagle's medium supplementedwith 5% FCS in the presence of selection. The levels of ectopicexpression were assessed by Western blotting prior to use of thecelllines.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Expression of IL-6 in human and murine leukocyte populations after HSV infection. It has previously been shown that HSV infections induce expression of IL-6 in vivo (14, 40), and we wanted to examineif selected leukocyte populations responded to HSV infection invitro with expression of IL-6. As seen from Fig. 1 human PBMCs,murine PCs, J774A.1, and RAW 264.7 cells all produced IL-6 mRNAfollowing HSV-1 infection. In contrast, no IL-6 mRNA was producedby THP-1 cells after HSV-1 infection. In most of the HSV-responsivecells, cotreatment with IFN- $gamma$ enhanced the levels of accumulatedIL-6 mRNA. Similar results were obtained with HSV-2 (data notshown). These results show that many human and murine leukocytepopulations express IL-6 after HSV infection.

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FIG. 1. Expression of IL-6 mRNA in various human and murine leukocyte populations. Primary cells were isolated as described in Materials and Methods. The primary cells and cell lines were seeded and left overnight to settle. The cells were infected with 3 × 10⁶ PFU of HSV-1 (KOS) per ml and stimulated with 10 IU of human or murine IFN- $gamma$ per ml. After 4 h of treatment, total RNA was isolated and subjected to RT-PCR using oligo(dT)₁₅ RT priming and PCR primers specific for murine $beta$ -actin, human IL-6, and murine IL-6. PBMC, peripheral blood mononuclear cells; PC, peritoneal cells; TG, thioglycolate.

Induction of IL-6 in macrophages is dependent on a functional viral genome and intermediary de novo protein synthesis. We also examined if the enhanced IL-6 mRNA accumulation was associated with secretion of IL-6 protein. Whereas RAW 264.7 cellsleft untreated or treated with heat-inactivated virus or mockpreparation produced little or no IL-6, infection with eitherHSV-1 or HSV-2 led to a strong induction of IL-6 protein (Fig.2A). IFN- $gamma$ alone did induce some IL-6, and an appreciable synergywas observed between IFN- $gamma$ and HSV infection. The ability of HSV-1to induce IL-6 expression did not occur through phagocytosis-mediateduptake of virus particles, since gL-deficient HSV-1, which canadsorb but not penetrate cells, was unable to affect IL-6 proteinlevels in supernatants from resting or IFN- $gamma$ -treated RAW 264.7cells (data not shown).

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FIG. 2. Characterization of IL-6 induction by HSV-kinetics and effects of cycloheximide, anti-TNF- $alpha$ , and UV-irradiation of the virus. RAW 264.7 cells were seeded and left overnight to settle. (A) The cells were treated with 3 × 10⁶ PFU of HSV-1 (KOS) per ml, 3 × 10⁶ PFU of HSV-2 (MS) per ml, and 10 IU of IFN- $gamma$ per ml. After 24 h, supernatants were harvested and analyzed for IL-6 by ELISA. The results are shown as means ± standard errors of the means. (B) The cells were treated as indicated with the following concentrations: 3 × 10⁶ PFU of HSV-1 (KOS) per ml or equivalent amount of UV-irradiated virus, 10 IU of IFN- $gamma$ per ml, 1,000 U of neutralizing anti-TNF- $alpha$ per ml, 10 µg of CHX per ml. After 4 h of treatment total RNA was isolated. (C) The cells were treated with 3 × 10⁶ PFU of HSV-1 (KOS) per ml and 10 IU of IFN- $gamma$ per ml. After the indicated time points total RNA was isolated. (B and C) The RNA was subjected to RT-PCR using oligo(dT)₁₅ RT-priming and PCR primers specific for murine $beta$ -actin and IL-6.

To further characterize the HSV-induced IL-6 expression, we tested if a functional virus genome was required for the induction.This is normally done by irradiating the virus with UV light priorto infection. Such experiments have previously revealed that theability of HSV to induce IL-12 p40 expression is sensitive toUV light (26) whereas the virus induces secretion of IFN- $alpha$ / $beta$ and TNF- $alpha$ through a mechanism displaying only little sensitivityto this treatment (12). When RAW 264.7 macrophage-like cellswere infected with UV-irradiated HSV-1, we observed that no IL-6was induced (Fig. 2B). UV treatment totally prevented the accumulationof mRNA for ICP27 ( $alpha$ ), ICP8 ( $beta$ ), and gD ( $gamma$ 1) normally observedafter infection of RAW 264.7 cells with live HSV-1 and HSV-2 (datanot shown). We also examined if virus-induced TNF- $alpha$ was involvedin the induction, since it is known that TNF- $alpha$ supports IL-6 expression(37). However, the presence of neutralizing TNF- $alpha$ antibodieshad no appreciable effect on the IL-6 mRNA levels. Given the UV-sensitivenature of the response, we also wanted to examine if de novo proteinsynthesis was required for the induction of IL-6 mRNA expression.We found that the protein synthesis inhibitor CHX per se did enhancethe IL-6 mRNA levels marginally. More importantly, however, theability of infection to affect IL-6 mRNA levels was abolishedby CHX treatment. Finally, we examined the kinetics of IL-6 mRNAaccumulation after HSV-1 infection. In the experiment shown, adetectable level of IL-6 mRNA was present constitutively (Fig.2C). After 2 h of infection a significant increase in the IL-6mRNA levels was observed, and they increased further between 2and 5 h postinfection and remained high through the 8 h of theexperiment.

Induction of IL-6 by mutant viruses in wild-type cells and by wild-type HSV-1 in macrophages unable to respond to double-stranded RNA. In order to identify the virus-cell interactions responsible for IL-6 induction, we analyzed the ability of a number of HSV-1mutants to induce expression of the cytokine in macrophages. First,we tested mutants with defects in the tegument protein VP16 (in1814),the immediate-early proteins ICP0 (dl1403), ICP4 (vi13) or ICP27(d27-1). As seen in Fig. 3A, all 4 mutants retained the capacityto induce IL-6, demonstrating that any of the four proteins alonewas redundant for IL-6 induction.

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FIG. 3. Induction of IL-6 by mutant viruses in wild-type cells and by wild-type HSV-1 in macrophages unable to activate PKR in response to double-stranded RNA. (A) RAW 264.7 cells were seeded and left overnight to settle. The cells were treated with 10 IU of IFN- $gamma$ per ml and 3 × 10⁶ PFU of wild-type or mutant HSV-1 per ml. After 4 h of treatment, total RNA was isolated and subjected to RT-PCR using oligo(dT)₁₅ RT-priming and PCR primers specific for murine $beta$ -actin and IL-6. (B) The RAW 264.7-derived cell lines pBK-CMV and PKR-M7 were seeded as above. Sixteen hours later the cells were treated with 10 IU of IFN- $gamma$ per ml and 3 × 10⁶ PFU of HSV-1 (KOS) per ml. After 4 h of treatment, total RNA was extracted and analyzed for IL-6 and $beta$ -actin by RT-PCR.

We also tested if macrophages unable to activate the double-stranded RNA-activated kinase PKR in response to infection werecapable of producing IL-6. To this end we used a RAW 264.7-derivedcell line stably expressing a PKR mutant (PKR-M7) lacking thefirst double-stranded RNA-binding domain which is required formaximal kinase activity (25). We found that whereas the cellline transfected with the parental vector was fully capable ofproducing IL-6 in infected cells, the PKR-M7-harboring cells didnot respond to infection or IFN- $gamma$ stimulation with expressionof IL-6 (Fig. 3B). Cotreatment with IFN- $gamma$ and HSV-1 did allowproduction of low amounts of IL-6.

Activation of DNA-binding activity to the IL-6 promoter after HSV infection. To identify virus-induced cellular signal transduction responsible for IL-6 expression, we performed an electrophoretic mobilityshift assay using probes derived from the murine IL-6 promoter.Nuclear extracts were prepared at different time points afterHSV and IFN- $gamma$ treatment, and the extracts were examined for DNA-bindingactivity. When using the probe corresponding to the $kappa$ B site localizedbetween 73 and 65 nucleotides (nt) upstream of the transcriptionalstart site, we found that binding was not induced or was onlyweakly induced after 1 h but was strongly enhanced after 2 h andremained elevated through the 6 h of the experiment (Fig. 4A).The CRE site (167 to 160 nt) and AP-1-binding site (277 and 271nt) were also analyzed, and we observed that a modest yet specificand reproducible induction occurred (Fig. 4B and C). This wasmost apparent after between 2 and 3.5 h, which interestingly correlateswith the onset of IL-6 mRNA accumulation (Fig. 2C). Finally weexamined the binding pattern of a C/EBP-binding site (158 and145 nt) in the promoter. As seen in Fig. 4D, no induction of C/EBPbinding to the probe was detected within the 6-h time frame chosenfor the experiment. All the above-described protein-DNA complexeswere sequence specific as assessed by competition with identicaland unrelated cold probes (data not shown). Together these resultsopen up the possibility of a role for NF- $kappa$ B-, AP-1-, and CRE-bindingproteins in virus-induced IL-6 expression.

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FIG. 4. Binding activity to $kappa$ B, CRE, AP-1, and C/EBP sites of the murine IL-6 promoter. RAW 264.7 cells were treated with 10 IU of IFN- $gamma$ per ml and infected with 3 × 10⁶ PFU of HSV-1 (KOS) per ml for the indicated time periods, and nuclear extracts were prepared. The extracts were tested for binding to the following probes: $kappa$ B (A), CRE (B), AP-1 (C), and C/EBP (D). Five micrograms of nuclear proteins and 20,000 cpm of ³²P-labeled probe were used per reaction. The binding was quantified by densitometric measurements of the autoradiographs. The results are shown as histograms using arbitrary units.

To evaluate the potential involvement of PKR in activation of these transcription factors, we used the PKR mutant cell line.This cell line (PKR-M7) and the empty-vector control cell line(pBK-CMV) were treated with mock preparation or HSV-1 plus IFN- $gamma$ for 3.5 h, and nuclear extracts were prepared. When examiningfor $kappa$ B-binding activity, we found that the constitutive band observedin the parental RAW 264.7 cells was absent (compare Fig. 4A and5A). However, both pBK-CMV and PKR-M7 activated $kappa$ B-binding activityto at least the same extent as RAW 264.7 did. In contrast to this,we found that the abilities of HSV-1 infection and IFN- $gamma$ treatmentto induce binding to CRE and AP-1 probes were impaired in PKR-M7cells compared to the pBK-CMV cells (Fig. 5B and C). Therefore,RAW 264.7 cells harboring the PKR mutant M7, which lacks the firstRNA-binding domain, are fully capable of activating NF- $kappa$ B in responseto HSV-1 infection but display reduced activation of AP-1- andCRE-binding factors.

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FIG. 5. PKR dependency of binding activity on the $kappa$ B, CRE, and AP-1 sites of the murine IL-6 promoter. RAW-pBK-CMV or RAW-PKR-M7 cells were mock infected or treated with 10 IU of IFN- $gamma$ per ml and 3 × 10⁶ PFU of HSV-1 (KOS) per ml. Nuclear extracts were prepared 3.5 h later, and the extracts were tested for binding to $kappa$ B (A), CRE (B), and AP-1 (C) probes. Five micrograms of nuclear proteins and 20,000 cpm of ³²P-labeled probe were used per reaction. The binding was quantified by densitometric measurements of the autoradiographs. The results are shown as histograms using arbitrary units.

HSV-induced IL-6 expression is repressed by inhibitors against NF- $kappa$ B and the p38 MAP kinase. To further analyze the signaling pathways involved in HSV-induced IL-6 expression, we tested the influence of a range of chemicalinhibitors on IL-6 mRNA accumulation. For this experiment, thecells were pretreated with the inhibitors 15 min prior to cytokinestimulation and HSV infection. Four hours after infection andstimulation, RNA was extracted and analyzed for IL-6 and $beta$ -actinmRNA (Fig. 6). We found that virus-induced accumulation of IL-6mRNA was not significantly affected by inhibitors against NF-ATactivation (CsA), protein kinase A (H89), or protein kinase C(GF109203X). In contrast, the p38 kinase inhibitor SB203580 andTPCK, which prevents NF- $kappa$ B activation, totally abolished IL-6production. Another inhibitor of NF- $kappa$ B activation, PDTC, had amore modest effect. Together these results support a role of NF- $kappa$ Band a p38-dependent pathway in HSV-induced IL-6 induction.

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FIG. 6. Effects of chemical inhibitors on HSV-induced IL-6 expression. RAW 264.7 cells were seeded and left overnight to settle. The cells were treated with inhibitors and left for 15 min prior to stimulation with 10 IU of IFN- $gamma$ per ml and infection with 3 × 10⁶ PFU of HSV-1 (KOS) per ml. Four hours later, total RNA was extracted and IL-6 and $beta$ -actin were detected by RT-PCR using primers specific for the two mRNA species.

Induction of IL-6 in RAW 264.7 cells expressing dominant negative I $kappa$ B $alpha$ and p38. To corroborate the above results with other data, we generated RAW 264.7-derived cell lines stably expressing dominant negativemutants of I $kappa$ B $alpha$ and p38. The cells were infected with HSV-1 andstimulated with IFN- $gamma$ . After 4 h, one-half of the cell cultureswere harvested and RNA was extracted. The remaining cell cultureswere left for 24 h prior to collection of the culture supernatants.The RNA and supernatants were analyzed for the presence of IL-6mRNA and protein, respectively. The cell line transfected withempty vector displayed an expression pattern similar to that ofthe parental RAW 264.7 cell line (compare Fig. 7A with Fig. 2Aand 3). In contrast, if the cells expressed the I $kappa$ B $alpha$ mutant, theability of HSV-1 to induce IL-6 alone or in concert with IFN- $gamma$ was severely compromised (Fig. 7B). Finally we found that overexpressionof dominant negative p38 only had a moderate effect on IL-6 inductionby virus alone but significantly compromised the synergy betweenIFN- $gamma$ and HSV-1 (Fig. 7C). Similar results were obtained withHSV-2 (data not shown).

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FIG. 7. Induction of IL-6 by HSV-1 in macrophages stably transfected with dominant negative I $kappa$ B $alpha$ and p38. RAW 264.7-derived cell lines with the following characteristics were generated: pcDNA3 (A), dominant negative I $kappa$ B $alpha$ (B), dominant negative p38V (C). The cells were seeded, infected with 3 × 10⁶ PFU of HSV-1 (KOS) per ml, and stimulated with 10 IU of IFN- $gamma$ per ml. After 4 h, cells to be analyzed for mRNA expression were lysed and total RNA was extracted. IL-6 and $beta$ -actin were detected by RT-PCR using primers specific for the two mRNA species (upper panel). Other cells were left for 24 h, at which point supernatants were harvested and analyzed for IL-6 protein by ELISA. The results (lower panel) are shown as means ± standard errors of the means.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The first line of defense against virus infections involves NK cells and macrophages. These cells are able to directly inhibitvirus replication through a number of antiviral effector mechanismsand also to cross-activate other cells of the immune system. Thislatter function is primarily mediated by cytokines. One cytokinewith a role in the immune response to virus infections is IL-6,which is a cytokine with pleiotropic activities. For instance,this cytokine supports differentiation of B lymphocytes, playsa role in T-cell differentiation, inhibits myeloid-cell growthwhile inducing differentiation of these cells into macrophages,and induces an acute-phase response in hepatocytes (3, 8).It has been shown that IL-6-deficient mice exhibit an impairedT-cell-dependent antibody response to vesicular stomatitis virusinfections, which are accompanied by increased virus titers inthese mice (20). During an HSV infection IL-6 is produced intwo phases: one early after infection, dependent on the presenceof virus, and one at later stages of infection, in a manner independentof the presence of virus (40). It has been demonstrated thatIL-6 does contribute to resistance against HSV-1 infections sinceIL-6-deficiency and transgenic IL-6 expression enhances susceptibilityand resistance, respectively, to HSV-1 infections (7, 23).

Here we have investigated the molecular mechanisms underlying the early IL-6 expression in various leukocyte populations.Among the cell types tested, all except one expressed IL-6 inresponse to HSV infections. Costimulation with IFN- $gamma$ further augmentedIL-6 mRNA accumulation. Thus, IL-6 is produced by leukocytes ofboth mouse and human origins as a primary response to HSVinfections.

The virus-host interactions responsible for IL-6 production were investigated by two approaches. First, we examined mutantviruses for their capacities to induce IL-6. Second, IL-6 expressionby a macrophage cell line expressing a dominant negative mutantof the double-stranded RNA-activated protein kinase PKR was tested.The PKR mutant used lacks the first double-stranded RNA-bindingdomain of PKR (25). The results obtained suggest that neitherthe virion-associated transactivator VP16 nor any one of the immediate-earlyproteins ICP0, ICP4, or ICP27 alone was essential for IL-6 induction.This is in agreement with previous studies with a permissive murineepithelial cell line (17). Despite the nonessential role ofany of the three immediate-early proteins alone for inductionof IL-6, a functional viral genome was required. This was evidencedby the lack of IL-6 expression after treatment with UV-irradiatedvirus.

When examining the role of PKR, we found that overexpression of a dominant negative PKR mutant abolished the ability of HSV-1to induce IL-6. However, the effect was not virus specific sinceIFN- $gamma$ was also unable to induce IL-6 in the mutant cell line.Cotreatment with HSV-1 and IFN- $gamma$ did allow some production ofIL-6. This result could suggest that PKR senses the accumulationof viral double-stranded RNA in the infected cell and inducessignal transduction leading to cytokine induction. In fact, througha mechanism dependent on PKR, double-stranded RNA is known toactivate the signal transduction cascades found here to be involvedin IL-6 induction (13, 45). The kinetics of IL-6 mRNA productionalso allows a role for double-stranded RNA in the process, sinceaccumulation of immediate-early viral mRNA precedes IL-6 mRNA(J. Melchjorsen and S. R. Paludan, unpublished data). However,we also observed that IFN- $gamma$ was unable to induce IL-6 expressionin the mutant cell line, which argues for a double-stranded RNA-independentrole of PKR in the process. HSV-1 has been reported to inhibitPKR in vitro through at least two different mechanisms (9,33). Yet, PKR-deficient mice display significantly enhancedsusceptibility to HSV-1 infections (18). Our study did not addresswhether PKR activity was affected by HSV infection in macrophages,but the reduced IL-6 expression in the PKR mutant cell line mayhelp to explain why PKR deficiency renders mice more susceptibleto HSV-1infections.

As to the cellular signaling and transcription factors responsible for IL-6 induction by HSV, our results suggest that NF- $kappa$ Band a p38-dependent pathway, likely ATF2/Jun, are important. NF- $kappa$ Bis a cardinal mediator of proinflammatory gene expression. Thedimeric transcription factor is present in the cytoplasm in restingcells in a latent form bound to the inhibitory subunit I $kappa$ B (5).Upon stimulation, I $kappa$ B is phosphorylated by the I $kappa$ B kinase andsubsequently degraded, allowing NF- $kappa$ B to migrate to the nucleusand promote transcription. HSV-1 and HSV-2 have previously beenshown to activate NF- $kappa$ B in various cell types (16, 31, 32),and we have shown that this does contribute to expression of proinflammatorymediators (26, 31). Here we show that NF- $kappa$ B also contributesto induction of IL-6 expression. As to the mechanism of NF- $kappa$ Bactivation, we found that it was independent of PKR. Others havereported that ICP4 and ICP27 are essential for sustained NF- $kappa$ Bactivity in HSV-1-infected C33 cells (32). In macrophages, however,other mechanisms seem to be involved, since viruses deficientin ICP4 and ICP27 displayed no apparent defect in their abilityto induce IL-6, which is dependent on NF- $kappa$ B.

Our results also suggest that a p38-dependent pathway, which could involve ATF2/Jun, contributes to HSV-induced IL-6 expression.First, we found that binding to the CRE-like site of the murineIL-6 promoter was induced after infection in IFN- $gamma$ -activated macrophages.This was not observed in RAW-PKR-M7 cells, suggesting a role forPKR in HSV-1-induced CRE-binding activity. Second, inhibitionof the ATF2 kinase p38 by SB203580 strongly reduces IL-6 expression.Third, macrophages stably transfected with dominant negative p38are unable to induce maximal IL-6 expression in response to HSV-1and IFN- $gamma$ . It is interesting, though, that IL-6 induction by HSV-1per se is only marginally affected. This result indicates thata p38-dependent pathway, possibly mediated through ATF2/Jun activationand recruitment to the CRE site of the IL-6 promoter, is essentialfor the synergistic induction of IL-6 by HSV and IFN- $gamma$ . Finally,the transient nature of the CRE-binding activity, which is incontrast to the sustained expression of IL-6, suggests that ATF2/Juncontributes to induction of IL-6 gene transcription rather thansustainedexpression.

We have not directly addressed the involvement of AP-1 in IL-6 expression, but we did find that PKR plays an important rolein HSV-1-induced AP-1 activation and IL-6 expression. However,indirect evidence suggests that AP-1 is not essential for IL-6production. HSV-1 activates AP-1 in baby hamster kidney cellsthrough a mechanism involving ICP0 and VP16 (16, 44). In ourhands, viruses harboring mutants in the genes encoding these proteinsexhibited unaltered ability to induce IL-6 expression. This suggeststhat AP-1 is not involved in HSV-induced IL-6production.

As to the role of C/EBP $beta$ in IL-6 expression, several studies have suggested that this transcription factor plays a centralrole in induction of many proinflammatory mediators (reviewedin reference 2). Different groups have reported that IFN- $gamma$ induces C/EBP $beta$ expression in many cell types including macrophages(36, 42). However, we were unable to demonstrate any inductionof C/EBP binding to the corresponding site in the IL-6 promoter.Although this suggests that initiation of IL-6 transcription inHSV-infected macrophages occurs independently of C/EBPs, it remainspossible that C/EBP $beta$ accumulates later after infection and/orstimulation and that the transcription factor is involved in sustainedIL-6expression.

In conclusion, the data presented here show that induction of IL-6 by HSV in leukocytes is triggered by a mechanism dependenton PKR, possibly accumulation of viral double-stranded RNA. Thecellular signaling pathways involved include notably NF- $kappa$ B anda p38-dependent pathway. Given the role of IL-6 and other proinflammatorycytokines in the host defense, this work contributes to the molecularunderstanding of the pathogenesis of HSVinfections.

	ACKNOWLEDGMENTS

The donation of mutant viruses, expression constructs, and cell lines by Bernard Roizman, Patricia G. Spear, David M. Knipe,Roger D. Everett, Chris M. Preston, Neal A. DeLuca, Paula Pitha,Helmut Holtmann, and John A. Corbett is greatlyappreciated.

This work was supported by grants from the Danish Health Science Research Council (grant number 12-1622), The Carlsberg Foundation(grant number 990803/10-911), and The Leo ResearchFoundation.

	FOOTNOTES

^* Mailing address: Department of Medical Microbiology and Immunology, The Bartholin Building, University of Aarhus, DK-8000Aarhus C, Denmark. Phone: (45) 8942 1767. Fax: (45) 8619 6128.E-mail: srp{at}microbiology.au.dk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Ace, C. I., T. A. McKee, J. M. Ryan, J. M. Cameron, and C. M. Preston. 1989. Construction and characterization of a herpes simplex virus type 1 mutant unable to transinduce immediate-early gene expression. J. Virol. 63:2260-2269[Abstract/Free Full Text].
2.	Akira, S., and T. Kishimoto. 1997. NF-IL6 and NF-kB in cytokine gene regulation. Adv. Immunol. 65:1-46[Medline].
3.	Akira, S., T. Taga, and T. Kishimoto. 1993. Interleukin-6 in biology and medicine. Adv. Immunol. 54:1-78[Medline].
4.	Ameglio, F., M. R. Capobianchi, C. Castilletti, P. Cordiali Fei, S. Fais, E. Trento, and F. Dianzani. 1994. Recombinant gp120 induces IL-10 in resting peripheral blood mononuclear cells; correlation with the induction of other cytokines. Clin. Exp. Immunol. 95:455-458[Medline].
5.	Baldwin, A. S., Jr. 1996. The NF- $kappa$ B and I $kappa$ B proteins: new discoveries and insights. Annu. Rev. Immunol. 14:649-683[CrossRef][Medline].
6.	Carlquist, J. F., L. Edelman, D. W. Bennion, and J. L. Anderson. 1999. Cytomegalovirus induction of interleukin-6 in lung fibroblasts occurs independently of active infection and involves a G protein and the transcription factor, NF- $kappa$ B. J. Infect. Dis. 197:1094-1100.
7.	Carr, D. J., and I. L. Campbell. 1999. Transgenic expression of interleukin-6 in the central nervous system confers protection against acute herpes simplex virus type-1 infection. J. Neurovirol. 5:449-457[Medline].
8.	Chomarat, P., J. Banchereau, J. Davoust, and A. K. Palucka. 2000. IL-6 switches the differentiation of monocytes from dendritic cells to macrophages. Nat. Immunol. 1:510-514[CrossRef][Medline].
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