Assembly of a Functional Beta Interferon Enhanceosome Is Dependent on ATF-2-c-jun Heterodimer Orientation

doi:10.1128/MCB.20.13.4814-4825.2000

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Molecular and Cellular Biology, July 2000, p. 4814-4825, Vol. 20, No. 13
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Assembly of a Functional Beta Interferon Enhanceosome Is Dependent on ATF-2-c-jun Heterodimer Orientation

James V. Falvo,¹ Bhavin S. Parekh,¹^, Charles H. Lin,¹^,² Ernest Fraenkel,¹ and Tom Maniatis¹^,^*

Department of Molecular and Cellular Biology¹ and Department of Chemistry and Chemical Biology,² Harvard University, Cambridge, Massachusetts 02138

Received 10 November 1999/Returned for modification 16 December 1999/Accepted 29 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Heterodimeric transcription factors, including the basic region-leucine zipper (bZIP) protein ATF-2-c-jun, are well-characterizedcomponents of an enhanceosome that mediates virus induction ofthe human beta interferon (IFN- $beta$ ) gene. Here we report that withinthe IFN- $beta$ enhanceosome the ATF-2-c-jun heterodimer binds in aspecific orientation, which is required for assembly of a complexbetween ATF-2-c-jun and interferon regulatory factor 3 (IRF-3).We demonstrate that correct orientation of the ATF-2-c-jun bindingsite is required for virus induction of the IFN- $beta$ gene and forIRF-3-dependent activation of a composite ATF-2- c-jun-IRF sitein the IFN- $beta$ promoter. We also show that in vitro the DNA-boundATF-2-c-jun heterodimer adopts a fixed orientation upon the bindingof IRF-3 at an adjacent site in the IFN- $beta$ enhancer and that theDNA-binding domain of IRF-3 is sufficient to mediate this effect.In addition, we show that the DNA-binding domain of ATF-2 is necessaryand sufficient for selective protein-protein interactions withIRF-3. Strikingly, in vivo chromatin immunoprecipitation experimentswith IFN- $beta$ reporter constructs reveal that recruitment of IRF-3to the IFN- $beta$ promoter upon virus infection is dependent on theorientation of the ATF-2-c-jun heterodimer binding site. Theseobservations demonstrate functional and physical cooperativitybetween the bZIP and IRF transcription factor families and illustratethe critical role of heterodimeric transcription factors in formationof the IFN- $beta$ enhanceosome.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The expression of specific sets of genes in response to different extracellular signals is required for regulation of theimmune and inflammatory responses. Most extracellular signalsactivate a number of different transcription factors. Moreover,individual transcription factors can be activated in responseto many different signals. Thus, a mechanism for integrating signalsand transcription factors is required for normal cellular regulation.One mechanism for signal integration is the assembly of multicomponenttranscriptional enhancer complexes known as enhanceosomes (4).The coordinate activation of specific sets of transcription factors,their assembly into a higher-order complex, and their interactionwith coactivator proteins and components of the basal transcriptionmachinery ensure that the appropriate genes are activated in responseto a given signal. An excellent example of this is the activationof the beta interferon (IFN- $beta$ ) gene in response to virus infection(35).

Type I IFNs, including IFN- $beta$ , are synthesized and secreted by mammalian cells in response to virus infection and thus mediatethe establishment of an antiviral state (59). Induction of IFN- $beta$ gene transcription depends on a remarkably compact enhancer region,spanning a region between 105 and 55 bp upstream of the startsite of mRNA transcription. Indeed, virtually every DNA base pairin this region is contacted by a transcription factor throughthe major or minor groove. Induction of IFN- $beta$ transcription doesnot require de novo protein synthesis; rather, it occurs throughvirus-mediated posttranslational modification of transcriptionfactors, which bind to specific positive regulatory domains (PRDs)within the IFN- $beta$ promoter (Fig. 1A). A heterodimer of NF- $kappa$ B p50and p65 and a heterodimer of the basic region-leucine zipper (bZIP)proteins ATF-2 and c-jun bind to PRDII and PRDIV, respectively.PRDIII and PRDI are recognized by a protein complex containingIFN regulatory factor 3 (IRF-3) and IRF-7, but the stoichiometryof these proteins within the enhanceosome is not known (35).Two molecules of the high-mobility-group protein I(Y) [HMGI(Y)]also recognize the IFN- $beta$ enhancer, one each at PRDII and PRDIV,and bind cooperatively with NF- $kappa$ B and ATF-2-c-jun (15, 17,53, 65). A formaldehyde cross-linking and chromatin immunoprecipitation(ChIP) procedure has been used to detect transcription factorsthat bind the endogenous IFN- $beta$ promoter before and after virusinfection. These studies have shown that NF- $kappa$ B p50 is bound tothe IFN- $beta$ promoter prior to virus induction, but the full complementof activators $---$ ATF-2, c-jun, IRF-3, IRF-7, and NF- $kappa$ B p50 and p65 $---$ associateswith the promoter following virus infection (61).

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FIG. 1. Orientation of asymmetric ATF-2-c-jun binding sites in the context of the IFN- $beta$ enhancer is critical for virus induction. (A) Diagram of the binding sites for ATF-2-c-jun, IRF proteins, NF- $kappa$ B, and HMGI(Y) in the IFN- $beta$ enhancer. (B) Nucleotide sequences and activities of $-$ 110 IFN- $beta$ enhancer reporters used in this study. Numbering indicates nucleotide positions relative to the start site of transcription in the wild-type promoter. The core 5' and 3' half-sites in each sequence are shaded. (C) Histogram showing the levels of CAT activities from uninduced and Sendai virus-induced HeLa cells transfected with the indicated reporters. Average results of multiple independent experiments (total number as noted) are shown for each reporter; error bars indicate the standard error of the mean. For each experiment, wild-type (WT) reporter was included and wild-type virus-induced activity was normalized to 100. The average CAT activities (percent conversion of unacetylated to acetylated chloramphenicol) for uninduced and virus-induced wild-type reporter (± standard error of the mean) were 1.10 ± 0.280 and 10.68 ± 3.68, respectively.

Recently, the CREB-binding protein (CBP) and p300 coactivator proteins were shown to be required for IFN- $beta$ expression (30,36, 49, 61, 67). Following virus infection, CBP and p300associate with IRF-3 (30, 31, 49, 61, 62, 67) andIRF-7 (61). Recruitment of CBP and p300, in turn, is requiredfor the recruitment of components of the preinitiation complexto the promoter, including TFIIB, TFIIA, and TFIID (23, 24).CBP and p300 are histone acetyltransferases, which promote transcriptionvia the formation of open chromatin structure (52); indeed,histones at the IFN- $beta$ promoter become hyperacetylated after virusinfection (40). Thus, a specific set of transcription factors,coactivators, and the architectural protein HMG I(Y) assembleinto a higher-order nucleoprotein complex, the enhanceosome, atthe IFN- $beta$ enhancer and activate transcription of the IFN- $beta$ genein response to virus infection (4, 35).

Assembly of the IFN- $beta$ enhanceosome depends on proper spatial alignment and orientation of the PRDs along the DNA helix, andformation of the complex is accompanied by a remodeling of DNAconformation (17, 55). Moreover, multiple protein-proteininteractions have been identified among the components of theenhanceosome (15, 36, 53, 66), suggesting that the specificpositioning of transcription factors within the complex is criticalfor enhanceosome assembly. The half-sites of PRDII and PRDIV arein fact asymmetric, and in the case of PRDII, the NF- $kappa$ B p50 subunitrecognizes the 5' half-site and the p65 subunit recognizes the3' half-site (55, 57). The positioning of heterodimeric transcriptionfactors thus presents a potential basis for correct assembly ofthe IFN- $beta$ enhanceosome.

Here, we report the critical role of ATF-2-c-jun heterodimer orientation in the assembly and function of the IFN- $beta$ enhanceosome.Using site-directed mutagenesis of IFN- $beta$ reporter constructs,we demonstrated that the orientation of cyclic AMP response element(CRE) consensus and nonconsensus half-sites within PRDIV is criticalfor virus induction and that asymmetric ATF-2-c-jun sites fromother gene promoters can exhibit similar effects in the contextof the IFN- $beta$ promoter. We also show that PRDIV and PRDIII-I functionas a strongly virus-inducible composite element (PRD431), criticallydependent on the orientation of PRDIV, when placed upstream froma heterologouspromoter.

Using site-specific photo-cross-linking of recombinant proteins to the IFN- $beta$ promoter, we have examined the orientation ofthe ATF-2-c-jun heterodimer bound to PRDIV. Although ATF-2-c-junbinds to PRDIV with only modest intrinsic preference in orientation,this orientation is fixed in the presence of IRF-1 or IRF-3, suchthat c-jun and ATF-2 recognize the 5' consensus and 3' nonconsensushalf-sites, respectively, which are in turn distal and proximalto the IRF site. Furthermore, we show that the DNA-binding domainof IRF-3 and the IRF binding site adjacent to PRDIV are requiredfor fixing of ATF-2-c-jun heterodimer orientation by IRF-3. Usingglutathione S-transferase (GST) association assays, we found thatATF-2 preferentially interacts with IRF-3, consistent with thepositions predicted by the cross-linking studies. Strikingly,the 66-amino-acid bZIP DNA-binding domain of ATF-2 is necessaryand sufficient for interaction with IRF-3. We thus demonstratedirect interactions between proteins of the IRF and bZIPfamilies.

An interesting result from our in vitro studies is that IRF-3 can fix the orientation of ATF-2-c-jun at PRD431 only when PRDIVis in the wild-type orientation. IRF-1, on the other hand, whichexhibits equal affinity for ATF-2 and c-jun in GST associationassays, fixes ATF-2-c-jun in the opposite orientation when PRDIVis reversed, such that c-jun is proximal to the IRF site. Consistentwith this finding, transfection of exogenous IRF-3 activates aPRD431 reporter with PRDIV in the wild-type but not the reverseorientation, while exogenous IRF-1 activates both reporters, indicatingthat formation of a functional IRF-3-ATF-2-c-jun complex at theIFN- $beta$ promoter in vivo depends on the orientation of PRDIV. Wehave directly examined the effect of PRDIV orientation on thebinding of transcription factors at the IFN- $beta$ promoter in vivousing ChIP assays of cells cotransfected with wild-type and mutantIFN- $beta$ promoter constructs. Our modification of the ChIP techniquepermits direct comparison of the binding of endogenous factorsto wild-type and mutant forms of gene promoters of interest. Remarkably,IRF-3 is recruited to the wild-type IFN- $beta$ promoter but not anIFN- $beta$ promoter with the ATF-2-c-jun binding site in reverse orientation.Thus, we have demonstrated that the orientation of a heterodimerictranscription factor within the context of an enhancer can becritical for recruitment of other transcription factors to a functionalenhancer complex. Given the importance of heterodimeric transcriptionfactors in the activation of numerous genes, other functionalnucleoprotein complexes may prove to exhibit transcription factororientation-dependentassembly.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmids. Site-directed mutagenesis of the $-$ 110 IFN- $beta$ CAT (chloramphenicol acetyltransferase) reporter at PRDIV was performed by a two-stepPCR method described previously (53). The XbaI-BspDI fragmentsof the PCR products were subcloned into the $-$ 110 IFN- $beta$ CAT reporter.The PRD431 and PRD4rev31 SEAP (secreted alkaline phosphatase)constructs were made by subcloning one to three copies of theoligonucleotides 5'-CTAGCTAAATGTAAATGACATAGGAAAACTGAAAGGGAGAAGTGAAAGTGTctag-3'and 5'-CTAGCTAAATGTAAACTATGTCAGAAACTGAAAGGGAGAAGTGAAAGTGTctag-3',respectively, into the XbaI site of E1b TATA CAT (29). The XhoI-EcoRIfragment was then subcloned into pSEAP2-Basic (Clontech). ThePRD31 SEAP constructs were made by subcloning the XhoI-EcoRI fragmentfrom the PRD31 CAT reporters (61) into pSEAP2-Basic. All sequenceswere verified either by dideoxy sequencing or with an ABI 310Genetic Analyzer (Perkin-Elmer).

The expression vectors pcDNA1-ATF-2, pcDNA1-c-jun, and pcDNA1-IRF-1 have been described previously (15, 54). The IRF-3E₅ expression vector, which contains serine-to-glutamic acid changesat positions 396, 398, 402, and 405 and a threonine-to-glutamicacid change at position 404, was prepared from wild-type H₆-hIRF-3expression vector (61) by standard PCR mutagenesis (C. H. Lin,M. G. Wathelet, and T. Maniatis, unpublisheddata).

Cell culture and transfections. HeLa and P19 cells (American Type Culture Collection, Manassas, Va.) were maintained in Dulbecco's modified Eagle medium (DMEM)supplemented with 10% fetal bovine serum, 2 mM L-glutamine, 100U of penicillin/ml, and 100 µg of streptomycin/ml in a 37°C incubatorat 5% CO₂. Transfections in HeLa cells were performed in six-wellplates using Lipofectamine (Life Technologies) at 25 µg/ml accordingto the manufacturer's protocol and induced with Sendai virus asdescribed elsewhere (61). For each experiment, 1.5 µg of CATor SEAP reporter plasmid was used along with 0.5 µg of $beta$ -galactosidasecontrol reporter plasmid (pCMV $beta$ ; Clontech). P19 cells were seededin six-well plates (3 × 10⁵ cells per well) and grown to approximately 75% confluency. Transfectionswere performed using FuGene6 (Boehringer Mannheim) at 2 µl ofreagent per ml of medium according to the manufacturer's protocol,and media and cells were assayed 48 h posttransfection. PRD431₂SEAP or PRD4rev31₂ SEAP reporters (200 ng) were cotransfectedwith pCMV $beta$ (200 ng), 270 ng of pcDNA1, 30 ng of ATF-2-c-jun expressionvector, and up to 300 ng of IRF expression vector as indicatedin the relevant figure legend; the total amount of DNA was keptconstant with pcDNA1 (Invitrogen). Extracts were assayed for $beta$ -galactosidaseactivity or CAT activity as described elsewhere (48). ColorimetricSEAP assays were performed essentially as described previously;DMEM lacking phenol red was used following transfection (9).

Recombinant proteins and protein-DNA photo-cross-linking. Proteins were expressed as hexahistidine or GST fusions in Escherichia coli BL21(DE3) using the expression vectors pET15-p50,pET25-p65, pET-25-HMGI, pET25-IRF-1, pGEX-IRF-3, pET15-ATF-2₁₉₅,and pET15-c-jun and purified as described elsewhere (50, 53).

Oligonucleotides of the PRDIV site with or without an intact IRF site at PRDIII (5'-AAT*GTAAATGACATAGGAAA*CTGA-3' or 5'-T*GTAAATGACATAGTCTAA*C-3'),the PRDII site (see Fig. 4A), or the IFN- $beta$ promoter containingsingle phosphorothioate substitutions at the positions indicatedby the asterisks on the sense (5') or antisense (3') strand weresynthesized by Operon Technologies. p-Azidophenacyl (AzP) bromide(Sigma) was coupled to the phosphorothioate moieties as follows.Phosphorothioate-substituted single-stranded oligonucleotide (1nmol) was incubated in 100 µl (final volume) of 20 mM NaHCO₃ (pH9.0)-45% dimethyl sulfoxide-5 mM AzP bromide (diluted from a 0.33M stock in methanol) for 2 h at room temperature in the dark.The reaction mixture was filtered through 2 columns of SephadexG-50 (Pharmacia Biotech) by centrifugation, ethanol precipitated,and resuspended in 15 µl of H₂O. The DNA was then labeled with2 µl of [ $gamma$ -³²P]ATP and 1 µl of polynucleotide kinase in 1× PNK buffer (NewEngland BioLabs) for 1 h at 37°C. The labeled DNA was then purifiedon a G-50 column as before, 0.5 nmol of the complementary strandwas added, and the oligonucleotides were annealed by heating to85°C and cooling to roomtemperature.

Approximately 100 pmol of DNA was then used in binding reactions with the recombinant proteins. The binding reaction mixturecontained 10 mM Tris HCl (pH 7.5), 50 mM NaCl, 1 mM EDTA, 5% glycerol,0.1% NP-40, and 100 µg of bovine serum albumin (BSA)/ml. All proteinswere titrated on the DNA probes to ensure minimally saturatingconditions as determined by electrophoretic mobility shift assay(B. S. Parekh and T. Maniatis, unpublished data). After incubationof the proteins and probes for 20 min, reactions were exposedto UV radiation on ice for 5 min with an Ultra-Lum UVC-515 UVmultilinker set at 310 nm; wavelengths below 300 nm were filteredout using a polystyrene culture dish. After the cross-linkingreaction, loading buffer containing sodium dodecyl sulfate (SDS),formamide, and bromophenol blue was added, and reactions wereresolved by SDS-polyacrylamide gel electrophoresis (SDS-PAGE)on 10% gels with molecular weight markers (Bio-Rad). Gels weredried and visualized byautoradiography.

Protein-protein interaction assays. GST fusion expression vectors for ATF-2₁₉₅ and c-jun (15) and the series of GST-ATF-2 constructs used in the ATF-2 deletionstudies, GST-ATF-2(1-505), GST-ATF-2(1-349), GST-ATF-2(350-505),and GST-ATF-2(350-415) (32), have been described previously.GST and GST fusion proteins were expressed in E. coli BL21 cells,purified as recommended by the manufacturer (Pharmacia), and dialyzedagainst 1× phosphate-buffered saline-0.1% Triton X-100-10% glycerol.³⁵S-labeled full-length or truncated derivatives of hexahistidine-taggedIRF-3 protein were synthesized by in vitro transcription-translationof pcDNA constructs in rabbit reticulocyte lysate using a TnTkit (Promega). GST or the GST fusion proteins were immobilizedto glutathione-agarose beads and incubated with in vitro-translated³⁵S-labeled proteins for 2 h at 4°C in binding buffer (50 mM KCl,20 mM Tris [pH 8.0], 0.2% NP-40, 50 µg of ethidium bromide/ml,5 mM dithiothreitol, 0.2% BSA), followed by two washes with bindingbuffer and two washes with binding buffer without BSA. Interactionswere then analyzed by SDS-PAGE on 10%gels.

ChIP assays. The ChIP assays were modified from the original protocol (38, 61) as follows. HeLa cells were seeded at 2.5 × 10⁶ cells per 10-cm-diameter plate (eight plates per condition, uninducedand virus induced), grown to approximately 60% confluency, andtransfected with 12 µg of $-$ 110 IFN- $beta$ SEAP and 12 µg of $-$ 110 IFN- $beta$ PRDIV reverse CAT per plate as described above. After inductionwith Sendai virus for 6 h, cells were fixed by adding formaldehydeto 1% (final concentration; diluted from a 10% stock in 100 mMNaCl, 1 mM EDTA, 0.5 mM EGTA, and 50 mM HEPES [pH 8.0]) for 30min at 37°C, followed by addition of glycine to 125 mM (finalconcentration) to quench the reaction. Fixed cells were washedtwice in phosphate-buffered saline, harvested, and resuspendedin 10 ml of ice-cold lysis buffer (0.25% Triton X-100, 0.5% NP-40,10 mM EDTA, 0.5 mM EGTA, 10 mM Tris HCl [pH 8.0], 1 mM phenylmethylsulfonylfluoride [PMSF]) for 10 min. Nuclei were pelleted by centrifugationand washed successively at room temperature in 0.2 mM NaCl-1 mMEDTA-0.5 mM EGTA-10 mM Tris HCl-1 mM PMSF and in 1 mM EDTA-0.5mM EGTA-10 mM Tris HCl-1 mM PMSF. Samples were then sonicated10 times with a 20-s constant burst using a Branson Sonifier 450.Supernatants were then purified by using a CsCl gradient and dialysiswith 1 mM EDTA-0.5 mM EGTA-10 mM Tris HCl-5% glycerol. Approximately50 µg of purified chromatin samples was immunoprecipitated with1 µg of anti-ATF-2, anti-c-jun, anti-NF- $kappa$ B p50, anti-NF- $kappa$ B p65(Santa Cruz Biotechnology), or anti-IRF-3 (SL14) (61). DNA isolatedfrom immunoprecipitated material following reversal of formaldehydecross-linking was amplified by PCR (cycles of 1 min each at 94,60, and 72°C) using T7 and CAT reverse primer or primers flankingthe pSEAP2 multiple cloning site (Clontech). PCR cycles were titratedto ensure that amplification was in the linear range. Formaldehydecross-linking was reversed for 50 µg of purified chromatin asa control for amplification of the transfected DNA by PCR. PCRproducts were resolved on 1.5% agarose gels and visualized usinga Stratagene Eagle Sight imagingsystem.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

The orientation of an asymmetric ATF-2-c-jun site is required for virus induction of the IFN- $beta$ enhancer. The central DNA sequence of PRDIV contains an asymmetric ATF/CREB site, which upon virus induction is bound by a heterodimerof ATF-2 and c-jun (14, 15, 61). The core ATF-2-c-jun bindingsite, 5'-ATGACATAGG-3', consists of a half-site (underlined) identicalto that of the consensus CRE, 5'-ATGACGTCAT-3' (21), and a nonconsensushalf-site. We previously speculated that c-jun and ATF-2 mightinteract specifically with the consensus and nonconsensus half-sitesof PRDIV (17), because both proteins can bind the CRE as homodimersbut only ATF-2 can bind PRDIV as a homodimer (13, 15). Totest the functional importance of the relative positions of theCRE consensus and nonconsensus half-sites, we reversed the orientationof the core ATF-2-c-jun site in PRDIV in the context of the IFN- $beta$ enhancer fused to the CAT gene. All mutations were made withinthe central eight base pairs of the site, preserving the flankingsequences (Fig. 1B). Reversal of the site results in a sharp decreaseof virus induction of the IFN- $beta$ reporter gene (Fig. 1C), eventhough it does not impair binding of recombinant ATF-2-c-jun heterodimerto the reporter (see Fig. 4 and 5; J. V. Falvo and T. Maniatis,unpublished data). It is important to note that this decreaseis not the consequence of the T-to-C mutation near the HMGI(Y)binding site at the 5' end of PRDIV in the reverse construct.An IFN- $beta$ enhancer reporter construct bearing a G-to-A mutationat position $-$ 91 exhibits wild-type inducibility by virus (Fig.1C) (14), and reversal of the site abrogates inducibility whilepreserving the 5' PRDIV sequence (Fig. 1C).

Substitution of the ATF-2-c-jun site in PRDIV with a consensus CRE site in the context of the IFN- $beta$ enhancer results in amarked increase in both basal and virus-induced levels of activity(Fig. 1C). This is consistent with the observations that singlebase substitutions in PRDIV that result in a more CRE-like sequenceresult in higher levels of virus induction of IFN- $beta$ reporters(14) and that ATF-2-c-jun binds with higher affinity to theCRE than to PRDIV (13). Furthermore, replacement of the PRDIVATF-2-c-jun site with an AP-1 site results in lower levels ofvirus inducibility (Fig. 1C), which is consistent with the loweraffinity of ATF-2-c-jun for the AP-1 site compared to the CREsite (19).

The asymmetry of the ATF-2-c-jun site within PRDIV is a feature observed in functional ATF-2-c-jun binding sites in the promoterregions of a number of genes, including c-jun (58), the urokinasegene (10), and the E-selectin gene (46). In addition, thepalindromic ATF-2-c-jun binding site in the tumor necrosis factoralpha (TNF- $alpha$ ) promoter (TNF- $alpha$ CRE) varies from the consensus CREat its central dinucleotide (37, 56). The ATF-2-c-jun bindingsites from the c-jun (cjun2), urokinase, and E-selectin gene promoters,but not the TNF- $alpha$ CRE, are all functional in the context of theIFN- $beta$ enhancer, resulting in wild-type levels of virus induction(Fig. 1C). Notably, the sites from the c-jun and urokinase genesare not functional when placed in the opposite orientation, whilethe E-selectin site remains functional in reverse orientation(Fig. 1C). None of the mutations impaired binding of ATF-2-c-junto the promoter (Falvo and Maniatis, unpublished). When the sitestested in the context of the IFN- $beta$ enhancer are examined, a correlationemerges between the polarity of the ATF-2-c-jun site, includingthe central dinucleotide, and virus induction of the reporter.First, in the functional reporters a CRE core half-site (5'-TGA-3')is present at the 5' position. In the case of the ATF-2-c-junsites in PRDIV, PRDIV G( $-$ 91)A, and cjun2, the CRE core half-siteis in the 5' position and a nonconsensus core half-site is inthe 3' position, and reversal of these sites results in a nonfunctionalreporter (Fig. 1B). When both half-sites are CRE core half-sites,as is the case of the urokinase, E-selectin, and TNF- $alpha$ ATF-2-c-junsites, the central dinucleotide appears to be a critical determinantof function. For all of the sites examined, functional reporterscontained purine-purine or pyrimidine-purine, but not pyrimidine-pyrimidineor purine-pyrimidine, as the central dinucleotide (Fig. 1B). Thus,the polarity of ATF-2-c-jun sites in the context of the IFN- $beta$ enhancer is a critical determinant of virusinducibility.

PRDIV and PRDIII-I function as a composite element in vivo. The PRDIV site and the neighboring PRDIII-I site are, in essence, a composite site for ATF-2-c-jun, HMGI(Y), and IRF-3 orIRF-7. Insertion of half a helical turn of DNA between PRDIV andPRDIII-I abolishes virus inducibility of the IFN- $beta$ enhancer, whileinsertion of a full helical turn of DNA preserves inducibility(55). To characterize the function of the PRDIV and PRDIII-Icomposite site (PRD431) in vivo, one to three copies of PRD431containing PRDIV in the forward or reverse orientation were placedupstream of the E1b TATA box minimal promoter (29) driving expressionof the SEAP gene. The activity of these constructs was comparedto that of isogenic reporters driven by two or three copies ofthe PRDIII-I site (61). Multimers of PRD431 were strongly virusinducible, while multimers of PRD4rev31 were much less inducible(Fig. 2). Thus, both in the context of the IFN- $beta$ enhancer andas a reiterated element before a heterologous promoter, PRDIVand PRDIII-I function as a composite virus-inducible element,critically dependent on PRDIV orientation.

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FIG. 2. PRDIV and PRDIII-I function as a composite element in vivo. SEAP activity in media from uninduced and Sendai virus-induced HeLa cells transfected with the indicated reporters is shown. Histograms display the average results of three independent experiments, and error bars indicate the standard error of the mean. Activity of SEAP reporters containing one to three copies of PRD31, PRD431, or PRD4rev31 is indicated.

Selective interactions between ATF-2 and IRF-3 are mediated by the bZIP region of ATF-2. Given the orientation-dependent functional cooperativity between the ATF-2-c-jun and IRF binding sites in PRDIV and PRDIII-I,we examined the possibility that ATF-2 and c-jun interact directlywith IRF proteins using GST association assays. We tested twoIRF proteins previously implicated in IFN- $beta$ regulation, IRF-1and IRF-3 (35). IRF-1 activates the IFN- $beta$ promoter in a cooperativefashion with ATF-2-c-jun, NF- $kappa$ B p50-p65, and HMGI in cotransfectionexperiments (55) and in vitro (24). The requirement of IRF-3for virus induction of the IFN- $beta$ gene in vivo has recently beendemonstrated by several laboratories (30, 49, 50, 61,67).

Full-length IRF-1 interacted to a similar extent with ATF-2 and c-jun, while full-length IRF-3 did not interact with ATF-2or c-jun (Fig. 3A). IRF-3 contains a C-terminal autoinhibitorydomain; relief of this intramolecular interaction by phosphorylationor truncation exposes its DNA-binding and protein-protein interactiondomains (31, 61). Indeed, a truncated form of IRF-3 lackingthis C-terminal domain interacts with ATF-2 but, strikingly, notwith c-jun. It is worth noting that when we compared the amountof retained IRF protein to input, the interaction between IRF-3and ATF-2 was consistently stronger (10 to 11% of input) thanthe interaction between IRF-1 and ATF-2 or c-jun (3 to 5% of input[Fig. 3A]).

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FIG. 3. Protein-protein interactions between ATF-2-c-jun and IRF proteins. (A) Selective interaction between IRF-3 and ATF-2. In vitro-translated, ³⁵S-labeled, hexahistidine-tagged IRF proteins were incubated with GST, GST-ATF-2 (murine ATF-2₁₉₅ splice variant), or GST-c-jun immobilized on glutathione-agarose beads. Protein that remained bound following washing is shown with 20% of the total ³⁵S-labeled fraction for comparison. (B) The bZIP region of ATF-2 is necessary and sufficient for interaction with IRF-3. GST association assays were performed as for panel A, with GST fusion proteins containing full-length human ATF-2 (amino acids 1 to 505; lane 3) or ATF-2 with the indicated deletions (lanes 4 to 6). These results are summarized schematically in panel C.

To further examine interactions between the activators bound at PRDIV and PRDIII-I, we mapped the region of ATF-2 that interactswith IRF-3 (Fig. 3B and C). As expected, the truncated IRF-3 proteininteracted with full-length ATF-2 (Fig. 3B, lane 3). Strikingly,deletion of the ATF-2 bZIP region abrogated interactions betweenATF-2 and IRF-3 (Fig. 3B, lane 4), while GST fusion proteins containingas few as 66 amino acids of the bZIP region retained the abilityto interact with IRF-3 (Fig. 3B, lanes 5 and 6). Thus, the DNA-bindingdomain of ATF-2 mediates its interaction with IRF-3.

IRF-1 and binding site orientation fix the orientation of ATF-2-c-jun heterodimer bound to the IFN- $beta$ enhancer. The experiments described above demonstrate specific ATF-2-c-jun-IRF interactions as well as the critical influence of ATF-2-c-junbinding site orientation on virus inducibility of the IFN- $beta$ enhancer.We next examined the effect of binding site orientation on theposition of the ATF-2-c-jun heterodimer itself, using recombinantproteins. We used a protein-DNA photo-cross-linking method inwhich a reactive AzP group is introduced into oligonucleotidesat specific positions in the phosphate backbone (27, 63).Recombinant proteins were incubated with modified, radioactivelylabeled DNA probes and exposed to UV light, and the cross-linkedprotein-DNA complexes were resolved by SDS-PAGE and visualizedby autoradiography. The suitability of this technique was confirmedby incorporating AzP groups at the 5' or 3' half-site of a PRDIIoligonucleotide and examining the photo-cross-linked product afterincubation with recombinant NF- $kappa$ B p50-p65 heterodimer. As expectedfrom earlier photo-cross-linking experiments with 5-bromodeoxyuridine-substitutedPRDII oligonucleotides (57), p50 bound specifically to the 5'half-site and p65 bound specifically to the 3' half-site (Fig.4A). Oligonucleotide probes consisting of the entire IFN- $beta$ enhancer,with wild-type sequence or with a reversed ATF-2-c-jun site atPRDIV, were synthesized to contain phosphorothioate substitutionsat positions flanking PRDIV at the 5' or 3' position. A set ofrecombinant proteins, including those sufficient for enhanceosomeassembly and activation of the IFN- $beta$ gene in vitro (24), wereprepared: NF- $kappa$ B p50 homodimer, p50-p65 heterodimer, and p65 homodimer;IRF-1; ATF-2 homodimer, c-jun homodimer, and ATF-2-c-jun heterodimer;and HMGI. We confirmed that ATF-2 homodimer and ATF-2-c-jun heterodimer,but not c-jun homodimer, bind to PRDIV (Parekh and Maniatis, unpublished).

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FIG. 4. IRF-1 fixes the orientation of ATF-2-c-jun at PRDIV in vitro. (A) Photo-cross-linking of NF- $kappa$ B p50-p65 to AzP-modified PRDII oligonucleotide as a control for cross-linking specificity. Recombinant p50-p65 heterodimer was incubated with radiolabeled PRDII probe bearing a single AzP group at the 5' or 3' half-site as indicated and resolved by SDS-PAGE. (B) Photo-cross-linking of ATF-2 (upper complex; top band in lane 8) and c-jun (lower complex) to the PRDIV site of the IFN- $beta$ enhancer in the presence or absence of other components of the enhanceosome. A radiolabeled oligonucleotide spanning the entire IFN- $beta$ promoter and bearing a single AzP group at the 5' half-site of PRDIV was used as a probe, and protein-DNA complexes were resolved by SDS-PAGE. The proteins included in the binding reaction prior to photo-cross-linking are indicated above the lanes, and relative positions of the proteins and the AzP group within the IFN- $beta$ enhancer are indicated schematically. The same experiment was performed using an IFN- $beta$ enhancer with AzP at the 3' half-site of PRDIV (C), using an IFN- $beta$ enhancer with the PRDIV reverse mutation and AzP at the 5' half-site (D), and using an IFN- $beta$ enhancer with the PRDIV reverse mutation and AzP at the 3' half-site (E).

The distinct molecular weights of the cross-linked ATF-2-DNA and c-jun-DNA complexes provided a rapid and sensitive methodof observing the effects of other IFN- $beta$ enhanceosome componentsupon ATF-2-c-jun heterodimer orientation (Fig. 4B to E). Surprisingly,ATF-2-c-jun bound to PRDIV with almost no specific orientation,although the CRE consensus half-site was slightly favored by c-jun,regardless of its orientation within the IFN- $beta$ promoter (Fig.4B to E, lanes 4). We next examined the effects of other componentsof the enhanceosome upon the orientation of ATF-2-c-jun. HMGI,NF- $kappa$ B p50, NF- $kappa$ B p65, and NF- $kappa$ B p50-p65 failed to influence thebinding orientation of ATF-2-c-jun (Figs. 4B to E, lanes 5 to8). IRF-1, however, was sufficient to fix the orientation of ATF-2-c-junsuch that regardless of the orientation of PRDIV in the probe,c-jun was bound exclusively to the consensus half-site and ATF-2was bound to the nonconsensus half-site (Fig. 4B to E, lanes 9).This is consistent with the ability of IRF-1 to interact withboth ATF-2 and c-jun (Fig. 3A). In complementary experiments,the ATF-2-c-jun heterodimer bound in a fixed orientation in thepresence of HMGI, IRF-1, and p50-p65, and removal of each component,with the exception of IRF-1, did not abolish this orientation(Figs. 4B and C, lanes 10 to 13; Fig. 4D and E, lanes 10 to 15).Thus, the combined effects of the orientation of the asymmetricPRDIV site and the presence of IRF-1 protein are critical forfixing the orientation of ATF-2-c-jun in the context of the IFN- $beta$ enhanceosome invitro.

Interaction of the IRF-3 DNA-binding domain with PRDIII fixes the orientation of the ATF-2-c-jun heterodimer at PRDIV. We next determined if IRF-3, like IRF-1, is necessary and sufficient to fix the orientation of ATF-2-c-jun bound to the IFN- $beta$ enhancer in vitro. A recombinant GST-IRF-3 fusion protein (50)was substituted for IRF-1 in the photo-cross-linking assays. Strikingly,IRF-3 is also necessary and sufficient to fix the orientationof ATF-2-c-jun on the wild-type IFN- $beta$ enhancer probe (Fig. 5A,lanes 4 to 15). In the wild-type orientation, the nonconsensushalf-site of PRDIV is adjacent to the IRF site, so ATF-2 is proximalto IRF-3. When PRDIV is placed in reverse orientation in the contextof the IFN- $beta$ enhancer, however, IRF-3 cannot fix the orientationof ATF-2-c-jun (Fig. 5B, lanes 4 to 14). This is consistent withthe observations that IRF-3, unlike IRF-1, selectively interactswith ATF-2 (Fig. 3A) and that IRF-3 and ATF-2-c-jun bind cooperativelyto the wild-type IFN- $beta$ enhancer but not to the IFN- $beta$ enhancerwith the PRDIV reverse mutation (T. H. Kim and T. Maniatis, unpublisheddata).

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FIG. 5. The DNA-binding domain of IRF-3 fixes the orientation of ATF-2-c-jun at PRDIV in vitro. (A) Photo-cross-linking of ATF-2 and c-jun to the PRDIV site of the IFN- $beta$ enhancer in the presence or absence of other components of the enhanceosome using an IFN- $beta$ enhancer probe with the AzP group at the 3' half-site of PRDIV as in Fig. 3C, using a GST fusion protein containing the DNA-binding domain of IRF-3 (amino acids 1 to 133). The same experiment was performed using an IFN- $beta$ enhancer with the PRDIV reverse mutation and the AzP at the 5' half-site (B). (C) Photo-cross-linking of ATF-2 and c-jun to a minimal PRDIV site in the absence (lanes 1 to 10) or presence (lanes 11 to 20) of an intact 3' IRF binding site from PRDIII. Radiolabeled oligonucleotides with AzP at the 5' half-site (lanes 1 to 5 and 11 to 15) or 3' half-site (lanes 6 to 10 and 16 to 20) were used as probes.

Our experiments with recombinant IRF-3 utilized the DNA-binding domain of the protein (amino acids 1 to 133), which when expressedby stable transfection is recruited along with the endogenouscomponents of the IFN- $beta$ enhanceosome during virus infection (40).Thus, we have established that the DNA-binding domain of IRF-3mediates its ability to fix the orientation of ATF-2-c-jun atPRDIV. The cross-linking experiments also indicated that bindingof IRF-3 to DNA was required to establish a fixed binding orientationof ATF-2-c-jun, as the presence of IRF-3 alone was not sufficientfor fixing ATF-2-c-jun orientation. This is of note because someproteins can influence the DNA-binding properties of bZIP transcriptionfactors by protein-protein interactions alone, such as hepatitisB virus X protein (34) and human T-cell lymphotropic virus type1 Tax protein (60). To examine this in detail, we performedphoto-cross-linking experiments with a minimal PRDIV oligonucleotidewith point mutations in the 3' IRF binding site (Fig. 5C, lanes1 to 10) and with a PRDIV oligonucleotide containing an intactIRF binding site (Fig. 5C, lanes 11 to 20). Remarkably, whileIRF-3 fails to fix ATF-2-c-jun heterodimer binding orientationto PRDIV in the absence of an IRF binding site (Fig. 5C, comparelanes 4 and 5 and lanes 9 and 10), the addition of an IRF bindingsite restores the ability of IRF-3 to fix ATF-2-c-jun bindingorientation (Fig. 5C, compare lanes 14 and 15 and lanes 19 and20). Thus, the ability of IRF-3 to determine the orientation ofATF-2-c-jun bound at PRDIV depends on the binding of IRF-3 tothe adjacent IRF binding site atPRDIII.

IRF-1 and IRF-3 activate PRD431 with differential dependence on ATF-2-c-jun binding site orientation. Our in vitro cross-linking experiments with IRF-1 and the IRF-3 DNA-binding domain indicate that while ATF-2-c-jun forms anoriented complex with IRF-1 on either the wild-type or PRDIV-reverseIFN- $beta$ promoter, this orientated complex only forms on the wild-typepromoter with IRF-3. This is, in turn, consistent with the observationsthat ATF-2-c-jun and IRF-3 bind cooperatively to the wild-typebut not PRDIV-reverse IFN- $beta$ promoter (Kim and Maniatis, unpublished),while binding of ATF-2-c-jun and IRF-1 to the IFN- $beta$ promoter isnot cooperative (55). These in vitro distinctions in interactionsbetween ATF-2-c-jun and the IRF proteins might be reflected inIRF-dependent transactivation of the PRD431 composite element;thus, we next examined the effects of ATF-2-c-jun binding siteorientation on transactivation mediated by full-length IRF-1 andIRF-3 invivo.

To uncouple IRF-1- and IRF-3-dependent transactivation from other virus-mediated activation pathways in vivo, we transfectedfull-length IRF-1 and IRF-3 into P19 embryonal carcinoma cells.These cells do not express IRF proteins (20) and have been usedto study IFN- $beta$ promoter-dependent activation in response to exogenousactivators (54, 55). IRF-3 contains a C-terminal autoinhibitorydomain which is phosphorylated in response to virus infection(30, 31, 61), so in these experiments we expressed a constitutivelynuclear form of IRF-3 containing phosphomimetic glutamic acidsubstitutions (Lin, Wathelet, and Maniatis,unpublished).

Transfection of increasing amounts of both IRF-1 (Fig. 6A) and IRF-3 (Fig. 6B) activates a minimal reporter consisting oftwo copies of PRD431. IRF-1 activates two copies of PRD4rev31to a lesser extent than that achieved with two copies of PRD431;IRF-3, however, essentially fails to activate two copies of PRD4rev31(compare Fig. 6A to Fig. 6B). Thus, IRF-3 activates the PRD431composite element only when the ATF-2-c-jun binding site is inthe correct orientation, while IRF-1 retains the ability to activatePRD431 if the ATF-2-c-jun binding site is in the reverse orientation,albeit to a lesser extent.

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FIG. 6. Activation of PRD431 and PRD4rev31 by IRF-1 and IRF-3. SEAP activity (absorbance at 410 nm after 16 h of incubation at 37°C) in media from murine P19 embryonal carcinoma cells cotransfected with PRD431₂SEAP or PRD4rev31₂SEAP reporters is shown. Empty vector (pcDNA1, 300 ng) or increasing amounts (10, 30, 100, or 300 ng) of IRF-1 (A) or IRF-3 (B) were cotransfected with 30 ng of ATF-2-c-jun expression vector; the amount of DNA was kept constant with additional pcDNA1. Histograms display the average results of three independent experiments, and the error bars indicate the standard error of the mean.

A correctly oriented ATF-2-c-jun heterodimer binding site is required to recruit IRF-3 to the IFN- $beta$ promoter in vivo. The ChIP assay has been used to detect the binding of endogenous and stably expressed exogenous transcription factors to theendogenous IFN- $beta$ promoter (40, 61). The assay can also beused to detect the binding of endogenous or exogenous factorsto transiently transfected reporter plasmids (25, 33). Totest the effect of reversal of the PRDIV ATF-2-c-jun core elementin vivo, we cotransfected wild-type ( $-$ 110 IFN- $beta$ SEAP) and PRDIV-reverse( $-$ 110 IFN- $beta$ PRDIVrev CAT) IFN- $beta$ reporters into HeLa cells andperformed ChIP assays on chromatin samples from uninduced andvirus-induced cells. Because the PCR products for the wild-typeand mutant reporter are amplified from the same immunoprecipitatedmaterial, this permits direct comparison of transcription factorbinding to each construct before and after virus infection invivo; relative levels of amplified product provide a readout forbinding. Control PCRs were performed with buffer (Fig. 7, lanes2 and 3) and with genomic DNA from untransfected HeLa cells (Fig.7, lanes 4 and 5) or from the transfected HeLa cells used in theimmunoprecipitations (Fig. 7, lanes 6 to 9).

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FIG. 7. ATF-2-c-jun binding site orientation-dependent recruitment of IRF-3 to the IFN- $beta$ promoter in vivo. HeLa cells were transiently cotransfected with a SEAP reporter containing the wild-type (WT) IFN- $beta$ promoter ( $-$ 110 IFN- $beta$ SEAP) and with a CAT reporter containing the PRDIV reverse mutant IFN- $beta$ promoter ( $-$ 110 IFN- $beta$ PRDIVrev CAT) and were left uninduced or treated with Sendai virus. Following formaldehyde cross-linking and chromatin purification, DNA immunoprecipitated with the indicated antibodies was amplified by PCR using primers specific for $-$ 110 IFN- $beta$ SEAP or $-$ 110 IFN- $beta$ PRDIVrev CAT as indicated (lanes 10 to 29). PCR product amplification from immunoprecipitated material with specific primers correlates with protein binding to the indicated reporter. A 123 bp ladder (Life Technologies) is included as a marker (lane 1). Control PCRs with buffer or genomic DNA from untransfected and transfected HeLa cells are included as controls (lanes 2 to 9).

As shown in Fig. 7, ATF-2 (lane 11), c-jun (lane 15), IRF-3 (lane 19), and NF- $kappa$ B p50 and p65 (lanes 23 and 27) associate withtransfected wild-type IFN- $beta$ promoter following virus infection,as is the case with the endogenous gene (40, 61). Bindingof NF- $kappa$ B p50 is not apparent with the transfected promoter priorto virus infection (Fig. 7, lane 22), in contrast to the endogenouspromoter (40, 61), possibly reflecting the influence of endogenouschromatin structure and/or the high levels of reporter DNA presentfollowing transient transfection. Strikingly, after virus infectionevery transcription factor except for IRF-3 (Fig. 7, lane 21)associates with the transfected IFN- $beta$ promoter containing a reversedPRDIV ATF-2-c-jun site. This demonstrates that the orientationof the ATF-2-c-jun binding site is critical for recruitment ofIRF-3 to the IFN- $beta$ promoter upon virusinfection.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Heterodimerization of transcription factors plays a critical role in the regulation of eukaryotic gene transcription, providinga wide range of combinations of factors for temporal and stimulus-specificpatterns of gene expression. Indeed, homodimers and heterodimersmay have opposite effects on gene expression, as illustrated bythe positive and negative effects of the c-jun homodimer and thec-fos-c-jun heterodimer, respectively, on the function of a compositeglucocorticoid response element (11). At the level of DNA recognition,binding site affinity or site specificity of a heterodimeric complexmay differ from that of a homodimeric complex. In some cases,heterodimerization either permits DNA binding, as is the casewith dimerization of myc with Max (2) and c-fos with c-jun(43), or prevents DNA binding, as is the case with Id proteinsheterodimerizing with E-box proteins (1).

Heterodimerization can also modulate affinity for a single binding site: dimerization of c-jun with c-fos or with ATF-2 specifiesbinding to the AP-1 or the CRE site, respectively (19), anddimerization of c-jun with ATF-2 permits recognition of PRDIVby c-jun (15). Half-site spacing and asymmetry within a DNA-bindingsite can fix the binding orientation of its cognate transcriptionfactor. This is elegantly illustrated by the binding of differentheterodimeric combinations of nuclear hormone receptors to specificresponse elements, such that spacing between direct repeats determinesthe compositions of the bound heterodimer (45). DNA-directedbinding orientation is also observed in the binding polarity ofthe NF- $kappa$ B p50-p65 heterodimer, which is dictated by half-sitesin the $kappa$ B motif (5, 54, 57). The structural flexibilityof sequences flanking the AP-1 site has been linked to the orientationof bound c-fos-c-jun heterodimer (28). Furthermore, heterodimerorientation can be directed by the binding of another protein.A well-characterized example of this is the complex formed betweenNF-AT and the c-fos-c-jun heterodimer at a composite NF-AT-AP-1site in the interleukin-2 promoter, the distal antigen-receptorresponse element ARRE2 (44). Through extensive contacts betweenthe DNA-binding domains of the two proteins, NF-AT recruits c-fos-c-junto the ARRE2 site in a fixed orientation (6, 7, 12). Orientationof c-fos-c-jun within the NF-AT-AP-1 complex may be importantfor the establishment of enhanceosomes at the interleukin-2 promoterand promoters of other genes regulated by NF-AT-AP-1 elements,but the details of such higher-order complexes remain unclear(44, 47).

DNA-binding-site orientation has been associated with the transactivation potential of cognate heterodimeric transcriptionfactors. For example, the orientation of reiterated response elementsfor a vitamin D₃ receptor-retinoid X receptor heterodimer wasshown to have a strong influence on ligand-dependent inductionof transcription (51). Through the use of a yeast reporter system,transcriptional activation mediated by c-fos-c-jun bZIP domainsfused to heterologous activation domains and engineered to bindin a fixed orientation to AP-1 sites was also shown to be dependenton binding site orientation (8). In the human immunodeficiencyvirus type 1 long terminal repeat, the orientation of a $kappa$ B siteadjacent to an Sp1 site is critical for induction of the longterminal repeat by phorbol-12-mystrate-13-acetate or TNF- $alpha$ , consistentwith preferential interactions between Sp1 and the NF- $kappa$ B p65 subunit(41, 42). Similarly, in the IFN- $beta$ enhancer the orientationof the NF- $kappa$ B p50-p65 binding site, PRDII, is critical for inductionby virus (17).

Here, using in vitro and in vivo methods, we have shown that the orientation of a heterodimeric transcription factor determinesassembly and function of the IFN- $beta$ enhanceosome. We have shownthat the orientation of the ATF-2-c-jun binding site at PRDIVis critical for virus induction of the IFN- $beta$ gene and for thefunction of the ATF-2-c-jun-IRF composite element. Unlike theexamples described above, however, the orientation of ATF-2-c-junat PRDIV is not directed solely by binding site sequence or bythe influence of a protein bound at an adjacent site. Instead,the combined effect of the polarity of the ATF-2-c-jun bindingsite at PRDIV and IRF protein bound at PRDIII establishes an ATF-2-c-jun-IRFnucleoprotein complex in which the ATF-2-c-jun heterodimer adoptsa fixed orientation. When the ATF-2-c-jun-IRF complex containsIRF-1, which interacts with both ATF-2 and c-jun, the heterodimercan be fixed in either orientation depending on ATF-2-c-jun bindingsite polarity. On the other hand, if the complex contains IRF-3,which interacts selectively with ATF-2, the oriented complex formsonly when the ATF-2-c-jun binding site is in the wild-typeorientation.

This is consistent with our in vivo results with exogenous IRF-1 and IRF-3; IRF-1 can activate a PRD431 reporter when PRDIVis in either orientation, while IRF-3 can only activate the PRD431reporter when PRDIV is in the wild-type orientation. This indicatesthat a functional complex between ATF-2-c-jun and IRF-3 failsto form at PRD431 when PRDIV is in the reverse orientation, potentiallyfrom inhibition of IRF-3 binding by the configuration of thiscomposite site. This possibility is strongly supported by ourChIP assays with wild-type and mutant IFN- $beta$ reporters, which showthat recruitment of IRF-3 to the IFN- $beta$ promoter in vivo dependson ATF-2-c-jun binding site orientation. Thus, reversal of ATF-2-c-junbinding site orientation in the context of the IFN- $beta$ enhancerabolishes recruitment of IRF-3 in vivo and results in reversedATF-2-c-jun heterodimer orientation in the presence of IRF-1 invitro (Fig. 8A). The relative positions of transcription factoractivation domains are critical for recruitment of CBP and p300proteins to the IFN- $beta$ promoter; thus, a specific activation domainsurface appears to be required for correct interactions betweentranscription factors and coactivators in the context of the IFN- $beta$ enhanceosome (36). Reversal of the ATF-2-c-jun binding siteat PRDIV strongly inhibits transcriptional activation mediatedby the IFN- $beta$ promoter in vivo by virus infection, as we have shown,or by recombinant NF- $kappa$ B, ATF-2-c-jun, and IRF-1 in vitro (24).A critical effect of reversal of the ATF-2-c-jun binding sitethus appears to be alteration of the activation domain surfaceof the IFN- $beta$ enhanceosome, whether by a lack of IRF-3, which inturn fails to fix the orientation of ATF-2-c-jun, or by reversalof the orientation of ATF-2-c-jun in the presence of IRF-1. Reversalof ATF-2-c-jun orientation in the presence of IRF-1 may impairthe ability of these factors to recruit coactivators even at theisolated PRD431 element, as we have shown that exogenous IRF-1activates a PRD431 reporter more efficiently than a PRD4rev31reporter.

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FIG. 8. Model of ATF-2-c-jun-IRF complex formation at the IFN- $beta$ PRDIV and PRDIII elements. (A) Summary of the effect of IRF protein binding on ATF-2-c-jun heterodimer binding orientation. In the absence of IRF protein, ATF-2 (red) and c-jun (green) do not adopt a fixed orientation at PRDIV. In the presence of IRF-1, the position of the ATF-2-c-jun heterodimer becomes fixed such that ATF-2 is bound to the nonconsensus half-site and c-jun is bound to the nonconsensus half-site, regardless of whether PRDIV is in the wild-type or reverse orientation. In the presence of IRF-3, ATF-2-c-jun orientation is fixed only when PRDIV is in the forward orientation, and in vivo only the wild-type binding site orientation permits recruitment of IRF-3 to the IFN- $beta$ promoter. (B) Three-dimensional model of the ATF-2-c-jun-IRF-3 complex bound to the IFN- $beta$ promoter. The DNA-binding domains of IRF-1 bound to PRDI (16) and of the GCN4 homodimer bound to a CRE site (22) were used to model IRF-3 (orange) bound to PRDIII and ATF-2 (red) and c-jun (green) bound to PRDIV, respectively. The DNA recognition helix of IRF-3, which makes a close approach to ATF-2, is shown in cyan. The sequence from the amino acids in IRF-1 in this helix are shown in cyan, and those in the neighboring loop are shown in orange, along with the corresponding IRF-3 sequence. The N-terminal amino acid sequence of the GCN4 bZIP region and the corresponding amino acids from ATF-2 (starting with amino acid 350) and c-jun are also shown for comparison; green and red amino acids correspond to the positions found at the N terminus of the helix in the diagram. The figure was prepared using the program MOLSCRIPT (26).

Notably, we have shown that the DNA-binding domain of IRF-3 is sufficient to form an oriented ATF-2-c-jun-IRF complex in vitro.Consistent with this, the IRF-3 DNA-binding domain is recruitedto the IFN- $beta$ promoter along with endogenous ATF-2-c-jun in theapparent absence of CBP and p300, based on lack of localized histonehyperacetylation (40). This further illustrates the importanceof interactions among transcription factor DNA-binding domainsin the assembly of the IFN- $beta$ enhanceosome. Recruitment of IRF-3to the IFN- $beta$ promoter by ATF-2-c-jun and interactions betweenthe DNA-binding domains of these factors draw an interesting parallelto recruitment of IRF-4 (also known as Pip, LSIRF, NF-EM5, orICSAT) to B-cell-specific enhancers by the ETS domain proteinPU.1. The binding of phosphorylated PU.1 permits the formationof a stable ternary complex with IRF-4 on DNA (3). Phosphorylation-independentinteraction between the DNA-binding domains of the two proteinscontributes to the stability of the ternary complex, and correctspacing between the IRF and ETS binding sites is critical forcomplex formation (3, 64). A critical interaction, however,occurs between the phosphorylated PEST domain of PU.1 and a putativealpha-helical region in IRF-4, which in the absence of PU.1 inhibitsIRF-4 binding to DNA (3, 39).

Using protein-DNA co-crystal structures of related IRF and bZIP proteins, we have constructed a model of the ATF-2-c-jun-IRF-3complex bound to the IFN- $beta$ enhancer (Fig. 8B). The DNA-bindingdomain of IRF-1 (16) was placed at the 5'-GAAA-3' sequence inPRDIII. Given the strongly enhanced inducibility of the IFN- $beta$ enhancer when CRE was substituted for PRDIV (Fig. 1C), the structureof GCN4 homodimer bound to CRE (22) was placed at the sequence5'-TGACATAG-3'. Based on our results, we have designated the bZIPsubunits proximal and distal to IRF-3 as ATF-2 and c-jun, respectively.It is interesting that at the region of closest approach betweenthe two proteins, the bZIP N terminus and the junction of theIRF DNA recognition helix and a neighboring loop, there are severaldifferences in amino acid sequence between ATF-2 and c-jun andbetween IRF-1 and IRF-3. Differences may also exist in the overallstructure of DNA-bound IRF-1 and IRF-3, as has been observed forIRF-1 and IRF-2 (18). Such structural differences may underliethe distinct features that we have observed in the interactionsof IRF-1 and IRF-3 with ATF-2-c-jun. It is important to note thatbinding of IRF proteins at PRDIII does not simply fix an intrinsicpreferential orientation of ATF-2-c-jun at PRDIV; fixing of intrinsicDNA binding orientation would result in the same distributionof orientations found in the absence of IRF proteins. Within theATF-2-c-jun-IRF complex, interaction of IRF protein at PRDIIImust further influence the properties of ATF-2-c-jun binding orientationat PRDIV, for example, through changes in protein structure inducedby protein-protein contacts, alteration of DNA structure, or occlusionof DNA phosphate or base pair contacts. Structural analysis ofthe ATF-2-c-jun-IRF-3 complex bound to the PRDIV or PRDIII elementis currently in progress and promises to reveal the details ofthese interactions at the atomic level. Given the complexity ofmany gene regulatory elements, the emerging role for enhanceosomesin transcription, and the array of potential heteromeric factorsthat function in eukaryotic gene regulation, the orientation ofDNA-bound transcription factors as illustrated by the ATF-2-c-jun-IRFcomplex may have general importance in the establishment of functionalhigher-order nucleoproteincomplexes.

	ACKNOWLEDGMENTS

J.V.F. and B.S.P. contributed equally to thiswork.

We thank Paul Clemons for his work in the initial stages of the ATF-2-c-jun protein-DNA cross-linking experiments and AseemAnsari for suggesting the AzP bromide photo-cross-linking technique.The IRF-3 E₅ expression vector was prepared by C.H.L. and MarcWathelet. We thank Michael Green and Paula Pitha for generouslyproviding GST-ATF-2 and GST-IRF-3 expression vectors. We thankTae Hoon Kim for critical reading of the manuscript and for sharingunpublished observations, and we thank Judith Grisham for editorialassistance. Special thanks go to Stephen C. Harrison, in whoselaboratory E.F. is a postdoctoralfellow.

This work was supported by grant AI20642 from the NIH to T.M. J.V.F. acknowledges the support of a National Defense Scienceand Engineering Graduate Research Fellowship. E.F. is supportedby the Cancer Research Fund of the Damon Runyon-Walter WinchellFoundation Fellowship, DRG1547.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular and Cellular Biology, Harvard University, 7 Divinity Ave.,Cambridge, MA 02138. Phone: (617) 495-1811. Fax: (617) 495-3537.E-mail: maniatis{at}biohp.harvard.edu.

Present address: GeneSoft Inc., South San Francisco, CA94080.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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3. Brass, A. L., A. Q. Zhu, and H. Singh. 1999. Assembly requirements of PU.1-Pip (IRF-4) activator complexes: inhibiting function in vivo using fused dimers. EMBO J. 18:977-991[CrossRef][Medline].

4. Carey, M. 1998. The enhanceosome and transcriptional synergy. Cell 92:5-8[CrossRef][Medline].

5. Chen, F. E., D.-B. Huang, Y.-Q. Chen, and G. Ghosh. 1998. Crystal structure of p50/p65 heterodimer of transcription factor NF- $kappa$ B bound to DNA. Nature 391:410-413[CrossRef][Medline].

6. Chen, L., J. N. M. Glover, P. G. Hogan, A. Rao, and S. C. Harrison. 1998. Structure of the DNA-binding domains from NFAT, Fos and Jun bound specifically to DNA. Nature 392:42-48[CrossRef][Medline].

7. Chen, L., M. G. Oakley, J. N. M. Glover, J. Jain, P. B. Dervan, P. G. Hogan, A. Rao, and G. L. Verdine. 1995. Only one of the two DNA-bound orientations of AP-1 found in solution cooperates with NFATp. Curr. Biol. 5:882-889[CrossRef][Medline].

8. Chytil, M., B. R. Peterson, D. A. Erlanson, and G. L. Verdine. 1998. The orientation of the AP-1 heterodimer on DNA strongly affects transcriptional potency. Proc. Natl. Acad. Sci. USA 95:14076-14081[Abstract/Free Full Text].

9. Cullen, B. R., and M. H. Malim. 1992. Secreted placental alkaline phosphatase as a eukaryotic reporter gene. Methods Enzymol. 216:362-368[Medline].

10. De Cesare, D., D. Vallone, A. Caracciolo, P. Sassone-Corsi, C. Nerlov, and P. Verde. 1995. Heterodimerization of c-Jun with ATF-2 and c-Fos is required for positive and negative regulation of the human urokinase enhancer. Oncogene 11:365-376[Medline].

11. Diamond, M. I., J. N. Miner, S. K. Yoshinaga, and K. R. Yamamoto. 1990. Transcription factor interactions: selectors of positive or negative regulation from a single DNA element. Science 249:1266-1272[Abstract/Free Full Text].

12. Diebold, R. J., N. Rajaram, D. A. Leonard, and T. K. Kerppola. 1998. Molecular basis of cooperative DNA bending and oriented heterodimer binding in the NFAT1-Fos-Jun-ARRE2 complex. Proc. Natl. Acad. Sci. USA 95:7915-7920[Abstract/Free Full Text].

13. Du, W. 1993. Synergistic activation of the human interferon- $beta$ gene promoter. Ph.D. dissertation. Harvard University, Cambridge, Mass.

14. Du, W., and T. Maniatis. 1992. An ATF/CREB binding site is required for virus induction of the human interferon $beta$ gene. Proc. Natl. Acad. Sci. USA 89:2150-2154[Abstract/Free Full Text].

15. Du, W., D. Thanos, and T. Maniatis. 1993. Mechanisms of transcriptional synergism between distinct virus-inducible enhancer elements. Cell 74:887-898[CrossRef][Medline].

16. Escalante, C. R., J. Yie, D. Thanos, and A. K. Aggarwal. 1998. Structure of IRF-1 with bound DNA reveals determinants of interferon regulation. Nature 391:103-106[CrossRef][Medline].

17. Falvo, J. V., D. Thanos, and T. Maniatis. 1995. Reversal of intrinsic DNA bends in the IFN $beta$ gene enhancer by transcription factors and the architectural protein HMG I(Y). Cell 83:1101-1111[CrossRef][Medline].

18. Fujii, Y., T. Shimizu, M. Kusumoto, Y. Kyogoku, T. Taniguchi, and T. Hakoshima. 1999. Crystal structure of an IRF-DNA complex reveals novel DNA recognition and cooperative binding to a tandem repeat of core sequences. EMBO J. 18:5028-5041[CrossRef][Medline].

19. Hai, T., and T. Curran. 1991. Cross-family dimerization of transcription factors Fos/Jun and ATF/CREB alters DNA binding specificity. Proc. Natl. Acad. Sci. USA 88:3720-3724[Abstract/Free Full Text].

20. Harada, H., K. Willison, J. Sakakibara, M. Miyamoto, T. Fujita, and T. Taniguchi. 1990. Absence of the type I IFN system in EC cells: transcriptional activator (IRF-1) and repressor (IRF-2) genes are developmentally regulated. Cell 63:303-312[CrossRef][Medline].

21. Karin, M., Z.-G. Liu, and E. Zandi. 1997. AP-1 function and regulation. Curr. Opin. Cell Biol. 9:240-246[CrossRef][Medline].

22. Keller, W., P. König, and T. J. Richmond. 1995. Crystal structure of a bZIP/DNA complex at 2.2 Å: determinants of DNA specific recognition. J. Mol. Biol. 254:657-667[CrossRef][Medline].

23. Kim, T. K., T. H. Kim, and T. Maniatis. 1998. Efficient recruitment of TFIIB and CBP-RNA polymerase II holoenzyme by an interferon- $beta$ enhanceosome in vitro. Proc. Natl. Acad. Sci. USA 95:12191-12196[Abstract/Free Full Text].

24. Kim, T. K., and T. Maniatis. 1997. The mechanism of transcriptional synergy of an in vitro assembled interferon- $beta$ enhanceosome. Mol. Cell 1:119-129[CrossRef][Medline].

25. Koipally, J., A. Renold, J. Kim, and K. Georgopoulos. 1999. Repression by Ikaros and Aiolos is mediated through histone deacetylase complexes. EMBO J. 18:3090-3100[CrossRef][Medline].

26. Kraulis, P. J. 1991. MOLSCRIPT: a program to produce both detailed and schematic plots of protein structures. J. Appl. Crystallogr. 24:946-950[CrossRef].

27. Lagrange, T., T.-K. Kim, G. Orphanides, Y. W. Ebright, R. H. Ebright, and D. Reinberg. 1996. High-resolution mapping of nucleoprotein complexes by site-specific protein-DNA photocrosslinking: organization of the human TBP-TFIIA-TFIIB-DNA quaternary complex. Proc. Natl. Acad. Sci. USA 93:10620-10625[Abstract/Free Full Text].

28. Leonard, D. A., and T. K. Kerppola. 1998. DNA bending determines Fos-Jun heterodimer orientation. Nat. Struct. Biol. 5:877-881

1.	Benezra, R., R. L. Davis, A. Lassar, S. Tapscott, M. Thayer, D. Lockshon, and H. Weintraub. 1990. Id: a negative regulator of helix-loop-helix DNA binding proteins. Control of terminal myogenic differentiation. Ann. N. Y. Acad. Sci. 599:1-11.
2.	Blackwood, E. M., and R. N. Eisenman. 1991. Max: a helix-loop-helix zipper protein that forms a sequence-specific DNA-binding complex with Myc. Science 251:1211-1217[Abstract/Free Full Text].
3.	Brass, A. L., A. Q. Zhu, and H. Singh. 1999. Assembly requirements of PU.1-Pip (IRF-4) activator complexes: inhibiting function in vivo using fused dimers. EMBO J. 18:977-991[CrossRef][Medline].
4.	Carey, M. 1998. The enhanceosome and transcriptional synergy. Cell 92:5-8[CrossRef][Medline].
5.	Chen, F. E., D.-B. Huang, Y.-Q. Chen, and G. Ghosh. 1998. Crystal structure of p50/p65 heterodimer of transcription factor NF- $kappa$ B bound to DNA. Nature 391:410-413[CrossRef][Medline].
6.	Chen, L., J. N. M. Glover, P. G. Hogan, A. Rao, and S. C. Harrison. 1998. Structure of the DNA-binding domains from NFAT, Fos and Jun bound specifically to DNA. Nature 392:42-48[CrossRef][Medline].
7.	Chen, L., M. G. Oakley, J. N. M. Glover, J. Jain, P. B. Dervan, P. G. Hogan, A. Rao, and G. L. Verdine. 1995. Only one of the two DNA-bound orientations of AP-1 found in solution cooperates with NFATp. Curr. Biol. 5:882-889[CrossRef][Medline].
8.	Chytil, M., B. R. Peterson, D. A. Erlanson, and G. L. Verdine. 1998. The orientation of the AP-1 heterodimer on DNA strongly affects transcriptional potency. Proc. Natl. Acad. Sci. USA 95:14076-14081[Abstract/Free Full Text].
9.	Cullen, B. R., and M. H. Malim. 1992. Secreted placental alkaline phosphatase as a eukaryotic reporter gene. Methods Enzymol. 216:362-368[Medline].
10.	De Cesare, D., D. Vallone, A. Caracciolo, P. Sassone-Corsi, C. Nerlov, and P. Verde. 1995. Heterodimerization of c-Jun with ATF-2 and c-Fos is required for positive and negative regulation of the human urokinase enhancer. Oncogene 11:365-376[Medline].
11.	Diamond, M. I., J. N. Miner, S. K. Yoshinaga, and K. R. Yamamoto. 1990. Transcription factor interactions: selectors of positive or negative regulation from a single DNA element. Science 249:1266-1272[Abstract/Free Full Text].
12.	Diebold, R. J., N. Rajaram, D. A. Leonard, and T. K. Kerppola. 1998. Molecular basis of cooperative DNA bending and oriented heterodimer binding in the NFAT1-Fos-Jun-ARRE2 complex. Proc. Natl. Acad. Sci. USA 95:7915-7920[Abstract/Free Full Text].
13.	Du, W. 1993. Synergistic activation of the human interferon- $beta$ gene promoter. Ph.D. dissertation. Harvard University, Cambridge, Mass.
14.	Du, W., and T. Maniatis. 1992. An ATF/CREB binding site is required for virus induction of the human interferon $beta$ gene. Proc. Natl. Acad. Sci. USA 89:2150-2154[Abstract/Free Full Text].
15.	Du, W., D. Thanos, and T. Maniatis. 1993. Mechanisms of transcriptional synergism between distinct virus-inducible enhancer elements. Cell 74:887-898[CrossRef][Medline].
16.	Escalante, C. R., J. Yie, D. Thanos, and A. K. Aggarwal. 1998. Structure of IRF-1 with bound DNA reveals determinants of interferon regulation. Nature 391:103-106[CrossRef][Medline].
17.	Falvo, J. V., D. Thanos, and T. Maniatis. 1995. Reversal of intrinsic DNA bends in the IFN $beta$ gene enhancer by transcription factors and the architectural protein HMG I(Y). Cell 83:1101-1111[CrossRef][Medline].
18.	Fujii, Y., T. Shimizu, M. Kusumoto, Y. Kyogoku, T. Taniguchi, and T. Hakoshima. 1999. Crystal structure of an IRF-DNA complex reveals novel DNA recognition and cooperative binding to a tandem repeat of core sequences. EMBO J. 18:5028-5041[CrossRef][Medline].
19.	Hai, T., and T. Curran. 1991. Cross-family dimerization of transcription factors Fos/Jun and ATF/CREB alters DNA binding specificity. Proc. Natl. Acad. Sci. USA 88:3720-3724[Abstract/Free Full Text].
20.	Harada, H., K. Willison, J. Sakakibara, M. Miyamoto, T. Fujita, and T. Taniguchi. 1990. Absence of the type I IFN system in EC cells: transcriptional activator (IRF-1) and repressor (IRF-2) genes are developmentally regulated. Cell 63:303-312[CrossRef][Medline].
21.	Karin, M., Z.-G. Liu, and E. Zandi. 1997. AP-1 function and regulation. Curr. Opin. Cell Biol. 9:240-246[CrossRef][Medline].
22.	Keller, W., P. König, and T. J. Richmond. 1995. Crystal structure of a bZIP/DNA complex at 2.2 Å: determinants of DNA specific recognition. J. Mol. Biol. 254:657-667[CrossRef][Medline].
23.	Kim, T. K., T. H. Kim, and T. Maniatis. 1998. Efficient recruitment of TFIIB and CBP-RNA polymerase II holoenzyme by an interferon- $beta$ enhanceosome in vitro. Proc. Natl. Acad. Sci. USA 95:12191-12196[Abstract/Free Full Text].
24.	Kim, T. K., and T. Maniatis. 1997. The mechanism of transcriptional synergy of an in vitro assembled interferon- $beta$ enhanceosome. Mol. Cell 1:119-129[CrossRef][Medline].
25.	Koipally, J., A. Renold, J. Kim, and K. Georgopoulos. 1999. Repression by Ikaros and Aiolos is mediated through histone deacetylase complexes. EMBO J. 18:3090-3100[CrossRef][Medline].
26.	Kraulis, P. J. 1991. MOLSCRIPT: a program to produce both detailed and schematic plots of protein structures. J. Appl. Crystallogr. 24:946-950[CrossRef].
27.	Lagrange, T., T.-K. Kim, G. Orphanides, Y. W. Ebright, R. H. Ebright, and D. Reinberg. 1996. High-resolution mapping of nucleoprotein complexes by site-specific protein-DNA photocrosslinking: organization of the human TBP-TFIIA-TFIIB-DNA quaternary complex. Proc. Natl. Acad. Sci. USA 93:10620-10625[Abstract/Free Full Text].
28.	Leonard, D. A., and T. K. Kerppola. 1998. DNA bending determines Fos-Jun heterodimer orientation. Nat. Struct. Biol. 5:877-881