Interferon Regulatory Factor 3 and CREB-Binding Protein/p300 Are Subunits of Double-Stranded RNA-Activated Transcription Factor DRAF1

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Mol Cell Biol, March 1998, p. 1359-1368, Vol. 18, No. 3
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Interferon Regulatory Factor 3 and CREB-Binding Protein/p300 Are Subunits of Double-Stranded RNA-Activated Transcription Factor DRAF1

Brian K. Weaver,¹^,² K. Prasanna Kumar,² and Nancy C. Reich²^,^*

Graduate Program in Molecular and Cellular Biology¹ and Department of Pathology,² State University of New York at Stony Brook, Stony Brook, New York 11794

Received 20 June 1997/Returned for modification 13 August 1997/Accepted 10 December 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Cells respond to viral infection or double-stranded RNA with the transcriptional induction of a subset of alpha/beta interferon-stimulatedgenes by a pathway distinct from the interferon signal pathway.The transcriptional induction is mediated through a DNA sequencecontaining the alpha/beta interferon-stimulated response element(ISRE). We previously identified a novel transcription factor,designated double-stranded RNA-activated factor 1 (DRAF1), thatrecognizes this response element. The DNA-binding specificityof DRAF1 correlates with transcriptional induction, thereby distinguishingit as a positive regulator of alpha/beta interferon-stimulatedgenes. Two of the components of DRAF1 have now been identifiedas interferon regulatory factor 3 (IRF-3) and the transcriptionalcoactivator CREB-binding protein (CBP)/p300. We demonstrate thatIRF-3 preexists in the cytoplasm of uninfected cells and translocatesto the nucleus following viral infection. Translocation of IRF-3is accompanied by an increase in serine and threonine phosphorylation.Coimmunoprecipitation analyses of endogenous proteins demonstratean association of IRF-3 with the transcriptional coactivatorsCBP and p300 only subsequent to infection. In addition, antibodiesto the IRF-3, CBP, and p300 molecules react with DRAF1 bound tothe ISRE target site of induced genes. The cellular response thatleads to DRAF1 activation and specific gene expression may serveto increase host survival during viral infection.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The interferon (IFN) system has evolved as a fundamental defense mechanism against viral infection. Cells respond to infectionwith the transcriptional activation of a set of antiviral genes,including the alpha/beta IFN (IFN- $alpha$ / $beta$ ) genes. Newly synthesizedIFNs are secreted and bind to cell surface receptors to conferan antiviral biological effect (reviewed in reference 13). Cellsproducing IFN have an established viral infection and thereforemay not be protected effectively by autocrine IFN. It is likelythat the critical role of IFN in the immune system is to curbviral dissemination by functioning as a paracrine cytokine. Complementarydefense mechanisms may function in a primary infected cell priorto the synthesis and action of IFN. In this report, we analyzea cellular response that may have evolved to increase host survivalduring the course of infection.

The effects of IFN- $alpha$ / $beta$ are mediated by the induction of a specific class of genes called IFN- $alpha$ / $beta$ -stimulated genes (ISGs) (reviewedin references 10, 12, 22, 28, and 44). Transcriptionalactivation of these genes is dependent on a DNA promoter sequencedesignated the IFN- $alpha$ / $beta$ -stimulated response element (ISRE). TheIFN- $alpha$ / $beta$ signal transduction pathway that leads to the inductionof these genes initiates with the activation of Janus tyrosinekinases and phosphorylation of a latent cytoplasmic transcriptionfactor, the IFN-stimulated gene factor 3 (ISGF3). ISGF3 subsequentlytranslocates to the nucleus and binds to the ISRE of induciblegenes. ISGF3 is a multimeric factor composed of members of thesignal transducer and activator of transcription factor (STAT)family, STAT1 and STAT2 (20, 43). These STATs are activatedby tyrosine phosphorylation and associate with a member of theIFN regulatory factor family, p48, to form the ISGF3 complex (50).We have identified a distinct pathway that is activated in virus-infectedcells, that is independent of IFN, and that leads to the formationof a novel ISRE-binding factor and the induction of ISGs (9,11).

Clear evidence for the direct induction of ISGs in response to viral infection was provided by studies with cells that aredeficient in autocrine IFN signaling, such as HEC-1B cells, whichcannot respond to IFNs (21, 51). Viral infection of thesecells results in the induction of a set of ISGs (2, 9, 11,36, 52-55). To begin to elucidate the mechanism by which cellsrespond to virus, we identified novel cellular DNA-binding factorsthat are activated in response to viral infection and can recognizethe ISRE (9, 11). One of the factors is activated in responseto infection by a DNA tumor virus (adenovirus), by an RNA virus(Newcastle disease virus [NDV]), or by double-stranded RNA (dsRNA).It appears that viral dsRNA produced during viral transcriptionor replication leads to the activation of this factor. Therefore,it has been designated dsRNA-activated factor 1 (DRAF1) (9).The DNA-binding characteristics of DRAF1 correlate with specificgene induction and thereby identify DRAF1 as a positive regulatorof ISG transcription independent of the action of IFN (11).

By characterizing the composition of DRAF1, we have made a major step toward understanding this response pathway. Evidenceprovided in this report identifies two of the subunits of DRAF1as IFN regulatory factor 3 (IRF-3) and the transcriptional coactivatorCREB-binding protein (CBP)/p300 (1, 7, 17; reviewed inreferences 18, 23, and 46). Both factors are present inthe DRAF1 DNA-binding complex, and the association of IRF-3 withCBP or p300 is dependent on viral infection.

	MATERIALS AND METHODS

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Cell cultures and reagents. HEC-1B cells and HeLa S3 cells (American Type Culture Collection [ATCC]) (hereafter referred to as HeLa cells) were grownin Dulbecco's modified Eagle medium (DMEM) containing 10% bovinecalf serum. HT1080 cells (ATCC) were grown in DMEM with 8% fetalbovine serum. THP-1 cells (ATCC) were grown in RPMI 1640 containing8% fetal bovine serum and 50 µM 2-mercaptoethanol. Pkr^0/0 murine embryo fibroblasts (MEFs) and Pkr^+/+ MEFs were gifts from Bryan R. G. Williams (The Cleveland ClinicFoundation, Cleveland, Ohio) and Charles Weissmann (Universityof Zurich, Zurich, Switzerland) (33, 57) and were grown inDMEM containing 10% fetal bovine serum and supplemented with nonessentialamino acids. Recombinant human alpha IFN (IFN- $alpha$ ) was providedby Hoffmann-La Roche Inc. (Nutley, N.J.) and was used at 1,000U/ml. N-Ethylmaleimide (NEM) was obtained from Sigma. Proteinphosphatase type 2A (PP2A) and okadaic acid were obtained fromUpstate Biotechnology Inc. Recombinant protein tyrosine phosphatase1B (PTP1B) was provided by Nicholas K. Tonks (Cold Spring HarborLaboratory, Cold Spring Harbor, N.Y.). Phosphoamino acid standards(phosphoserine, phosphothreonine, and phosphotyrosine) were obtainedfrom Sigma. Thin-layer cellulose chromatography (TLC) plates wereobtained from VWR Scientific. Prestained and unstained proteinmolecular weight standards were obtained from Gibco BRL. Unstainedmolecular weight standards were used for mass estimation of proteins.Anti-glutathione S-transferase (GST) antibodies, anti-CBP antibodies(A-22), anti-p300 antibodies (N-15), and specific blocking peptideswere purchased from Santa Cruz Biotechnology Inc. dsRNA treatmentwas performed with poly(rI) · poly(rC) (Pharmacia) and with serum-freemedia.

Plasmid constructs. Reverse transcription-PCR of THP-1 cell cytoplasmic RNA was used to amplify a 303-bp fragment corresponding to amino acids107 to 208 of the human IRF-3 protein (1). This cDNA fragmentwas subcloned into bacterial expression plasmid pGEX2T (Pharmacia),and GST fusion proteins were used for immunization of rabbitsand mice. A full-length human IRF-3 cDNA was generated by reversetranscription-PCR with primers corresponding to the 5' and 3'untranslated regions of the gene. The coding sequence of the IRF-3cDNA was subcloned into pGEX2TK (Pharmacia), and the resultingGST-IRF-3 recombinant gene was cloned into pCDNA3. This plasmidwas stably expressed in HT1080 cells (HT1080/GST-IRF-3 cells).The expressed GST-IRF-3 molecule and associated proteins wereisolated by binding to glutathione beads (Pharmacia) for 20 minat 4°C, followed by washing in detergent-containing buffer priorto protein elution.

Viral infections. NDV, a gift from Paula M. Pitha-Rowe (The Johns Hopkins University, Baltimore, Md.), was propagated in the allantoic cavitiesof 10-day-old embryonated hen eggs. Viral titers were determinedby hemagglutination of chicken erythrocytes. Viral infectionswere performed as described previously (11). Briefly, cellswere washed with serum-free media and then overlaid with 5 mlof serum-free media containing NDV at 100 hemagglutination unitsper ml. After 1 h, the cells were fed media containing serum.Mock infections were performed with allantoic fluid from uninfectedhen eggs.

Immunoassays. Protein extracts were prepared by fractionation of cells with a Dounce homogenizer under hypotonic conditions, followed bypreparation of nuclear and cytoplasmic extracts as described previously(14, 42). Alternatively, whole-cell extracts were preparedby lysing cells on ice in buffer containing 50 mM Tris (pH 7.6),400 mM NaCl, 0.5% Nonidet P-40, 5 mM potassium EDTA, 1 mM EGTA,10 mM sodium phosphate (pH 7.2), 50 mM sodium fluoride, and 2mM sodium vanadate. The insoluble material was removed by centrifugationat 12,000 × g and 4°C. All extracts were prepared in the presenceof 1 mM phenylmethylsulfonyl fluoride (Sigma) and 1 µg each ofleupeptin, pepstatin A, and aprotinin (Boehringer Mannheim Biochemicals)per ml.

Immunoprecipitations were performed by incubating extracts with an excess of antibody to IRF-3 or control antibody for 4 hat 4°C. Immunocomplexes were bound to protein G-agarose (GibcoBRL), washed, separated by sodium dodecyl sulfate (SDS)-polyacrylamidegel electrophoresis (PAGE), and electroblotted to an Immobilon-Ptransfer membrane (Millipore). Proteins were detected by immunoblottingwith primary antibody, followed by anti-mouse or anti-rabbit secondaryantibody (Amersham) and enhanced chemiluminescence reagents (DuPontNEN).

DNA-binding assays. Protein extracts were analyzed for specific ISRE-binding proteins by two methods. The first was an electrophoretic mobilityshift assay (EMSA) done as described previously (9, 11).Nuclear extracts were incubated with a ³²P-labeled oligonucleotide probe containing the human ISG15 ISRE(41) for 20 min at room temperature. The effects of specificantibodies were tested by incubation with nuclear extracts at4°C for 60 min prior to the addition of the probe.

Alternatively, specific ISRE-binding proteins were detected by incubation with ISRE-Sepharose beads, followed by SDS-PAGEand immunoblotting. Briefly, an ISG15 double-stranded oligonucleotidecontaining the ISRE (5'-GGGAAAGGGAAACCGAAACTGAA-3') (ISRE in italictype) or a mutated double-stranded oligonucleotide (5'-GGGAAAGGGAAACCCAAACTGAA-3')(mutation in boldface type) (9) was multimerized and coupledto CNBr-activated Sepharose 4B (Pharmacia). Approximately 5.0mg of total cellular protein, isolated by Dounce homogenizationand extraction, was incubated with ISRE-Sepharose in the presenceof 100 µg of nonspecific plasmid DNA and 50 µg of salmon spermDNA (Pharmacia) at 4°C. The affinity beads were collected by centrifugationand washed, and bound proteins were separated by SDS-PAGE, followedby immunoblotting with antibody to IRF-3.

Protein phosphatase and alkylation treatments. Nuclear extracts were treated in vitro with recombinant PTP1B at 37°C for 1 h in buffer containing 25 mM HEPES (pH 7.0) and0.2% 2-mercaptoethanol (Sigma). PTP1B was inhibited by the inclusionof 5 mM sodium vanadate prior to incubation. Nuclear extractswere treated in vitro with PP2A by incubation at 30°C for 1 hin buffer containing 50 mM Tris (pH 7.0), 0.1 mM CaCl₂, and 1mM MnCl₂. PP2A was inhibited by the inclusion of 10 nM okadaicacid prior to incubation. For protein alkylation, nuclear extractswere incubated in the absence or presence of 10 mM NEM for 30min at room temperature, and then dithiothreitol was added to10 mM to inactivate any of the remaining NEM.

Metabolic labeling and phosphoamino acid analysis. For ³²P metabolic labeling, cells were incubated with 250 µCi of [³²P]orthophosphate (DuPont NEN) per ml in phosphate-free media andinfected with NDV or mock infected. The time of NDV infectionwas varied, while the total time of metabolic labeling for eachsample was kept constant. Whole-cell extracts were prepared bydetergent lysis, normalized for equivalent trichloroacetic acid-precipitablecounts, and subjected to immunoprecipitation with either controlantibody or antibody to IRF-3. SDS-PAGE gels were either fixedand dried or electroblotted to Immobilon-P membranes and exposedto film. Labeling with [³⁵S]methionine-[³⁵S]cysteine (DuPont NEN) at 160 µCi/ml was performed with methionine-and cysteine-free media. Detergent cell lysates were normalizedfor protein prior to analysis. Gels were treated with En³Hance (DuPont NEN) prior to exposure to film.

For phosphoamino acid analysis, the ³²P-labeled IRF-3 and adjacent areas from control gels were excised from membranes and subjectedto hydrolysis in 5.7 N HCl at 110°C as described previously (6,8). Phosphoamino acids were identified by two-dimensional electrophoresisat pH 3.5 and pH 1.9 on a TLC plate as described previously (6,8). Unlabeled phosphoamino acid internal standards were detectedwith ninhydrin staining. Radioactive bands were quantified witha PhosphorImager (445 SI; Molecular Dynamics).

	RESULTS

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Activation of DRAF1 by NDV infection. Cells respond to viral infection with the activation of ISGs by two distinct mechanisms. One mechanism involves the actionof IFN- $alpha$ / $beta$ cytokines produced by virus-infected cells. As previouslydescribed, stimulation of HeLa cells with IFN- $alpha$ induces the appearanceof the ISGF3 transcription factor. This induction is shown byan EMSA with a radiolabeled ISRE probe (Fig. 1, lane 2). Infectionof HeLa cells with NDV, a paramyxovirus that produces dsRNA duringthe course of infection, activates two ISRE-binding transcriptionfactors: IFN- $alpha$ / $beta$ -induced ISGF3 and a novel factor, DRAF1 (Fig.1, lane 5) (9, 11). ISGF3 activation in HeLa cells in responseto NDV infection is due to autocrine IFN production. This becomesevident by NDV infection of cells unable to respond to IFN (HEC-1Bcells) (21, 52). In IFN-unresponsive HEC-1B cells, DRAF1 isinduced following viral infection, but ISGF3 is not (Fig. 1, lane8). We showed previously that the appearance of DRAF1 precedesthe appearance of ISGF3 in cells that respond to autocrine IFNand thereby DRAF1 functions as a direct response to virus (9,11).

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FIG. 1. Activation of ISRE-binding factors by IFN- $alpha$ and NDV. HeLa cells were either untreated (control [c]; lanes 1 and 4), treated with IFN- $alpha$ for 1 h (lanes 2 and 3), or infected with NDV for 3 h (lanes 5 and 6). HEC-1B cells were either untreated (lane 7) or infected with NDV for 3 h (lanes 8 and 9). Nuclear extracts were prepared and analyzed by an EMSA with a radiolabeled ISRE probe. The specificity of the protein-DNA complexes was shown by competition with a 100-fold excess of unlabeled ISRE oligonucleotide (lanes 3, 6, and 9).

DRAF1 is sensitive to phosphatase and alkylation. The activation of DRAF1 requires the function of a protein kinase, since the appearance of DRAF1 is blocked by the kinaseinhibitors genistein and staurosporine (9). To determine whetherDRAF1 is phosphorylated on tyrosine, the effect of PTP1B on DRAF1was examined by an EMSA (Fig. 2A). Nuclear extracts were preparedfrom uninfected or NDV-infected HEC-1B cells and incubated invitro with PTP1B prior to DNA binding. DRAF1 was apparent in extractsfrom NDV-infected cells (Fig. 2A, lane 2) but was completely abrogatedby treatment with PTP1B (lane 3). The effect was inhibited bythe addition of sodium vanadate, a specific inhibitor of tyrosinephosphatases (Fig. 2A, lane 4). This result suggests that DRAF1is tyrosine phosphorylated and that this modification is requiredfor its ability to bind to DNA. Since the STAT family also requirestyrosine phosphorylation for DNA binding, we tested the effectsof specific antibodies to STAT1, STAT2, STAT3, STAT5, and STAT6on the appearance of DRAF1 in an EMSA, but they had no effect(data not shown).

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FIG. 2. (A) Effect of a protein tyrosine phosphatase (PTP) on DRAF1. HEC-1B nuclear extracts from untreated cells (lane 1) or cells infected with NDV (lanes 2 to 4) were used in an EMSA with a radiolabeled ISRE probe. Prior to the DNA-binding reaction, the extracts were incubated in the absence (lanes 1 and 2) or in the presence (lanes 3 and 4) of recombinant PTP1B. Tyrosine phosphatase activity was inhibited by the inclusion of 5 mM sodium vanadate (van) (lane 4). (B) Effect of a serine/threonine protein phosphatase on DRAF1. HEC-1B nuclear extracts from untreated cells (lane 1) or cells infected with NDV (lanes 2 to 4) were used in an EMSA. Prior to the DNA-binding reaction, the extracts were incubated in the absence (lanes 1 and 2) or in the presence (lanes 3 and 4) of PP2A. Protein phosphatase activity was inhibited by the inclusion of 10 nM okadaic acid (OA) (lane 4). (C) Effect of protein alkylation on the appearance of DRAF1. HEC-1B nuclear extracts from untreated cells (lane 1) or cells infected with NDV (lanes 2 and 3) were used in an EMSA. Prior to the DNA-binding reaction, the extracts were either untreated (lanes 1 and 2) or treated with 10 mM NEM (lane 3).

A similar analysis was performed to examine the role of serine or threonine phosphorylation on DRAF1 activity (Fig. 2B). Nuclearextracts containing DRAF1 were incubated in the presence of PP2A,a serine- and threonine-specific protein phosphatase, before theEMSA. DRAF1 activity was partially reduced after dephosphorylationwith PP2A (Fig. 2B, compare lanes 2 and 3). This effect was inhibitedby the addition of okadaic acid, a specific inhibitor of PP2A(Fig. 2B, lane 4).

Although DRAF1 is similar to ISGF3 in its ability to bind to an ISRE-like target, DRAF1 does not contain the DNA-binding subunitof ISGF3, p48 (or ISGF3 $gamma$ ) (9). The p48 protein belongs to theIRF family of DNA-binding proteins (38, 40, 47, 50). Acharacteristic of IRF proteins is their sensitivity to alkylationwith NEM (34). To test whether DRAF1 is also sensitive to alkylation,nuclear extracts containing DRAF1 were treated with NEM and thenanalyzed by an EMSA (Fig. 2C). The NEM treatment completely abrogatedthe DNA-binding activity of DRAF1, indicating that DRAF1 DNA bindingis sensitive to alkylation with NEM (Fig. 2C, lane 3).

Antibodies to IRF-3 react with DRAF1. Recently, several new members of the IRF family of proteins were identified. This family now includes p48, IRF-1, IRF-2, IRF-3,ICSBP, ICSAT/Pip/LSIRF/IRF-4, IRF-5 (EMBL accession number U51127),IRF-6 (EMBL accession number U73029), and IRF-7 (1, 16,19, 23a, 25, 35, 38, 40, 50, 56, 59). Severalcharacteristics of IRF-3 made it a candidate subunit of DRAF1.Overexpression of IRF-3 was reported to activate the expressionof a reporter gene driven by an ISG promoter (1). In addition,IRF-3 is constitutively expressed in all cell types tested, whereasthe expression of some of the IRF proteins is cell type restrictedor is seen only following IFN stimulation (1). This ubiquitouspattern of IRF-3 expression is in accord with DRAF1 activationin a variety of cell types.

To determine whether DRAF1 contains IRF-3, the effect of a specific antibody generated against IRF-3 was tested (Fig. 3A).The immunogen used to produce the antibody corresponded to a uniqueregion of IRF-3 that shares only three contiguous amino acidswith other IRF proteins. The specific antibody does not cross-reactwith heterologous IRFs, such as p48, IRF-1, or IRF-2 (data notshown). Nuclear extracts were prepared from HEC-1B cells thatwere either untreated or infected with NDV. The nuclear extractswere incubated in the absence of added antibody (Fig. 3A, lanes1 and 4), in the presence of control antibody (lanes 2 and 5),or in the presence of specific anti-IRF-3 antibody (lanes 3 and6), and DRAF1 was subsequently analyzed by an EMSA. The additionof control antibody had no effect on DRAF1 (Fig. 3A, lane 5),while the specific anti-IRF-3 antibody completely abrogated itsappearance (lane 6). The inclusion of a GST-IRF-3 fusion proteinin the DNA-binding reaction could reverse the effect of the anti-IRF-3antibody on the DRAF1 complex (Fig. 3B, lanes 5 and 6), but aGST-p48 fusion protein had no effect (lane 7). In addition, thedepletion of IRF-3 from nuclear extracts by immunoprecipitationalso depleted DRAF1 activity (data not shown). These results indicatethat IRF-3 is a subunit of DRAF1.

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FIG. 3. (A) Effect of antibody to IRF-3 on DRAF1. Nuclear extracts from untreated HEC-1B cells (lanes 1 to 3) or cells infected with NDV (lanes 4 to 6) were used in an EMSA with a radiolabeled ISRE probe. Prior to the addition of the probe, either no antisera (Ab) (lanes 1 and 4), control murine antisera (c) (1:50 dilution) (lanes 2 and 5), or specific murine antisera to IRF-3 (1:50 dilution) (lanes 3 and 6) were added to the DNA-binding reaction mixtures. (B) Inhibition by GST-IRF-3 fusion protein of anti-IRF-3 antibody effects. Nuclear extracts from untreated HEC-1B cells (lane 1) or cells infected with NDV (lanes 2 to 7) were used in an EMSA. Prior to the addition of the probe, either 1 µg of control rabbit antibody (Ab) (lane 3) or 1 µg of rabbit antibody to IRF-3 (lanes 4 to 7) was added. Antibody incubation was done in the absence of added GST fusion protein (lanes 3 and 4), in the presence of 200 ng (lane 5) and 600 ng (lane 6) of GST-IRF-3 (amino acids 107 to 208), or in the presence of 200 ng of GST-p48 (amino acids 103 to 225) (lane 7). (C) Effect of NDV infection on the ability of IRF-3 to bind to the ISRE. Whole-cell extracts were prepared from HEC-1B cells that were either untreated (lanes 1 and 3) or infected with NDV for 6 h (lanes 2 and 4). The extracts were incubated with ISRE-Sepharose beads (lanes 1 and 2) or with rabbit antibody to IRF-3 (lanes 3 and 4). The bound proteins were separated by SDS-PAGE and detected by immunoblotting (IB) with a murine antibody ( $alpha$ ) to IRF-3. IP, immunoprecipitation. Positions of prestained molecular mass standards are shown in kilodaltons on the left.

Partial purification of DRAF1 and UV cross-linking to DNA previously had revealed a DNA-binding component of approximately60 to 70 kDa (11). To determine if IRF-3 could be this DNA-bindingsubunit, we tested the binding of IRF-3 to the ISRE either beforeor after NDV infection by use of an immobilized ISRE affinityresin (Fig. 3C). Cytoplasmic and nuclear protein extracts wereprepared and combined to represent total cellular protein. Cellswere either untreated or infected with NDV, and extracts wereincubated with ISRE-Sepharose beads. Proteins bound to ISRE-Sepharosewere analyzed by SDS-PAGE and immunoblotting with antibody toIRF-3. The results indicated that IRF-3 was capable of bindingto ISRE-Sepharose only after infection with virus (Fig. 3C, lane2). This difference in binding capability was not due to differentlevels of IRF-3 in the two extracts, since a control immunoprecipitationshowed equivalent levels of IRF-3 protein (Fig. 3C, lanes 3 and4). An increase in the apparent molecular mass of IRF-3 was alsonoted following NDV infection. IRF-3 isolated from untreated cellsmigrated in SDS-PAGE with a molecular mass of approximately 62kDa and shifted to approximately 64 kDa after infection.

IRF-3 exists in the cytoplasm and translocates to the nucleus following viral infection. We previously demonstrated that DRAF1 activation occurs in the absence of new protein synthesis (9). Proteins comprisingDRAF1 must therefore preexist within the cell. To determine IRF-3cellular localization, cytoplasmic and nuclear extracts were preparedfrom HEC-1B cells that were either untreated or infected withNDV. The protein extracts were normalized for cell equivalentsand assayed for IRF-3 by immunoprecipitation and immunoblotting(Fig. 4A). In uninfected cells, IRF-3 was found entirely in thecytosolic fraction (Fig. 4A, compare lanes 2 and 6). However,after viral infection, IRF-3 could be detected in the nuclearfraction, indicating that a nuclear translocation event had takenplace (Fig. 4A, lane 8). The same cytoplasm-to-nucleus translocationcould be seen with a GST-IRF-3 fusion protein stably expressedin cells (Fig. 4B). Following infection, the endogenous IRF-3protein or the transfected GST-IRF-3 protein displayed slowermigration in SDS-PAGE. The modification responsible for the alterationin migration appears to be a prerequisite for IRF-3 translocationto the nucleus and subsequent DNA binding.

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FIG. 4. (A) Cellular localization of IRF-3 in control and virus-infected cells. Nuclear and cytoplasmic extracts were prepared from untreated HEC-1B cells (lanes 1, 2, 5, and 6) or cells infected with NDV for 6 h (lanes 3, 4, 7, and 8). Extracts were normalized for cell equivalents and subjected to immunoprecipitation (IP) with control rabbit antibody (c) (lanes 1, 3, 5, and 7) or rabbit antibody to IRF-3 (lanes 2, 4, 6, and 8). The immunoprecipitated proteins were separated by SDS-PAGE and detected by immunoblotting (IB) with a murine antibody ( $alpha$ ) to IRF-3. Numbers at left are in kilodaltons. (B) Cellular localization of a transfected GST-IRF-3 chimera. Nuclear (nuc) and cytoplasmic (cyto) extracts were prepared from untreated HT1080/GST-IRF-3 cells (lanes 1 and 2) or cells infected with NDV for 6 h (lanes 3 and 4). Extracts were normalized for cell equivalents and subjected to immunoprecipitation with a rabbit antibody to IRF-3. The immunoprecipitated proteins were separated by SDS-PAGE and detected by immunoblotting (IB) with a murine antibody ( $alpha$ ) to IRF-3 (upper panel). The blot was subsequently stripped and reprobed with a rabbit antibody ( $alpha$ ) to GST (lower panel).

Serine phosphorylation of IRF-3 increases following NDV infection. A possible modification that could cause IRF-3 to exhibit slower migration in SDS-PAGE after viral infection is phosphorylation.To analyze the phosphorylation state of IRF-3, HEC-1B cells werelabeled with [³²P]orthophosphate during either mock infection or infection withNDV (Fig. 5A). Whole-cell lysates were prepared and subjectedto immunoprecipitation with either a control antibody (Fig. 5A,lanes 1, 3, and 5) or antibody to IRF-3 (lanes 2, 4, and 6). Inthe absence of viral infection, IRF-3 was modified by phosphorylationat a low level (Fig. 5A, lane 2). At 3 h postinfection, the levelof IRF-3 phosphorylation increased 1.5-fold (Fig. 5A, lane 4),and after 6 h, the phosphorylation level increased approximately3-fold over the basal level (lane 6). Since the relative levelsof IRF-3 were the same (Fig. 5A, lower panel), the results indicatedthat IRF-3 protein phosphorylation increased. This finding correlateswith the characteristic slower migration.

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FIG. 5. (A) Increase in IRF-3 phosphorylation during viral infection. Whole-cell extracts were prepared by detergent lysis of HEC-1B cells that were metabolically labeled with [³²P]orthophosphate for a total of 7 h during either mock infection (0 h) (lanes 1 and 2) or infection with NDV for 3 h (lanes 3 and 4) or 6 h (lanes 5 and 6). Extracts were subjected to immunoprecipitation (IP) with a control murine antibody (c) (lanes 1, 3, and 5) or a murine anti-IRF-3 antibody (lanes 2, 4, and 6). Immunoprecipitated proteins were denatured in SDS sample buffer, and 75% of the sample was separated by SDS-PAGE. The gel was fixed, dried, and exposed to film (upper panel). The remaining 25% was analyzed by SDS-PAGE and immunoblotting (IB) with a rabbit polyclonal antibody ( $alpha$ ) to IRF-3 (lower panel). The positions of the prestained molecular mass standards are shown in kilodaltons on the left. (B) Effect of protein phosphatase treatment on the migration of IRF-3 in SDS-PAGE. Cytoplasmic (C) and nuclear (N) extracts were prepared from HEC-1B cells that were either untreated (lanes 1 and 2) or infected with NDV (lanes 3 to 7). A total of 100 µg of cytoplasmic extract or 35 µg of nuclear extract was incubated in the absence of phosphatase (lanes 1 to 3), in the presence of PP2A (lanes 4 and 5), or in the presence of PTP1B (PTP) (lanes 6 and 7). The activities of PP2A and PTP1B were inhibited by the inclusion of 10 nM okadaic acid (OA) (lane 5) and 5 mM sodium vanadate (van) (lane 7), respectively. Proteins were separated by SDS-PAGE and detected by immunoblotting (IB) with a murine antibody ( $alpha$ ) to IRF-3. (C) Phosphoamino acid analysis of ³²P-labeled IRF-3. Cells were metabolically labeled with [³²P]orthophosphate, and lysates from mock-infected cells (upper panels) or NDV-infected cells (lower panels) were immunoprecipitated (IP) with control (c) antibody (boxes 1 and 3) or antibody to IRF-3 (boxes 2 and 4). Following SDS-PAGE, proteins were electroblotted to Immobilon-P membranes, and the area containing IRF-3 or the adjacent area from control immunoprecipitations was subjected to partial acid hydrolysis. The hydrolysates were resolved by two-dimensional electrophoresis on a TLC plate. Positions of the serine, threonine, and tyrosine phosphoamino acid internal standards are indicated by dotted circles (pS, pT, and pY, respectively), and origins are denoted by a plus sign.

To determine the type of amino acid phosphorylation of IRF-3 after viral infection, the effects of protein phosphatases wereevaluated (Fig. 5B). Extracts were prepared from untreated orinfected HEC-1B cells and incubated in the absence or presenceof protein phosphatases to analyze IRF-3 migration. CytoplasmicIRF-3 from control cells migrated at its normal position (Fig.5B, lane 1). Nuclear extracts from control cells contained nodetectable IRF-3 (Fig. 5B, lane 2). Following viral infection,IRF-3 with the characteristic slower migration appeared in nuclearextracts (Fig. 5B, lane 3). Treatment of nuclear IRF-3 with aserine- and threonine-specific phosphatase, PP2A, resulted ina return of IRF-3 to its original migration position prior toinfection (Fig. 5B, lane 4). This result was specific for PP2Aactivity, since inclusion of okadaic acid inhibited the effect(Fig. 5B, lane 5). In contrast, treatment of nuclear IRF-3 witha tyrosine phosphatase, PTP1B, had no effect on the migrationof IRF-3 (Fig. 5B, lane 6). This result indicates that IRF-3 undergoesan increase in serine and/or threonine phosphorylation after viralinfection that is responsible for the reduction in the relativemigration observed in SDS-PAGE.

Since treatment of DRAF1 with PTP1B inhibits its ability to bind to DNA (Fig. 2A), it remained possible that IRF-3 was modifiedby tyrosine phosphorylation. To further investigate the type ofphosphorylation modifying IRF-3, we performed a phosphoamino acidanalysis (Fig. 5C). HEC-1B cells were metabolically labeled with[³²P]orthophosphate during either mock infection or infection withNDV. Whole-cell lysates were subjected to immunoprecipitation,SDS-PAGE, and electroblotting to an Immobilon-P membrane. The³²P-labeled IRF-3 protein was excised from the membrane, as wasthe adjacent area from the control immunoprecipitation. Proteinsfrom the four membrane pieces were subjected to partial acid hydrolysisfor various times, and the products were separated by two-dimensionalTLC. A representative TLC autoradiogram is shown in Fig. 5C. IRF-3immunoprecipitated from mock-infected cells clearly showed thepresence of phosphoserine (Fig. 5C, box 2). Following NDV infection,the amount of phosphoserine in IRF-3 increased and the presenceof phosphothreonine was also detected (Fig. 5C, box 4). The phosphoserinecontent of IRF-3 appeared to increase after infection by approximatelythreefold, consistent with the increase in phosphate incorporationin IRF-3 revealed by immunoprecipitation (Fig. 5A). No phosphotyrosinewas detected in IRF-3 either before or after viral infection.

Activation of DRAF1 in PKR-deficient cells. Since serine phosphorylation is involved in the modification of IRF-3 and DRAF1 in response to virus or dsRNA, the functionof a dsRNA-activated kinase is indicated. For this reason, a potentialrole of the dsRNA-dependent protein kinase (PKR) in this signalpathway was evaluated. PKR is a serine and threonine protein kinasethat becomes activated by binding to dsRNA (reviewed in references27 and 29). It has been identified as a signal-transducingkinase in the activation of transcription factor NF- $kappa$ B and hasbeen implicated in IFN induction, the antiviral response, andthe regulation of cell growth (30, 32, 33, 37, 57).

To determine whether PKR functions in the activation of IRF-3 and DRAF1, cells lacking PKR were tested for DRAF1 induction.Mice deficient in functional PKR (Pkr^0/0) were generated by targeted gene disruption (57). MEFs derivedfrom these mice (Pkr^0/0) and from parental wild-type mice (Pkr^+/+) were infected with NDV. Nuclear extracts were prepared and assayedfor the appearance of DRAF1 activity by an EMSA (Fig. 6). BothDRAF1 and ISGF3 were activated in the Pkr^+/+ and Pkr^0/0 MEFs following NDV infection and, more significantly, the levelswere similar in both cell types. The ISGF3 activity was likelydue to autocrine IFN production during viral infection. Theseresults suggest that PKR is not required for DRAF1 formation andbinding to the ISRE.

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FIG. 6. Activation of DRAF1 in Pkr^0/0 MEFs. Wild-type (Pkr^+/+) MEFs or PKR-deficient (Pkr^0/0) MEFs were either untreated (lanes 1 and 4) or infected with NDV for 3 h (lanes 2, 3, 5, and 6). Nuclear extracts were prepared and analyzed by an EMSA with a radiolabeled ISRE probe. The specificity of the protein-DNA complexes was shown by competition with a 100-fold excess of unlabeled ISRE oligonucleotide (lanes 3 and 6).

Association of IRF-3 with CBP and p300 following viral infection. A previous study indicated that IRF-3 did not function as an independent transcriptional activator (1). The DNA-bindingdomain of a heterologous protein (GAL4) was fused to IRF-3, andthe chimera was tested for GAL4-targeted gene expression afterviral infection. The GAL4-IRF-3 fusion protein did not activatetranscription, suggesting that IRF-3 may interact with other factorsto elicit gene regulation. For this reason, we analyzed the abilityof IRF-3 to physically interact with other cellular proteins followingviral infection.

Untreated or NDV-infected HEC-1B cells were metabolically labeled with [³⁵S]methionine-[³⁵S]cysteine, and extracts were analyzed for proteins that coimmunoprecipitatedwith IRF-3 (Fig. 7A). Following viral infection, a prominent radiolabeledband with an apparent molecular mass of approximately 300 kDacoimmunoprecipitated with IRF-3 (Fig. 7A, lane 4). The coimmunoprecipitatedprotein was not present in control antibody immunocomplexes (Fig.7A, lanes 1 and 3) or in uninfected cells (lane 2). To establishthat the coimmunoprecipitated protein was of cellular origin andwas also present in other cells, an analysis was performed withHeLa cells (Fig. 7B). HeLa cells were either treated with dsRNAor infected with NDV and metabolically labeled with [³⁵S]methionine-[³⁵S]cysteine. Immunoprecipitations with anti-IRF-3 antibody againdemonstrated a coimmunoprecipitated protein of approximately 300kDa only following dsRNA treatment or viral infection (Fig. 7B,lanes 4 and 8). The same result was obtained following infectionwith dl312 adenovirus (data not shown).

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FIG. 7. (A) Association of IRF-3 with a 300-kDa cellular protein following HEC-1B cell infection with NDV. Detergent cell lysates were prepared from cells following metabolic labeling with [³⁵S]methionine-[³⁵S]cysteine during either mock infection (lanes 1 and 2) or infection with NDV for 6 h (lanes 3 and 4). Extracts were subjected to immunoprecipitation (IP) with a control rabbit antibody (c) (lanes 1 and 3) or a rabbit anti-IRF-3 antibody (lanes 2 and 4). The immunoprecipitated proteins were separated by SDS-PAGE and detected by fluorography. The positions of the prestained molecular mass standards are shown in kilodaltons on the left. (B) Presence in HeLa cells treated with dsRNA or infected with NDV of a 300-kDa cellular protein associated with IRF-3. Detergent cell lysates were prepared from cells that were metabolically labeled with [³⁵S]methionine-[³⁵S]cysteine. Cells were untreated (lanes 1 and 2), treated with 150 µg of poly(rI) · poly(rC) per ml for 2 h (lanes 3 and 4), mock infected (lanes 5 and 6), or infected with NDV for 6 h (lanes 7 and 8). The immunoprecipitation analysis was performed as described in panel A. (C) Association of the IRF-3-associated 300-kDa protein with the ISRE following virus infection. Whole-cell extracts were prepared from HEC-1B cells that were metabolically labeled with [³⁵S]methionine-[³⁵S]cysteine and either mock infected (lanes 1 and 2) or infected with NDV for 6 h (lanes 3 and 4). The extracts were incubated with DNA-Sepharose beads prepared with native ISRE (wt) (lanes 2 and 4) or with a mutated ISRE (mt) (lanes 1 and 3). The DNA-bound proteins were detected as described in panel A. (D) Copurification of the 300-kDa protein with stably expressed GST-IRF-3 fusion protein. Detergent cell lysates were prepared from HT1080/GST-IRF-3 cells that were metabolically labeled with [³⁵S]methionine-[³⁵S]cysteine and either mock infected (lane 1) or infected with NDV for 6 h (lane 2). Extracts were incubated with glutathione-agarose beads and washed, and bound proteins were separated and detected as described in panel A. Asterisks indicate migration of 300-kDa proteins.

Association of the 300-kDa cellular protein with IRF-3 could also be demonstrated with techniques that did not depend on aspecific immunoprecipitating antibody. The presence of the 300-kDaprotein in ISRE-DNA complexes was seen with the use of an immobilizedISRE affinity resin (as performed with IRF-3 in Fig. 3) (Fig.7C). Cell lysates were prepared from control or NDV-infected cellsmetabolically labeled with [³⁵S]methionine-[³⁵S]cysteine, and proteins were incubated with either a native ISREoligonucleotide linked to Sepharose beads or a mutated ISRE oligonucleotidelinked to the beads. The IRF-3-associated 300-kDa protein wasfound in DNA complexes only with the native ISRE sequence andonly following viral infection (Fig. 7C, lane 4). In addition,a GST-IRF-3 fusion protein stably expressed in HT1080 cells wastested for its ability to associate with the 300-kDa cellularprotein (Fig. 7D). Cells expressing GST-IRF-3 were metabolicallylabeled with [³⁵S]methionine-[³⁵S]cysteine before or after infection. Cell lysates were prepared,and radiolabeled GST-IRF-3 was collected on glutathione beads.Analysis by SDS-PAGE demonstrated an association of the 300-kDaprotein with GST-IRF-3 only following viral infection (Fig. 7C,lane 2).

The molecular mass of the protein associated with IRF-3 prompted us to investigate the possibility of its identity with thetranscriptional coactivators CBP and p300 (Fig. 8) (7, 17).An immunoprecipitation-immunoblotting assay was performed withcontrol HEC-1B cells or cells infected with NDV (Fig. 8A). Proteinsin the immunocomplexes with anti-IRF-3 antibody were separatedby SDS-PAGE, transferred to an Immobilon-P membrane, and immunoblottedwith antibodies to CBP and p300. Antibodies to CBP and p300 reactedwith the coimmunoprecipitated protein following viral infection(Fig. 8A, lane 2). In addition to a prominent CBP/p300 proteinband, there were several smaller reactive species. These may correspondto cleavage products that transfer more efficiently to the Immobilon-Pmembrane than the larger native molecules. The results demonstrateda physical interaction of IRF-3 with CBP and/or p300 followingviral infection that is of sufficient affinity to resist detergentlysis of cells and standard immunoprecipitation techniques.

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FIG. 8. (A) Identification of the IRF-3-associated protein as CBP/p300. Detergent cell lysates were prepared from HEC-1B cells that were either mock infected (lane 1) or infected with NDV for 6 h (lane 2). Extracts were subjected to immunoprecipitation with rabbit anti-IRF-3 antibody ( $alpha$ ). Immunoprecipitated proteins were separated by SDS-PAGE and detected by immunoblotting (IB) with a mixture of specific rabbit antibodies to p300 and CBP (upper panel) or with a murine antibody to IRF-3 (lower panel). Numbers at left are in kilodaltons. (B) Presence of CBP and p300 in the DRAF1 complex. Nuclear extracts from untreated HEC-1B cells (lane 1) or cells infected with NDV (lanes 2 to 10) were used in an EMSA with a radiolabeled ISRE probe. Prior to the addition of the probe, no antibody (Ab) (lanes 1 and 2), 2 µg of control rabbit antibody (c) (lane 3), 2 µg of specific rabbit antibody to IRF-3 (lane 4), 2 µg of specific rabbit antibody to p300 (lanes 5 and 8), 2 µg of specific rabbit antibody to CBP (lanes 6 and 9), or 1 µg of antibodies to both p300 and CBP (lanes 7 and 10) was added to the DNA-binding reaction mixtures. The effect of the anti-p300 and anti-CBP antibodies was blocked by the inclusion of 0.2 µg of control peptide(s) used as an immunogen to generate the antibodies (lanes 8 to 10).

To determine if the CBP and p300 molecules were associated with IRF-3 in the DRAF1 DNA-binding complex, the effects of specificantibodies to either CBP or p300 were evaluated (Fig. 8B). Nuclearextracts were prepared from uninfected or infected cells and usedin an EMSA with the radiolabeled ISRE probe to display the DRAF1complex. Antibodies were added to the DNA-binding reaction mixtureto evaluate their ability to supershift or inhibit the appearanceof DRAF1. Specific antibodies to either p300 or CBP partiallyinhibited the appearance of DRAF1 (Fig. 8B, lanes 5 and 6), andinclusion of both anti-CBP and anti-p300 antibodies to the bindingreaction mixture completely eliminated the appearance of DRAF1(lane 7). Similar amounts of control antibodies had no effecton DRAF1 (Fig. 8B, lane 3), and as previously demonstrated, anti-IRF-3antibodies completely eliminated the appearance of DRAF1 (lane4). These results confirm the presence of CBP, p300, and IRF-3in the DRAF1 ISRE-binding complex and appear to indicate thateither of the related molecules CBP and p300 can associate withIRF-3 following infection.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The cellular response to viral infection appears to result in the transcriptional induction of the IFN- $alpha$ / $beta$ genes and in thedirect induction of a subset of the ISGs (2, 9, 11, 36,52-55). Viral induction of the ISGs is not dependent on autocrineIFN, since it can be seen in cells deficient in the response toIFN, such as HEC-1B cells (21, 51). We provided evidence previouslythat viral activation of a specific ISRE-binding factor, DRAF1,leads to the transcriptional induction of specific ISGs (9,11). The activation of DRAF1 may be a general response to invadingvirus, since both a DNA virus (adenovirus) and an RNA virus (NDV)as well as dsRNA can activate DRAF1 (9, 11). Viral dsRNAappears to be generated during viral transcription or replicationand to act as a mediator of DRAF1 activation. DRAF1 may functionto activate antiviral genes, antiproliferative genes, and/or apoptosis.Since the appearance of DRAF1 precedes the autocrine IFN-inducedappearance of ISGF3 in response to IFN, DRAF1 may afford the hostsome measure of defense to infection (9). Other investigatorshave described the appearance of another ISRE-binding factor,activated in response to vesicular stomatitis virus, VIBP (5).The relationship of this factor to DRAF1 or to another factorthat we have detected in some cells, DRAF2, remains to be determined(9, 11).

To begin to elucidate the mechanism by which DRAF1 is activated, we investigated the component nature of DRAF1. IRF moleculesare capable of recognizing an inner core sequence of the ISRE(25, 38, 40, 42, 50), so we turned our attention toIRFs and specifically to IRF-3. The presence of IRF-3 in DRAF1was directly tested with specific antibody to IRF-3 in a DNA-bindingreaction. Antibody to IRF-3 eliminated the appearance of DRAF1,demonstrating the presence of IRF-3 in the complex. IRF-3 appearsto reside exclusively in the cytoplasm of cells and to translocateto the nucleus following viral infection. Scanning the primaryamino acid sequence of IRF-3 does not reveal a consensus nuclearlocalization sequence (NLS) (reviewed in references 15 and 45).In this respect, IRF-3 is distinct from some IRF family members,such as IRF-1, which contain a putative NLS and localize to thenuclear compartment (31). However, it is possible that IRF-3does contain a functional NLS that is masked prior to infection.IRF-3 may also contain a nuclear export signal (NES) that is functionalonly prior to infection (reviewed in reference 49). The mechanismsthat control IRF-3 cellular localization remain to be determinedand could depend on serine phosphorylation regulating an NLS oran NES or interactions with as-yet-unidentified factors. Sincetyrosine phosphorylation appears to be required for DRAF1 DNAbinding and IRF-3 does not contain phosphotyrosine, another DRAF1subunit may be tyrosine phosphorylated.

Identification of IRF-3 as a subunit of DRAF1 allowed us to use coimmunoprecipitation assays to search for IRF-3-associatedproteins. Metabolic radiolabeling of cells revealed a coimmunoprecipitatedprotein with an apparent molecular mass of approximately 300 kDa.Use of characterized antibodies revealed the presence of the transcriptionalcoactivators CBP and p300 in immunocomplexes with IRF-3 only followingviral infection and in the DRAF1 DNA-binding complex. The CBPand p300 coactivators have been shown to associate with a growingnumber of transcription factors (reviewed in references 18,23, and 46). In the IFN signal pathway, CBP and p300 moleculesinteract with the STAT1 and STAT2 subunits of ISGF3 (4, 26,48, 58). CBP and p300 molecules do not bind to DNA directlybut have several properties that may contribute to their rolein transcriptional activation: physical association with basaltranscription factors, intrinsic acetyltransferase activity thatappears to play a role in histone acetylation and chromatin conformation,and acetylation of specific transcription factors (3, 24,39, 46). IRF-3 nuclear translocation and association withCBP and p300 in response to viral infection lead to the generationof DRAF1 and the activation of a subset of ISGs (11). In addition,it is possible that DRAF1 is involved in the induction of oneor more of the type I IFN genes. DRAF1 may function to activategenes that play a role in host survival via either known antiviraland antiproliferative mechanisms or as-yet-unidentified mechanisms.

	ACKNOWLEDGMENTS

We thank Christopher Daly for providing unpublished observations critical to the completion of the manuscript. We also thankall the members of our laboratory for help and suggestions, CarrieMahlum and Emily Huang for technical assistance, and Dianna Berryfor assisting in the production of antibodies to IRF-3. The giftsof PTP1B from Nicholas K. Tonks and PKR-deficient MEFs from BryanR. G. Williams and Charles Weissmann are greatly appreciated.We also thank Joav Prives and Dafna Bar-Sagi for assistance withthe phosphoamino acid analyses and Michael Katze for helpful discussionsconcerning PKR. Recombinant human IFN- $alpha$ was a gift from Hoffmann-LaRoche Inc.

This work was supported by grants from the National Institutes of Health (RO1CA50773 and PO1CA28146) and The Council for TobaccoResearch (3717) to N.C.R.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Pathology, State University of New York at Stony Brook, Stony Brook,NY 11794-8691. Phone: (516) 444-7503. Fax: (516) 444-3424. E-mail:nreich{at}path.som.sunysb.edu.

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Abstract
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Materials & Methods
Results
Discussion
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