Functional Analysis of Human Herpesvirus 8-Encoded Viral Interferon Regulatory Factor 1 and Its Association with Cellular Interferon Regulatory Factors and p300

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Journal of Virology, September 1999, p. 7334-7342, Vol. 73, No. 9
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Functional Analysis of Human Herpesvirus 8-Encoded Viral Interferon Regulatory Factor 1 and Its Association with Cellular Interferon Regulatory Factors and p300

Ladislav Burý $s$ ek,¹ Wen-Shuz Yeow,¹ Barbora Lubyová,¹ Merrill Kellum,¹ Susan L. Schafer,¹ Yao Qi Huang,² and Paula M. Pitha¹^,³^,^*

Oncology Center¹ and Department of Molecular Biology and Genetics,³ The Johns Hopkins University School of Medicine, Baltimore, Maryland 21231, and Hematology Division, Department of Medicine, New York University Medical Center, New York, New York 10016²

Received 12 January 1999/Accepted 24 May 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Human herpesvirus 8/Kaposi sarcoma-associated virus (HHV-8/KSHV) contains, in addition to genes required for viral replication,a unique set of nonstructural genes which may be part of viralmimicry and contribute to viral replication and pathogenesis invivo. Among these, HHV-8 encodes four open reading frames (ORFs)that showed homology to the transcription factors of the interferonregulatory factor (IRF) family. The ORF K9, viral IRF 1 (vIRF-1),has been cloned, and it was shown that, when overexpressed, itdown modulates the interferon-mediated transcriptional activationof the interferon-stimulated gene 15 (ISG 15) promoter, and therole of vIRF-1 in viral mimicry was implied. However, the molecularmechanism of this effect has not been clarified. Here, we extendthis observation and show that vIRF-1 also downregulates the transcriptionalactivity of IFNA gene promoter in infected cells by interferingwith the transactivating activity of cellular IRFs, includingIRF-1 and IRF-3. We further show that ectopic expression of vIRF-1in NIH 3T3 cells confers resistance to tumor necrosis factor alpha-inducedapoptosis. While vIRF-1 is unable to bind DNA with the same specificityas cellular IRFs, we demonstrate by in vitro binding assay thatit can associate with the family of cellular IRFs, such as IRF-1and the interferon consensus sequence binding protein. vIRF-1interaction domain was localized between amino acids (aa) 152and 243. While no binding between the full-size IRF-3 and vIRF-1could be detected by the same assay, we show that vIRF-1 alsotargets the carboxy-terminal region (aa 1623 to 2414) of the transcriptionalcoactivator p300 which could also bind IRF-3 and IRF-1. Theseresults demonstrate that vIRF-1 can modulate the transcriptionof the IFNA genes by direct heterodimerization with members ofthe IRF family, as well as by competitive binding with cellulartranscription factors to the carboxy-terminal region ofp300.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The human herpesvirus 8/Kaposi Sarcoma-associated herpesvirus (HHV-8/KSHV) may be the causal factor in Kaposi sarcoma, AIDS-associatedbody cavity-based lymphoma or pleural effusion lymphoma, and multicentricCastelman's disease. HHV-8 is a gammaherpesvirus, such as Epstein-Barrvirus (EBV) (4) and herpesvirus saimiri, which are oncogenic(1). The analyses of HHV-8 genomic sequences (44) showedthat this virus contains, in addition to genes required for viralreplication, a unique set of nonstructural genes which may bepart of viral mimicry and essential for viral replication andpathogenicity invivo.

Two of the HHV-8 analogues of cellular IRFs, open reading frame (ORF) K9-encoded viral interferon (IFN) regulatory factor(vIRF; named vIRF-1 in this study) and vIRF-2 (11), have beencloned. The expression of vIRF-1 can be induced by tetradecanoylphorbol acetate (TPA) treatment in BCBL-1 cells (30); the presenceof vIRF-1 antisense RNA reduced the expression of several HHV-8lytic genes, including interleukin-6 (IL-6) in TPA-treated BCBL-1cells (26). In that study it was suggested that vIRF-1 playsan important role in the regulation of HHV-8 replication cycle.Several groups (15, 26, 38, 57) have shown that vIRF-1can function as a repressor on promoters containing IFN-sensitiveresponse element and that NIH 3T3 cells constitutively overexpressingvIRF-1 gained the ability to grow in soft agar and to form tumorsin nude mice. These data indicate that vIRF-1, like IRF-2, behavesas an oncogene. However, the molecular mechanism by which vIRF-1downmodulates IFN-stimulated activation of IFN-stimulated gene(ISG) promoters or confers to NIH 3T3 cells the ability to growin soft agar and in nude mice has not been clarified. We haverecently cloned and characterized a second HHV-8 encoded vIRF,vIRF-2, that encodes a short protein of 163 amino acids (aa) (11).vIRF-2 is a DNA binding protein with a specificity distinct fromthat of cellular IRF, since it binds to oligonucleotide correspondingto the NF- $kappa$ B site. In a transient-transfection assay, vIRF-2 inhibitsthe virus-mediated induction of promoters of IFN genes as wellas RelA-stimulated activity of the human immunodeficiency viruslong terminal repeat. Thus, the properties and, consequently,the biological functions of vIRF-1 and vIRF-2 seem to bedistinct.

Transcriptional factors of the IRF family have been shown to play an essential role in the regulated expression of IFN andISGs (34). All the cellular IRF proteins identified show homologyin their 5' DNA binding domain (DBD), which is characterized byfive highly conserved tryptophan (W) repeats; three of these repeatscontact DNA recognizing the GAAA sequence (14). The carboxy-terminalhalves of these proteins are diverse. IRF-1 was originally identifiedby its ability to bind the GAAAGT sequence present in multiplecopies in the promoter of IFNB gene, and it was proposed thatIRF-1 serves as a positive activator of IFN genes in virus-infectedcells, while a closely related homologue, IRF-2, acts as a repressor(17). However, homozygous deletion of the IRF-1 gene has notaffected the virus-mediated activation of IFNA and IFNB genesexpression (29, 42), whereas it downmodulated the expressionof IL-12 and the antiviral effects of IFNs (43). Another memberof this family, p48, interacts with phosphorylated STAT1 and STAT2transcription factors forming ISGF3 complex (6, 7) in IFN-treatedcells. This complex binds to the IFN-stimulated response element(ISRE) in the promoter of ISGs and activates their transcription.Homozygous deletion of p48 in mice abolishes sensitivity of thesemice to the antiviral effect of IFNs and impairs the inductionof IFNA and IFNB genes in a cell-type-specific manner (19, 22).Several other members of the IRF family have been identified.The IFN consensus sequence binding protein (ICSBP) is expressedexclusively in cells of immune system, including monocytes, Bcells, and T cells (9). It complexes with IRF-1 and thus repressesthe transactivation mediated by IRF-1 (33, 48, 53). In mice,homologous deletion of ICSBP results in the deregulation of hematopoiesisand lymphopoiesis (20) and the defective expression of IL-12(16). IRF-3 is expressed constitutively in most of the tissuesand cell types (3) and strongly cooperates with virus in stimulationof IFN gene expression. In infected cells, IRF-3 is phosphorylatedand transported into the nucleus where it binds the transcriptionalcoactivator p300/CBP (27, 55). It appears, therefore, thatIRF-3 plays a critical role in virus-mediated signaling (21,32, 46, 47). Another IRF that was shown recently to playa critical role in the induction of IFNA genes is IRF-7 (2,28, 45, 51). IRF-7 also strongly cooperates with the virus-mediatedinduction of IFN genes, particularly IFNA genes, and was shownalso to play a role in the regulated expression of viral QP promoterof the EBV-encoded EBNA-1 gene (36, 56).

Both IRF-1 and IRF-2 also modulate cell growth. Overexpression of IRF-1 has a growth-inhibitory effect and induces apoptosis(23, 49). In contrast, overexpression of IRF-2 in NIH 3T3cells confers oncogenic transformation and tumor formation innude mice, implicating IRF-2 as a potential oncogene. IRF-1, however,can reverse the IRF-2-induced transformation, as well as suppressc-myc and c-fos-induced transformation (18). Fibroblasts fromIRF-1^/ mice show resistance to UV- and drug-induced apoptosis (49,50). Since the deletion of IRF-1 on chromosome 5q31.3 is frequentlyfound in leukemia, it was suggested that IRF-1 might functionas a tumor suppressor gene (8, 54).

The aim of the present study was to further characterize the functional role of vIRF-1 in the expression of the early inflammatorygene (IFNA), as well as to determine the molecular mechanismsby which vIRF-1 exerts some of its biological effects. We haveshown that in infected cells, vIRF-1 specifically represses thetranscriptional activity of IFNA gene promoters, while, in uninfectedcells, overexpression of vIRF-1 confers resistance to tumor necrosisfactor alpha (TNF- $alpha$ )-induced apoptosis. By using in vitro pull-downassay, we have further demonstrated a specific interaction betweenvIRF-1 and cellular IRFs, including IRF-1, and demonstrated thatvIRF-1 contains an interaction-associated domain (IAD) by whichit associates with IRF-1. We have further demonstrated an in vitrointeraction between vIRF-1 and the C'-terminal domain of p300.We therefore conclude that, by specific interaction with IRF-1,vIRF-1 may lessen both the antiviral and antiapoptotic functionsof IRF-1 while, by its interaction with p300, vIRF-1 may competefor binding of both IRF-1 and IRF-3 and so decrease their transactivatingpotential.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture and transfections. NIH 3T3 cells were grown in Dulbecco modified Eagle medium (DMEM) and 10% fetal bovine serum (FBS). The BCBL-1 cells weregrown in RPMI supplemented with 10% FBS. In the transfection assays,subconfluent NIH 3T3 cells (2 × 10⁵ cells/35-mm plate) were cotransfected with 1 µg of reporter chloramphenicolacetyltransferase (CAT) plasmid and 1 µg of each indicated expressionplasmid by using the calcium phosphate coprecipitation method(31) or Superfect (Qiagen). The total amount of DNA was adjustedto 3 µg with empty vector pcDNA3.1 (Invitrogen) for each experiment.When indicated, cells were infected with Newcastle disease virus(NDV) (multiplicity of infection of 5) at 24 h after transfectionfor 16 h. Protein extracts were prepared by the freeze-thaw methodat 48 h after transfection, and CAT assays were done as describedpreviously (40). The same amount of protein was used for eachreaction. Thin-layer chromatography plates were quantified byusing a PhosphorImager (MolecularDynamics).

Viability assay. Cells (1.5 × 10⁵/ml) in DMEM containing 10% FBS, 1 µg of actinomycin D per ml, and increasing concentrations of TNF- $alpha$ wereseeded (100 µl) into 96-well panels and grown in CO₂ at 37°C for24 h. Viable cells were measured by the MTT assay (12).

Plasmids. (i) Cloning of vIRF-1. The vIRF-1 DNA corresponding to K9 ORF of HHV-8 was amplified from DNA extracted from KS tumor specimen by 25 cycles of PCR.Primers 5'-AGTAAGCTTGCGGGACAATGGACCCAGGCC and 3'-TTGTCTAGATTATTGCATGGCATCCCATAAwere based on the published HHV-8 sequences; the resulting 1,368-bpvIRF-1 fragment was inserted into the HindIII and XbaI sites ofpcDNA3.1 vector (Invitrogen) to construct pcDNA/vIRF-1. The cDNAwas amplified by use of Pfu polymerase (Stratagene) and then sequenced.The comparison of the sequenced analysis with that deposited inGenBank indicated that the cloned KS/vIRF-1 contained five pointmutations, four of which resulted in the amino acid change. Therefore,we have amplified and cloned vIRF-1 also from the genomic libraryof BCBL-1 cells. The DNA sequence of BCBL1/vIRF-1 was identicalto that deposited in GenBank. Both the KS/vIRF-1 and the BCBL1/vIRF-1had identical functional properties as seen in the transient-transfectionassay, and neither of them was able to bind DNA. For consistencywith the published results (26), the data presented here wereobtained with BCBL1/vIRF-1-containingplasmids.

(ii) Construction of truncated and fusion vIRF-1. To generate GST/vIRF-1 fusion proteins, full-length cDNA was amplified by PCR with the primers 5'-GCCGGAATTCAATGGACCCAGGCand 3'-CATCTCGAGGCATGGCATCCCATAA and inserted in frame into EcoRI-XhoIsites of pGEXT4 vector (Pharmacia). The N'-terminal 489-bp fragmentcoding for N' vIRF-1 (aa 1 to 158) was amplified by PCR with theprimers 5'-ATAGGATCCATGGACCCAGGCCAAAGACC and 3'-AGACTCGAGGTGCCTTTAAACGAGGCGTC.The C'-terminal 908-bp fragment of vIRF-1 (aa 152 to 449) wasamplified by PCR with the 5' primer TCTGGATCCGACGCCTCGTTTAAAGGCAC.The 3' primer was identical to that used for amplification ofglutathione S-transferase (GST)-vIRF-1. The 273-bp fragment vIRF-1A(aa 152 to 243) was amplified with primers 5'-TCTGGATCCGACGCCTCGTTTAAAGGCACand 3'-AGACTCGAGCTAACAAGATGGCACGGGCGTTAC. The 464-bp fragmentvIRF-1B (aa 152 to 307) was amplified with the primers 5'-TCTGGATCCGACGCCTCGTTTAAAGGCACand 3'-AGACTCGAGCTATTGGGTAGCCATACCTGGCC, and the 461-bp fragmentvIRF-1C (aa 295 to 449) was amplified with the primer 5'-ATAGGATCCGCCATGGCAGTGGGGTCTCCGGGCCAGand a 3' primer identical to that used for the amplification ofGST-vIRF-1. All of these vIRF-1 fragments were cloned into BamHI-XhoIsites of pGEXT4 vector. Amplifications were done by using 30 cycleswith Pfu polymerase from the BCBL1/vIRF-1 expression plasmid.The constructed proteins were expressed in bacteria and were checkedby sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE)to determine the correct molecularweight.

(iii) Construction of truncated p300 proteins. The expression plasmids coding for amino- and C'-terminal parts of human p300 were provided by G. Nabel (37). The 1,161-bpfragment p300A (aa 1243 to 1630) was amplified by PCR with theprimers 5'-TCAGGATCCGCCATGTTTGTTGAATGTACAGAGTGCGGA and 3'-ACTCTCGAGCTATGCATCCCGACCATCCAT.The 776-bp fragment p300B (aa 1623 to 1882) was amplified withthe primers 5'-TCAGGATCCCCGATGGATGGTCGGGATGCGTTT and 3'-ACTCTCGAGCTACATGCTATTGGGAGGGGTA.The 1,596-bp fragment p300C (aa 1882 to 2414) was amplified withthe primers 5'-TCAGGATCCGCCATGCCACCCTACTTGCCCAG and 3'-ACTCTCGAGCTAGTGTATGTCTAGTGTACTCTGTGAGAGG.All of these p300 fragments were cloned into BamHI-XhoI sitesof vector pcDNA3.1. Amplifications were done by use of 30 cycleswith Pfu polymerase from the p300 expression plasmid, and constructedproteins were checked by in vitro translation to determine thecorrect molecularweight.

(iv) Expression and reporter plasmids. CMV/IRF-1 and CMV/IRF-2 expression plasmids were obtained from T. Taniguchi (University of Tokyo, Tokyo, Japan). The CMV/IRF-3plasmid was as described previously (3). pSG5/ICSBP plasmidwas obtained from K. Ozato (9). The IFNA4CAT reporter plasmidwas described previously (41). In order to express deletionmutants of vIRF-1 in mammalian cells, the corresponding vIRF-1fragments were subcloned from pGEX4T vector into the BamHI-XhoIsites of pCMV-TAG expression plasmid(Stratagene).

Preparation of GST fusion proteins. Escherichia coli DH5 $alpha$ cells (200 ml at an optical density at 600 nm of 0.6) harboring the recombinant expression vectors wereinduced with 0.4 mM isopropyl- $beta$ -D-thiogalactopyranoside (IPTG;Sigma) at 37°C for 2.5 h. Cells were then washed with phosphate-bufferedsaline (PBS), resuspended in 10 ml of sonication buffer (PBS supplementedwith 1% Triton X-100 and 1 mM phenymethylsulfonyl fluoride), andincubated with 10 mg of lysozyme (Sigma) per ml on ice for 15min. The cell suspension was sonicated, and the lysate was clearedby centrifugation (12,000 × g for 10 min at 4°C). The supernatantswere mixed with glutathione-agarose beads (200 µl of a 1:1 slurryin PBS) (Pharmacia) at 4°C for 1 h, and the beads were washedthree times with ice-cold sonication buffer. The purity and quantityof fusion proteins were examined by Tricine-SDS-10% PAGE followedby Coomassie bluestaining.

GST pull-down assay. The ³⁵S-labeled proteins were synthesized in vitro by using the coupled TNT T7 transcription-translation system (Promega) accordingto the manufacturer's instructions. A total of 1 µg of nonlinearizedexpression plasmid was used in each reaction, followed by incubation(90 min, 30°C) in the presence of 4 µl of Translabel (DuPont)amino acid mixture. GST fusion proteins (0.5 µg) bound to glutathione-agarosebeads were incubated with 10-µl reaction mixture aliquots of ³⁵S-labeled proteins in 250 µl of binding buffer (10 mM Tris-Cl,pH 7.6; 100 mM NaCl; 0.1 mM EDTA, pH 8.0; 1 mM dithiothreitol[DTT]; 5 mM MgCl₂; 0.05% Nonidet P-40; 8% glycerol; mammalianprotease inhibitor cocktail [Sigma]) at 4°C for 90 min. Afterthree washes (10 min at room temperature) with binding buffer,the proteins bound to the beads were solubilized in sample lysisbuffer and resolved on Tricine-SDS-10% PAGE. When indicated, 1µg of rabbit polyclonal antibody against the C-terminal peptideof human IRF-1 (Santa Cruz) was added to the binding reaction.The gel was dried and exposed to a PhosphorImagerscreen.

Electrophoretic mobility shift analysis. DNA binding reactions were performed at room temperature for 30 min in 20 µl of binding buffer (12 mM Tris-HCl, pH 8.0; 2mM MgCl₂; 12 mM EDTA, pH 8.0; 40 mM NaCl; 6 mM DTT; 7% glycerol)containing 1 ng of GST-IRF-1 protein, the indicated amount ofHis₆-vIRF-1 protein, 1 µg of poly(dI-dC), 1 µg of BSA, and 10⁵ cpm of the indicated ³²P-labeled double-stranded probe. Protein-DNA complexes were thenresolved in a nondenaturing (50 mM Tris, 380 mM glycine, 2 mMEDTA) 7% polyacrylamide gel, dried, and exposed to a PhosphorImagerscreen. The sequence of PRD-I probe used was 5'-GAGAAGTGAAAGTGGGAACCCTCTCCTT.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

vIRF-1 can inhibit IRF-1- or IRF-3-stimulated transcriptional activity of IFN- $alpha$ ₄ promoter in infected cells. Results from other laboratories (15, 26, 57), as well as our own previous data (38), showed that in a transient-expressionassay vIRF-1 repressed the IFN-stimulated transcriptional activityof the ISRE-containing promoters ofISGs.

To determine whether the vIRF-1 repression is limited to the IFN-mediated stimulation of ISGs or whether it can also modulatethe virus-stimulated expression of early inflammatory genes, suchas type I IFN genes, we analyzed the effect of vIRF-1 on the virus-mediatedstimulation of IFNA4 reporter plasmid in a transient-expressionassay (41). This plasmid contains IFNA4 gene promoter region,including the virus-inducible elements with an IRF-E site butno NF- $kappa$ B site. Constitutive expression of the IFNA4 CAT plasmidin NIH 3T3 cells was very low, but the transcriptional activityof the IFNA promoter was significantly stimulated (15-fold) uponinfection with NDV (Fig. 1) (3). Cotransfection with vIRF-1-expressingplasmid inhibited the CAT expression by about two- to threefold.We have previously shown that, in a transient-transfection assay,virus-mediated stimulation of the IFNA4 gene promoter could beenhanced by cotransfection with IRF-1 (3), IRF-3 (21), orIRF-7 (2). While cotransfection with IRF-1 has increased virus-mediatedactivation of IFNA4 promoter threefold, IRF-3-enhanced virus stimulatedthe activity of IFNA4 promoter by sixfold (Fig. 1). Cotransfectionwith vIRF-1 effectively inhibited the IRF-1-mediated stimulationof the IFNA gene promoter in infected cells, indicating that vIRF-1interfered with the transactivation potential of IRF-1. Similarly,synergism between virus- and IRF-3-mediated activation was alsoinhibited in cells overexpressing vIRF-1; however, the inhibitoryeffect by vIRF-1 could be demonstrated only at higher levels ofvIRF-1 (Fig. 1). These data indicate that vIRF-1 interferes withthe IRF-1- and IRF-3-mediated transcriptional activation of IFNA4promoter in infected cells.

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FIG. 1. vIRF-1 inhibited synergistic activation of IFNA4 promoter by NDV and IRF-1 or IRF-3. The IFNA4 CAT reporter plasmid (1 µg) was cotransfected into NIH 3T3 cells with 1 µg of either pcDNA vector (Con), IRF-1, or IRF-3 expression plasmids, together with increasing amount of vIRF-1 expression plasmid (1 and 4 µg). Cells were infected with NDV 24 h after transfection for 16 h and analyzed for CAT activity. Error bars show standard errors for triplicate experiments.

Expression of vIRF-1 in NIH 3T3 cells confers resistance to apoptosis. IRF-1 was shown to inhibit cell growth and induce apoptosis. The fibroblast cells derived from mice with homozygous deletionof IRF-1 gene were resistant to drug- and UV-induced apoptosis(50). Since we have found that vIRF-1 interferes with the functionof IRF-1 in infected cells, we wished to examine whether vIRF-1could also interfere with the cellular function of IRF-1. TheNIH 3T3 cell line that constitutively expressed transfected vIRF-1(Fig. 2A) and showed a decreased sensitivity to the antiviraleffect of mouse IFN- $alpha$ and IFN- $beta$ (data not shown) was analyzedfor its sensitivity to TNF- $alpha$ -induced apoptosis (24). The NIH3T3/vIRF-1 and the parental NIH 3T3 cells were treated with anincreasing concentration of TNF- $alpha$ in the presence of actinomycinD, and the cell viability was determined 24 h later by MTT assay(12). The results, shown in Fig. 2B, demonstrate that NIH 3T3/vIRF-1cells were less susceptible to TNF- $alpha$ -induced apoptosis than werethe parental NIH 3T3 cells. At the TNF- $alpha$ concentration of 4 pg/ml,no cell death could be detected in NIH 3T3/vIRF-1 cells, whilemore than 50% of the NIH 3T3 cells were killed. The same degreeof difference in cell killing between the vIRF-1-expressing cloneand the parental line was seen in cells treated with double-strandedRNA (data not shown).

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FIG. 2. NIH 3T3 cells expressing vIRF-1 showed resistance to TNF- $alpha$ -mediated apoptosis. (A) Expression of vIRF-1 mRNA in the clone (3T3/vIRF-1) selected for studies of apoptosis (Northern blot). The NIH 3T3 cell line expressing vIRF-1 was generated as described in Materials and Methods. (B) Comparison of TNF- $alpha$ -induced cell killing in control NIH 3T3 cells and NIH 3T3/vIRF-1 cells. Cells were treated with the indicated concentrations of mouse TNF- $alpha$ and actinomycin D (1 µg/ml) for 24 h, and the cell viability was determined by MTT assay. The data represent an average (± the standard error of the mean) of two separate experiments done in triplicate.

These data further suggest that the expression of vIRF-1 interferes with the functions of IRF-1 even in the absence of viralinfection.

vIRF-1 interacts with cellular IRF transcription factors in vitro. It was previously reported by others that recombinant, full-length vIRF-1 was unable to bind ISRE elements and a positiveregulatory domain (PRD-I) present in the IFNB promoter (15,57). Since vIRF-1 contains an N'-terminal 85-aa peptide whichis not present in any other cellular IRFs and which could interferewith binding of the putative DNA binding domain (DBD), we examinedwhether the removal of this peptide would restore DNA binding.However, the N'-terminal-truncated vIRF-1 expressed as a GST fusionprotein (aa 85 to 449) was also unable to bind these probes (datanot shown). These data indicated that the inhibition by vIRF-1was not the result of competition with IRF-1 for the DNA bindingas demonstrated for IRF-1 and IRF-2. It was shown that the activityof cellular IRFs could be modulated by their association eitherwith other family members or other transcription factors (10,39, 48). We therefore examined whether the observed inhibitoryeffect of vIRF-1 could be mediated by its interactions with cellularIRFs or other cellular transcriptioncofactors.

To analyze the interaction between vIRF-1 and the members of the IRF family of transcription factors, we used in vitro pull-downassay. GST-vIRF-1 fusion protein was immobilized on glutathione-agarosebeads and incubated with the in vitro-synthesized ³⁵S-labeled IRF proteins. The immobilized vIRF-1 bound stronglyIRF-1 (Fig. 3A, lanes 1 to 3), and 21% of the input ³⁵S-labeled IRF-1 was bound to immobilized vIRF-1. No binding wasdetected to control beads containing GST only. Furthermore, addingantibody that recognized a C'-terminal peptide of IRF-1 (lane4) inhibited the binding of IRF-1 to GST-vIRF-1 by about fivefold.These data indicate that the observed binding of IRF-1 to vIRF-1is specific. Only 0.2% of in vitro translated IRF-2 bound to theimmobilized GST-vIRF-1, a level of binding which we consideredto be insignificant (lane 7). We were also unable to detect anyspecific binding of in vitro-translated IRF-3 to GST-vIRF-1 (Fig.3A, lanes 8 to 10). Although the binding of ICSBP to immobilizedGST-vIRF-1 was lower than the binding of IRF-1, 6% of the inputICSBP was retained on GST-vIRF-1 beads (lanes 11 to 13). It shouldbe mentioned at this point that Zimring et al. (57) failed todetect any association between in vitro-cotranslated vIRF-1 andIRF-1.

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FIG. 3. (A) Analysis of interactions between vIRF-1 and cellular IRF transcription factors by in vitro pull-down assay. Recombinant GST-vIRF-1 fusion protein was immobilized on glutathione-agarose beads and incubated with indicated ³⁵S-labeled IRF proteins as described in Materials and Methods. In lanes 1, 5, 8, and 11, 20% of the respective in vitro-labeled input IRF was loaded onto the gel. Lanes 2, 6, 9, and 12 show binding to beads containing GST protein only. Lanes 3, 7, 10, and 13 show binding of IRF-1, IRF-2, IRF-3, and ICSBP, respectively. The binding in the presence of antibody (1 µg) against C-terminal peptide of IRF-1 is shown in lane 4. (B) Virus infection does not modulate IRF-1-GST-vIRF-1 interaction in cell lysates. NIH 3T3 cells were transfected with IRF-1 expression plasmid, and 24 h later cells were infected with NDV (multiplicity of infection of 5) for 16 h. Cell lysates from control ( $-$ ) or infected cells (NDV) were then subjected to pull-down assay. GST-vIRF-1-bound proteins were resolved on SDS-10% PAGE and immunoblotted with anti-IRF-1 antibody (lane 3). Input (lane 1) represents 1% of total protein added into binding reaction. No detectable interaction was observed with control, GST-containing beads (lane 2). (C) Detection of vIRF-1 and vIRF-2 protein interactions. In vitro ³⁵S-labeled vIRF-1 and vIRF-2 proteins were incubated with GST-vIRF-1 or GST bound to glutathione-agarose beads. Bound proteins were resolved by SDS-10% PAGE. Input vIRF-1 (lane 1) represents 20% of ³⁵S-labeled vIRF-1 translation mixture added to beads.

To further examine whether viral infection modifies the binding of IRF-1 to vIRF-1, we analyzed the binding of IRF-1 fromcell lysates of transiently transfected NIH 3T3 cells with IRF-1expressing vector and infected with NDV. As seen in Fig. 3B, asignificant amount of IRF-1 was coprecipitated with GST-vIRF-1beads from cell lysates of IRF-1-transfected NIH 3T3 cells (about30% of input); however, the binding was not significantly differentif the lysates were prepared from NDV-infected cells (Fig. 3B).Since viral infection stimulated the expression of endogenousIRF-1 gene, the IRF-1 signal in infected cells was higher thanin uninfected cells. Virus stimulation therefore did not influencethe interaction between IRF-1 and vIRF-1.

We further examined whether vIRF-1 was able to form homodimers or interacted with vIRF-2 by using the pull-down assay with³⁵S-labeled vIRF-1. As seen in Fig. 3C, vIRF-1 was retained bothby GST-vIRF-1 and GST-vIRF-2 immobilized on agarose beads (lanes3 and 4), while no vIRF-1 was pulled down by the control, GST-containingagarose beads (lane 2). These data indicate that, in vitro, vIRF-1can form homodimers as well as interact with vIRF-2.

Identification of the vIRF-1 binding domain. To determine which part of vIRF-1 protein interacted with IRF-1, we constructed GST fusion proteins with the N'-terminal (aa1 to 158) and C'-terminal (aa 152 to 449) parts of vIRF-1. TheC'-terminal part of vIRF-1 molecule was further divided to threepeptides designated parts A (aa 152 to 243), B (aa 152 to 307),and C (aa 295 to 449) (Fig. 4A), which were also expressed asGST fusion proteins. The mobility and purity of these recombinantfusion peptides is shown in Fig. 4B. When used in the pull-downassay, GST-vIRF-1C' was able to bind effectively in vitro-translated³⁵S-labeled IRF-1 (Fig. 4C, lane 4), while no binding of the labeledIRF-1 to GST-vIRF-1N' was detected (lane 3), indicating that IRF-1interacts specifically with the C'-terminal part of vIRF-1. Todetermine precisely the IAD of vIRF-1, we analyzed the bindingof ³⁵S-IRF-1 to the immobilized GST-vIRF-1A, -1B, and -1C fusion peptides.It can be seen (Fig. 4C, lanes 5 and 6) that IRF-1 binds to bothimmobilized GST-vIRF-1A and GST-vIRF-1B fusion peptides, whileno interaction with GST-vIRF-1C peptide was observed (lane 7).Since the A and B peptides partially overlap, we conclude thatthe vIRF-1 IAD is located between aa 152 and 243.

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FIG. 4. Mapping of vIRF-1 interaction domain. (A) Positional scheme of vIRF-1 deletion mutants. Numbers correspond to amino acid boundaries of respective fragments. (B) Coomassie blue-stained gel illustrating the purity and size of the respective GST-vIRF-1 fusion fragments. (C) In vitro interaction between IRF-1 and different vIRF-1 fragments as detected by pull-down assay. ³⁵S-labeled IRF-1 input (20%) and its binding to GST beads are shown in lanes 1 and 2, respectively. IRF-1 was pulled down by GST-vIRF-1C' (lane 4) and not by GST-vIRF-1N' (lane 3). Both GST-vIRF-1A (lane 5) and GST-vIRF-1B (lane 6) fragments actively bound IRF-1, while no IRF-1 binding was detected with GST-vIRF-1C fragment (lane 7).

Using the transient-transfection assay, we assessed the ability of the C'-terminal peptides of vIRF-1 to inhibit transcriptionalactivity of the IFNA4 promoter. We cotransfected IFNA4 CAT reporterplasmid together with IRF-1 and vIRF-1A, -1B, and -1C (Fig. 4)expressing plasmids into NIH 3T3 cells, which were then infectedwith NDV. The results in Fig. 5A show that C'-terminal vIRF-1peptides were able to downregulate the transcriptional activityof the IFNA4 promoter. All the C'-terminal peptides were betterinhibitors than the full-length vIRF-1, indicating that, in thefull-length protein, the IAD may be less accessible or activelyregulated by other domains of the molecule. Interestingly, theC peptide of vIRF-1 that was not able to bind effectively to IRF-1in the GST pull-down assay was also inhibitory. Since in our preliminaryresults the C peptide of vIRF-1 did not interact strongly withthe p300 protein (data not shown), the observed inhibition ofIFNA4 activity by the vIRF-1C peptide may be due to its interactionwith other regulatory proteins. These data indicate that vIRF-1peptides that are able to bind either IRF-1 or p300 can also downregulatetheir transactivating activities onto IFNA4 promoter in the transient-transfectionassay.

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FIG. 5. (A) The C'-terminal peptides of vIRF-1 disrupt the specific activation of the IFNA4 promoter by NDV and IRF-1. The cotransfections were done as described in Fig. 1 by using 1 µg of each IRF-1, IFNA4 CAT, and the respective plasmid encoding the C'-terminal vIRF-1 peptides. The relative levels of vIRF-1 peptides in transfected cells were comparable (data not shown). Error bars show the standard errors for triplicate experiments. (B) vIRF-1 modulates the binding of IRF-1 to PRD-I oligonucleotide. Gel retardation assays were performed with purified recombinant GST-IRF-1 and His₆-vIRF-1 proteins and ³²P-labeled PRD-I probe. A total of 1 ng of GST-IRF-1 was preincubated alone (lane 1) or in the presence of 3, 5, or 7 ng of His₆-vIRF-1 (lanes 2 to 4). The same reaction as in lane 2 was performed in the presence of 3 µl of vIRF-1 antiserum (AS, lane 5).

To test whether the formation of vIRF-1 and IRF-1 heterodimers affects the DNA binding activity of IRF-1, we subjected a preincubatedmixture of purified recombinant GST-IRF-1 and His₆-vIRF-1 proteinstogether with radioactively labeled DNA probe corresponding tothe PRD-I binding site in the IFNB gene promoter to electrophoreticmobility shift analysis. As can be seen in Fig. 5B, incubationof 1 ng of GST-IRF-1 with PRD-I probe resulted in the formationof one distinct DNA-protein complex A (lane 1). When His₆-vIRF-1protein (3 ng) was added to binding reaction, the intensity ofcomplex A increased and a new complex with a slower mobility wasformed (lane 2). This new complex could represent a vIRF-1-IRF-1heterodimer. However, when an increased amount of His₆-vIRF-1protein (5 and 7 ng) was preincubated with GST-IRF-1, the DNAbinding activity of GST-IRF-1 diminished (lanes 3 and 4). To confirmthe presence of His₆-vIRF-1 protein in the GST-IRF-1 DNA complex,antiserum against vIRF-1 was added to the binding reaction. Asseen in Fig. 5B, lane 5, in the presence of vIRF-1 antiserum,two new complexes with lower mobilities (B and S) were detected.These data indicate that at equal molar ratio, IRF-1-vIRF-1 heterodimercan bind PRD-I element, but an excess of vIRF-1 blocks bindingof IRF-1 toDNA.

Interaction of vIRF-1 and IRF-1 with the transcription coactivator, p300. Interaction between transcription factors of the IRF family, IRF-3 and IRF-7, and transcription coactivator p300 has beenshown to have a functional impact (2, 21, 27, 52, 55).Therefore, we tested the affinity of vIRF-1 for p300 by the pull-downassay. The N'- and C'-terminal parts of p300 (for details, seeMaterial and Methods) were translated in vitro and subjected topull-down assay on immobilized GST-vIRF-1 fusion proteins. Theinteraction between IRF-1 and p300 was analyzed by using the sameassay. As shown in Fig. 6A, only C'-terminal part of p300 wasable to bind to immobilized GST-vIRF-1 or GST-IRF-1 (lanes 7 and10), while no significant interaction between the N'-terminalpart of p300 and vIRF-1 or IRF-1 could be detected (lanes 3 and4). We further found that the C'-terminal domain of vIRF-1 stronglybinds to p300C' (lane 8), whereas the binding of p300C' to GST-vIRF-1N'beads was very low and probably insignificant (lane 9). No bindingof either the N'-terminal or the C'-terminal part of p300 to GSTalone was detected (lanes 2 and 6). These data indicate that bothvIRF-1 and IRF-1 bind in vitro to a C'-terminal half of p300 transcriptioncoactivator. This region of p300 is targeted by a variety of transcriptionfactors, including STAT-1, c-Fos, E1A, TFIIB, NF- $kappa$ B, and kinasepp90 (13). To map precisely the region of p300 binding to vIRF-1and IRF-1 proteins, we divided p300C' molecule into three fragments:A (aa 1239 to 1622), B (aa 1623 to 1882), and C (aa 1882 to 2414)(Fig. 6B). The mobility and purity of in vitro-translated A, B,and C peptides on SDS gel is shown in Fig. 6C (lanes 1, 2, and3). It can be seen (Fig. 6C) that in a pull-down assay only theB and C peptides were able to bind to the immobilized GST-vIRF-1C'fusion protein (lanes 8 and 9). The B and C peptides also boundto the immobilized GST-IRF-1 fusion protein (lanes 11 and 12).No significant binding of A peptide to GST-vIRF-1C' or GST-IRF-1beads was observed (lanes 7 and 10). None of these peptides boundto GST beads only (lanes 4 to 6). These data indicate that bothvIRF-1 and IRF-1 proteins bind to a C'-terminal region of p300protein containing the C/H3 and Q-rich domains (aa 1623 to 2414)and may compete for the same binding site.

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FIG. 6. In vitro binding analysis of vIRF-1 and IRF-1 to p300. (A) Interaction of vIRF-1 and IRF-1 with the N'- and C'-terminal parts of p300. Binding of in vitro ³⁵S-labeled N'-terminal half of p300 to immobilized GST-vIRF-1 and GST-IRF-1 is shown in lanes 3 and 4. The binding of the in vitro ³⁵S-labeled C-terminal half of p300 to immobilized GST-vIRF-1 and GST-IRF-1 is shown in lanes 7 and 10. The binding of the C-terminal half of the p300 to N- and C-terminal parts of GST-vIRF-1 is shown in lanes 8 and 9, respectively. Lanes 2 and 6 show the binding to GST beads only, and lanes 1 and 5 show the input of the ³⁵S-labeled N- or C-terminal part of p300 (20%). (B) Positional scheme of p300 deletion mutants. The numbers correspond to the amino acid boundaries of the respective fragments. (C) Mapping of p300 binding site for vIRF-1 and IRF-1 by in vitro pull-down assay. Recombinant GST-vIRF-1C' and GST-IRF-1 fusion proteins were immobilized on glutathione-agarose beads and incubated with indicated ³⁵S-labeled p300 peptides as shown in Fig. 6B. In lanes 1 to 3, 20% of the in vitro-labeled p300 fragments A, B, and C were analyzed on an SDS gel. Lanes 4 to 6 show the binding to beads containing GST protein only. Lanes 7 to 9 show the binding of the indicated p300 fragment to GST-vIRF-1C' beads, and lanes 10 to 12 show the binding of the indicated p300 fragment to GST-IRF-1 beads.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

HHV-8 is the first identified viral genome that contains ORFs homologous to the cellular transcriptional factors of the IRFfamily. While cellular IRFs are DNA binding proteins, neitherthe full-size vIRF-1 nor its 5'-end deletion mutant was able tobind oligonucleotides with specificities similar to those of thecellular IRFs. The vIRF-1 shows partial homology in its N-terminalregion with a DBD of IRF-3 and IRF-4. However, only two of thefive characteristic W repeats in cellular IRFs are preserved invIRF-1. Nevertheless, it is unlikely that the amount of W repeatin the N terminus of vIRF-1 accounts entirely for the inabilityof this protein to bind DNA. This region of vIRF-1 is very similarto vIRF-2, which we have recently shown to be able to bind oligonucleotidecorresponding to the NF- $kappa$ B binding site (11). In contrast, vIRF-1cannot bind to NF- $kappa$ B probe (data not shown). However, it is possiblethat the C'-terminal part of the vIRF-1 may interact with andmask the binding domain of vIRF-1. The full-size mouse IRF-4 (PIP)is also unable to bind DNA because of the interaction betweenthe N'-terminal and C'-terminal parts of the PIP protein (10).However, when this interaction is prevented either by deletionof the C-terminal part of the PIP protein or by its binding toanother transcription factor, PU.1, the DNA binding capacity ofPIP is restored (39). Experiments are in progress to examinewhether 3' deletion mutants of vIRF-1 regain the ability to bindDNA.

It was suggested previously that the expression of vIRF-1 may contribute to viral mimicry and enable HHV-8 to escape the antiviraleffect of IFN since vIRF-1 was shown to downregulate IFN-stimulatedtranscriptional activity of various ISG promoters; however, themechanism by which vIRF-1 exerts this effect was not clarified(15, 26, 38, 57). We have further extended this observationand shown in this study that vIRF-1 inhibited virus-mediated transcriptionalactivation of the IFNA4 promoter. Furthermore, vIRF-1 effectivelydownmodulated the synergistic interaction between virus and IRF-1or IRF-3, indicating that vIRF-1 interferes with the transactivationability of these two cellular IRFs. In the absence of demonstrablevIRF-1 DNA binding, we examined the possibility that vIRF-1 isblocking the transactivation activity of IRF-1 and IRF-3 by directinteraction with these proteins, as was demonstrated for ICSBP-mediatedinhibition of IRF-1 activation (53). Our data show that GST-vIRF-1interacts strongly with both in vitro-translated IRF-1 and IRF-1present in the cellular extracts from infected and uninfectedcells. However, in the same assay, no interaction between vIRF-1and in vitro-translated IRF-3 was detected. There may be at leasttwo reasons for this discrepancy. (i) IRF-3 is phosphorylatedin infected cells (21, 27, 46, 55), and there is an indicationof an interaction between the C'- and N'-terminal parts of theunphosphorylated IRF-3 peptide (unpublished results). Therefore,it is possible that IRF-3 has to be phosphorylated in the C' terminusto uncover the interacting domain. (ii) It was shown that IRF-3interacts with the C'-terminal part of the CBP/p300 transcriptionalcofactor (27, 52, 55) and that this interaction is functional,since E1A inhibits IRF-3-mediated transactivation by targetingp300 (21). Our results show that vIRF-1 also interacts withC'-terminal part of p300, and thus the observed inhibition couldbe the result of competitive binding between IRF-3 and vIRF-1to p300. Additional experiments are being performed to determinewhich of these mechanisms areoperative.

The observation that vIRF-1 can inhibit virus-mediated activation of type I IFN gene promoter also in fibroblast cells lackingthe IRF-1 gene (data not shown) further indicates that vIRF-1inhibition is not limited to IRF-1-mediated activation (57).While vIRF-1 interacts strongly with IRF-1, it also binds p48(data not shown) and ICSBP in vitro. Since the IFN-stimulatedinduction of ISGs is mediated by the ISGF3 $gamma$ complex consistingof p48, STAT1, and STAT2 proteins, the interaction of vIRF-1 withp48 could result in the disruption of this complex; however, theformation of ISGF3 $gamma$ complex in IFN-treated cells does not seemto be prevented in cells overexpressing vIRF-1 (37a). Studieswith p48 and IRF-1 knockout mice revealed that the establishmentof maximal antiviral state is impaired in cells that have deletedeither of these genes and showed that both IRF-1 and p48 haveessential and nonredundant functions in the antiviral responseto IFNs (22). The interaction of vIRF-1 with ICSBP is also ofinterest since ICSBP interacts with IRF-1 and inhibits its transactivatingability in a cell-type-specific manner (48). Therefore, it ispossible that binding of vIRF-1 to ICSBP could result in a potentiationof IRF-1 transcriptionalactivity.

The association of vIRF-1 with IRF-1 may alter not only the cellular responses to IFNs and viral infection but also a varietyof cellular responses not related to viral infection. IRF-1 isa prototype transcription factor that can modulate the expressionof a number of cellular genes, including those involved in theregulation of cell growth, susceptibility to transformation, andapoptosis. It was shown that the ectopic expression of IRF-1 inhibitscell growth, while overexpression of IRF-2 (35) and vIRF-1 (15)causes the oncogenic transformation in NIH 3T3 cells. It was alsoshown that the overexpression of IRF-1 could reverse the IRF-2-transformedNIH 3T3 cells to a normal phenotype (18). These data indicatethat the balance between IRF-1 and its antagonists may significantlyaffect cells growth. Notably, we have shown in this study thatthe vIRF-1-overexpressing NIH 3T3 cells are resistant to TNF- $alpha$ -inducedapoptosis. As previously reported, similar observations were alsomade with cells that contained homozygous deletion of IRF-1 (22)or in which the expression of IRF-1 was impaired (25). It wasshown that IRF-1 has an essential role in the regulation of theexpression of p21^waf cell cycle inhibitor. The promoter of p21^waf contains three potential IRF-1 binding sites and can be activatedby IRF-1. Basal expression of p21^waf was found to be dramatically decreased both in IRF-1^/ mouse fibroblast (50), as well as in NIH 3T3 cells overexpressingvIRF-1 (15) that were tumorigenic. It remains to be determinedwhether the observed resistance of NIH 3T3/vIRF-1 cells to TNF- $alpha$ -inducedapoptosis could be entirely related to deregulation of p21^waf or whether vIRF-1 by targeting CBP/p300 coactivator and displacingbinding of IRF unrelated transcription factors downregulates theexpression of proapoptotic genes as demonstrated recently in NIH3T3 expressing catalytic variant of PKR (5).

In conclusion, our results suggest that, by inserting IRF-like ORF into viral genome, HHV-8 developed an effective mechanismof viral mimicry which allows the virus to both overcome the inductionof type I IFN genes and to inhibit their functions. However, theexpression of vIRF-1 can result in changes not directly relatedto viral mimicry. As shown in the present study, there are atleast two mechanisms by which vIRF-1 modulates expression of cellulargenes. First, the association of vIRF-1 with the cellular multifunctionalfactor IRF-1 alters its functional diversity in multiple cellularresponses. Second, competitive binding of vIRF-1 with specifictranscription factors to a discrete domain of the transcriptionalcoactivator p300 may also affect an expression of IRF-1-independentgenes and result in a more general inhibition of gene transcription.Therefore, it will be important to identify target genes expressionof which is modulated by vIRF-1.

	ACKNOWLEDGMENTS

This study was supported by grants CA76946 (NCI) and AI19737 (NIAID) from the National Institutes of Health (P.M.P.).

We thank J. Nicholas for the $lambda$ phage library and the BCBL-1 cells and J. Hiscott, T. Taniguchi, and K. Ozato for the p65,IRF-1, IRF-2, and ICSBP expression plasmids, respectively, andG. Nabel for p300 plasmids. We also thank R. Pine for sharinghis unpublishedresults.

	FOOTNOTES

^* Corresponding author. Mailing address: The Johns Hopkins University, Oncology Center, 418 N. Bond St., Baltimore, MD 21231-1001.Phone: (410) 955-8871. Fax: (410) 955-0840. E-mail: parowe{at}jhmi.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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