Oligomerization Mediated by a Helix-Loop-Helix-Like Domain of Baculovirus IE1 Is Required for Early Promoter Transactivation

doi:10.1128/JVI.75.13.6042-6051.2001

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Journal of Virology, July 2001, p. 6042-6051, Vol. 75, No. 13
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.13.6042-6051.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Oligomerization Mediated by a Helix-Loop-Helix-Like Domain of Baculovirus IE1 Is Required for Early Promoter Transactivation

Victoria A. Olson, Justin A. Wetter, and Paul D. Friesen^*

Institute for Molecular Virology and Department of Biochemistry, Graduate School and College of Agricultural and Life Sciences, University of Wisconsin $---$ Madison, Madison, Wisconsin 53706

Received 17 January 2001/Accepted 9 April 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

IE1 is a principal transcriptional regulator of Autographa californica multicapsid nucleopolyhedrovirus (AcMNPV). Transactivationby IE1 is stimulated when early viral promoters are cis linkedto homologous-region (hr) enhancer sequences of AcMNPV. This transcriptionalenhancement is correlated with the binding of IE1 as a dimer tothe 28-bp palindromic repeats comprising the hr enhancer. To definethe role of homophilic interactions in IE1 transactivation, wehave mapped the IE1 domains required for oligomerization. We reporthere that IE1 oligomerizes by a mechanism independent of enhancerbinding, as demonstrated by in vitro pull-down assays using fusionsof IE1 (582 residues) to the C terminus of glutathione S-transferase.In vivo oligomerization of IE1 was verified by immunoprecipitationof IE1 complexes from extracts of plasmid-transfected SF21 cells.Analyses of a series of site-directed IE1 insertion mutationsindicated that a helix-loop-helix (HLH)-like domain extendingfrom residue 543 to residue 568 is the primary determinant ofoligomerization. Replacement of residues within the hydrophobicface of the putative dimerization domain disrupted IE1 homophilicinteractions and caused loss of IE1 transactivation of hr-dependentpromoters in plasmid transfection assays. Thus, oligomerizationis required for IE1 transcriptional stimulation. HLH mutationsalso reduced IE1 stability and abrogated transactivation of non-hr-dependentpromoters. These data support a model wherein IE1 oligomerizesprior to DNA binding to facilitate proper interaction with thesymmetrical recognition sites within the hr enhancer and therebypromote the transcription of early viralgenes.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The principal transcriptional regulator of Autographa californica multicapsid nucleopolyhedrovirus (AcMNPV) is the immediate-earlyprotein IE1. Highly conserved among members of the family Baculoviridae,IE1 regulates baculovirus early gene expression, as first demonstratedby plasmid transfection assays (2, 13, 15, 18-20, 22,25, 28, 33, 36). In similar assays, IE1 was also requiredfor late gene expression and is one of six viral factors requiredfor plasmid DNA replication (17, 26, 30). Consistent witha role in viral transcription and DNA replication, IE1 is detectedthroughout infection and localizes to the nucleus, where it associateswith viral DNA replication factories (5, 7, 29). A temperature-sensitivemutation has implicated IE1 in the proper timing of the AcMNPVlife cycle (8, 34). Thus, the participation of IE1 in multipleviral processes suggests that it is essential for the achievementof productiveinfection.

IE1 is a 582-residue (67-kDa) phosphoprotein with separable domains contributing to promoter transactivation and DNA binding(Fig. 1A). The N terminus of IE1 contains transcription-stimulatorydomains (residues 8 to 118 and 168 to 222) that are dispensablefor DNA binding (18, 38, 39). The C-terminal half of IE1participates in DNA binding (18, 38), but the residues involvedin binding site recognition are unknown. IE1 transactivation ofviral early promoters is enhanced when the promoter is cis linkedto AcMNPV homologous-region (hr) sequences, which function astranscription enhancers and possible origins of DNA replication(12, 14, 20, 22, 28, 32, 33, 36). The hr enhancercontains multiple copies of a 28- to 30-bp imperfect palindrome(28-mer) which is the minimal motif required for enhancer activityand plasmid DNA replication (11, 14, 22, 36, 37). Currentevidence indicates that IE1 interacts specifically with the 28-meras a dimer and must bind to both palindromic half sites for stimulationof hr enhancer activity (11, 20, 23, 37, 38).

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FIG. 1. Structure of IE1 and GST-IE1 fusions. (A) Functional domains. The 582-residue IE1 protein possesses transcriptional transactivation domains (residues 8 to 118 and 168 to 222) within its N-terminal half and unmapped DNA-binding and oligomerization domains within its C-terminal half. (B) GST-IE1. Residues 1 to 233 of GST (crosshatched) were fused to the N terminus of full-length IE1 (residues 1 to 582). (C) Genetic organization of ie-1^HA expression plasmids. Sequences encoding the HA epitope were inserted into the ie-1 open reading frame after residue 579. The resulting ie-1^HA gene or mutations thereof were placed under control of the full-length ie-1 promoter (prm; nucleotides $-$ 546 to +51) for transient-expression assays. Transcription initiates (arrow) from the CAGT (+1) initiator motif.

The binding of oligomeric IE1 to a symmetrical recognition sequence suggests that oligomerization contributes to IE1 functions.Indeed, the activity of transcriptional activators is often regulatedby homophilic interactions (reviewed in references 27 and 31).Site-specific IE1 mutations that eliminate DNA binding have beencharacterized (18, 38). A subset of these mutated forms ofIE1 fail to bind the palindromic 28-mer as a homodimer but retainthe capacity to bind as a heterodimer with wild-type IE1 (38).In contrast, IE1 containing mutations in a C-terminal helix-loop-helix(HLH)-like domain fail to bind DNA as either a homodimer or aheterodimer (38). These findings suggested that oligomerizationmediated by C-terminal IE1 residues is required for DNA bindingand is therefore critical to IE1function.

To investigate the role of oligomerization and define the molecular mechanism of IE1 transactivation, we used a combinationof in vitro and in vivo assays that tested IE1 homophilic interactions.As determined by in vitro pull-down assays using glutathione S-transferasefused to the N terminus of IE1 (GST-IE1), we report here thatIE1 oligomerizes in the absence of viral DNA and other cellularfactors. Immunoprecipitations of differentially tagged IE1 synthesizedin cultured cells confirmed that IE1 forms oligomeric complexesin vivo. By using a panel of site-specific IE1 mutations, we mappedthe residues required for oligomerization to the HLH-like domainat the IE1 C terminus. Mutations that altered hydrophobic residuesof the predicted helices eliminated oligomerization, both in vitroand in vivo. Furthermore, loss of IE1 oligomerization was concomitantwith loss of positive activation of hr-dependent and non-hr-dependentpromoters in plasmid transfection assays. Collectively, thesefindings indicated that IE1 homophilic interactions are requiredfor promoter transactivation and support IE1's role as a sequence-specific,HLH-containing transregulator of early virustranscription.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmids. (i) IE1 insertions and substitutions. IE1 insertion mutations were generated in pSP64/IE1 by using BglII linkers which inserted three to eight amino acids intothe ie-1 open reading frame (38). IE1 amino acid substitutionswere generated by site-directed mutagenesis of pIE1_BS (33) andsubsequently cloned into pSP64/IE1 for in vitro transcriptionand translation reactions (38). pIE1 encodes the wild-type ie-1gene under the control of its own full-length promoter (28).

(ii) IE1^HA and IE1^FLAG expression plasmids. pSP64/IE1 was digested with BstBI, end repaired with Klenow fragment, and ligated to an SpeI linker (5'-GG ACT AGT CC-3')to form pSP64/IE1^SpeI. After digestion with SpeI, the complementary oligonucleotides5'-CT AGC ATG TAC CCA TAC GAC GTC CCA GAC TAC GCT G-3' and 5'-CTAGC AGC GTA GTC TGG GAC GTC GTA TGG GTA CAT G-3' were added byintramolecular ligation to give pSP64/IE1^HA, in which 16 amino acid residues (GTSMYPYDVPDYAASP), includingthe hemagglutinin (HA) epitope (underlined), were inserted afterIE1 residue 579. Similarly, complementary oligonucleotides 5'-CTAGC GAC TAC AAA GAC GAT GAC GAT AAG CTT G-3' and 5'-CT AGC AAGCTT ATC GTC ATC GTC TTT GTA GTC G-3' were used to give pSP64/IE1^FLAG, in which 15 amino acid residues (GTSDYKDDDDKLASP), includingthe FLAG (Eastman Kodak) epitope (underlined), were inserted afterIE1 residue 579. Proper insertion of the epitope tags was verifiedby nucleotide sequencing. The NdeI-SstI fragment of pSP64/IE1^HA was inserted into the corresponding sites of pIE1_BS to generatepIE1^HA/BS (Fig. 1C). pIE1^HA insertion and substitution mutations were generated by insertingthe appropriate restriction fragment from mutated pSP64/IE1 intothe corresponding sites of pIE1^HA/BS, including the Eco47III-NdeI fragment to give pIE1^I70HA/BS, pIE1^I118HA/BS, and pIE1^I156HA/BS; the HpaI fragment to give pIE1^I143HA/BS; the NdeI-AlwNI fragment to give pIE1^I311HA/BS, pIE1^I418HA/BS, pIE1^I425HA/BS, and pIE1^I553HA/BS; the NdeI-BstBI fragment to give pIE1^I243HA/BS, pIE1^I391HA/BS, and pIE1^I462HA/BS; and the StuI-BstBI fragment to give pIE1^{(524/526)HA/BS}, pIE1^{(537/538)HA/BS}, pIE1^{(543/547)HA/BS}, pIE1^{(550/554)HA/BS}, pIE1^{(561/564)HA/BS}, and pIE1^{(565/568)HA/BS}. For the latter nine plasmids, the BstBI site at residue 579within pIE1^HA/BS was reinstated (GGG [Gly] $right-arrow$ GAA [Glu]) by PCRmutagenesis.

(iii) GST-IE1 plasmids. Sequences encoding GST residues 1 to 233 were fused to those encoding full-length IE1 (residues 1 to 582) (Fig. 1B). For expressionin Escherichia coli, an ie-1-containing Sau3AI fragment from pIE1_BSwas inserted into the BamHI site of pGEX-3X (Pharmacia) to givepGEX/IE1 encoding GST-IE1. To generate pGEX/IE1 mutations, theappropriate restriction fragment was replaced with those of mutatedpSP64/IE1 plasmids, including the NdeI-SphI fragment to give pGEX/IE1^I243, pGEX/IE1^I391, and pGEX/IE1^I425 and the StuI-XbaI fragment to give pGEX/IE1^(524/526), pGEX/IE1^(550/554), pGEX/IE1^(561/564), and pGEX/IE1^(565/568).

(iv) Luciferase reporters. The HindIII-NdeI fragment of pGEM-luc (Promega) encoding luciferase was inserted into the corresponding sites of p35 promoter-containingplasmids pBAS35K-CAT/28mer-up⁺ (36) and p( $Delta$ 3'-162/ $Delta$ 5'-154)35K-CAT (9) to give pBAS35K-Luc/28mer-up⁺ and pFL35K-Luc, respectively. Through multiple steps, the polyadenylationsignal from pIE1^hr/PA (4) was subsequently inserted into each plasmid to givepBAS35K-Luc/28mer-up⁺/PA and pFL35K-Luc/PA, representing hr-dependent and UAR-dependentreporter plasmids,respectively.

(v) IE1 antigen expression plasmid. After digestion with SpeI, pSP64/IE1^SpeI was intramolecularly ligated to complementary oligonucleotides 5'-CT AGC CAC CAT CACCAT CAC CAT TAA AGA TCT G-3' and 5'-CT AGC AGA TCT TTA ATG GTGATG GTG ATG GTG G-3'. The resulting plasmid, pSP64/IE1^His, encodes IE1 with a His₆ tag (GTSHHHHHH) and a stop codon insertedafter residue 579. IE1^His sequences were inserted into vector pET11b (Novagen) to givepET-IE1^His. Sequences encoding IE1 residues 157 to 556 were subsequentlyremoved by digestion with StuI and AlwNI, and the vector was endrepaired with Klenow fragment and intramolecularly ligated togive pET-IE1^His157-556.

In vitro protein synthesis. Coupled in vitro transcription-translation reactions were conducted in accordance with the manufacturer's protocol (TNT system;Promega). Circular plasmid DNA (0.6 µg) was added to mixtures(30 µl) containing rabbit reticulocyte lysate, amino acids, Tran³⁵S-labeled methionine and cysteine (NEN), SP6 polymerase, and RNasin(Promega). After a 2-h incubation at 30°C, samples (3 µl) of thereaction mixture were subjected to denaturing sodium dodecyl sulfate(SDS)-10% polyacrylamide gel electrophoresis (PAGE). Protein productionwas quantified by using a Molecular Dynamics PhosphorImager (model450).

GST-IE1 binding assay. E. coli strain JM83 harboring plasmids pGEX-3X or pGEX/IE1 was grown in Luria-Bertani broth with ampicillin. Cells were collected,suspended in NETN buffer (20 mM Tris [pH 8], 100 mM NaCl, 1 mMEDTA, 0.5% NP-40, protease inhibitors [Boehringer Mannheim]),and lysed by sonication. After clarification, glutathione-agarosebeads (Pierce) were added and the combination was mixed for 30min at 4°C. The beads were washed five times and suspended inNETN buffer to give a 50% (vol/vol) slurry. Protein was elutedfrom a sample of beads by boiling, and the yield was determinedby SDS-PAGE and staining with colloidal Coomassie G-250 (Zaxis).To compare levels of in vitro IE1 protein bound as a measure ofIE1 oligomerization, GST and GST-IE1 protein levels were normalizedby diluting beads in NETN-0.5% dry milk. After washing with NETN-0.5%dry milk, a slurry of protein-bound beads (20 µl) was mixed within vitro-synthesized, ³⁵S-labeled IE1 (10 µl) in 500 µl of NETN-0.5% dry milk. After a2-h incubation at 4°C, the beads were washed three times withNETN and bound protein was eluted by boiling. Proteins were quantifiedby SDS-PAGE and phosphorimaging (MolecularDynamics).

Electrophoretic mobility shift assays (EMSAs). An $alpha$ -³²P-end-labeled DNA probe containing the 28-mer of hr5 was prepared and mixed with in vitro-synthesized IE1 as describedpreviously (38). Protein-DNA complexes were subjected to nondenaturing5% polyacrylamide-Tris-glycine gel electrophoresis also as previouslydescribed (37). For antibody supershifts, IE1^HA- and IE1^FLAG-bound DNA complexes were incubated with 12CA5 anti-HA (BAbCO)or M2 anti-FLAG (Eastman Kodak) monoclonal antibodies, respectively,prior toelectrophoresis.

Cells and plasmid transfections. Spodoptera frugiperda IPLB-SF21 (40) cells were propagated in TC100 growth medium (GIBCO Laboratories) supplemented with2.6 mg of tryptose broth per ml and 10% heat-inactivated fetalbovine serum. For transfections, SF21 cell monolayers were washedwith TC100 and overlaid with a transfection mixture containingN-[1-(2,3-dioleoyloxy)propyl]-N,N,N-trimethylammonium methyl sulfate-L- $alpha$ -phosphatidylethanolamine,dioleoyl (C_18:1, [cis]-9) (DOTAP-DOPE) and plasmid DNA in TC100.After 4 h at room temperature, the mixture was replaced with supplementedTC100.

Reporter transfection assays. SF21 cells (2 × 10⁶/60-mm-diameter plate) were transfected with luciferase reporter plasmid DNA (2 µg), either alone or withthe indicated IE1^HA-encoding plasmids (0.5 µg). Cells were collected 48 h later,washed with phosphate-buffered saline (21), and lysed by suspensionin 250 µl of 1× cell culture lysis reagent (Promega). After clarification,the level of luciferase activity in the cell lysate (20 µl) wasdetermined by using a luminometer (Monolight 3010) in accordancewith the manufacturer's (Promega) instructions. When purifiedluciferase (Promega) was used, the assay was linear from 10⁴ to 10⁸ relative lightunits.

Immunoprecipitations. SF21 cells (7 × 10⁶/100-mm-diameter plate) were transfected with plasmid DNA (11 µg) encoding untagged, wild-type IE1 and IE1^HA. Cells were collected 24 h later, washed with phosphate-bufferedsaline (21), and lysed by suspension in 900 µl of E1A buffer(250 mM NaCl, 0.1% NP-40, 50 mM HEPES [pH 7], protease inhibitors)for 45 min on ice. After clarification by centrifugation (16,000× g) for 10 min at 4°C, lysate (300 µl) was mixed with 918 µlof WCE buffer (10 mM HEPES [pH 7], 400 mM NaCl, 0.10 mM EGTA,protease inhibitors) containing $approx$ 10 µg (2 µl) of HA.11 monoclonalantibody ( $alpha$ -HA; BAbCO). After 4 h on ice, a 50% slurry of proteinG-Sepharose beads (Sigma) in WCE buffer was added and mixed for6 h at 4°C. Immune complexes were washed six times with WCE buffer-0.1%SDS and eluted by boiling in 1% SDS-2.5% $beta$ -mercaptoethanol.

$alpha$ -IE1 polyclonal serum. Protein production was induced in E. coli strain BL21(DE3) (Novagen) harboring pET-IE1^His157-556 by addition of 1 mM IPTG (isopropyl- $beta$ -D-thiogalactopyranoside).After cell lysis, inclusion bodies were collected and solubilizedin binding buffer (20 mM Tris-HCl, 500 mM NaCl, 5 mM imidazole)containing 6 M urea. His-tagged protein was purified by Ni²⁺ affinity chromatography (1), dialyzed against phosphate-bufferedsaline, and concentrated. Protein purity was >95%, as judged bySDS-PAGE. New Zealand White rabbits were immunized, and antiserawere prepared by the University of Wisconsin Medical School PolyclonalAntibody Service using standardprocedures.

Immunoblot analysis. Protein samples in SDS and $beta$ -mercaptoethanol were electrophoresed on SDS-7.5% polyacrylamide gels. After protein transfer,nitrocellulose membranes were incubated with a 1:20,000 dilutionof $alpha$ -IE1, followed by alkaline phosphatase-conjugated goat anti-rabbitimmunoglobulin G (Jackson ImmunoResearch Laboratories) or a 1:1,000dilution of $alpha$ -HA (HA.11), followed by alkaline phosphatase-conjugatedgoat anti-mouse immunoglobulin G (Jackson ImmunoResearch Laboratories).Signal development was performed by using nitroblue tetrazoliumchloride-BCIP (5-bromo-4-chloro-3'-indolylphosphate p-toluidinesalt) colorimetric detection as described previously (16) orthe Western-Star Chemiluminescent Detection System(Tropix).

Image processing. Immunoblots were scanned at a resolution of 300 dots/in. by using a UMAX PowerLook III. The files were printed from AdobePhotoshop by using a Tektronics Phaser 450 dye sublimationprinter.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

In vitro oligomerization of IE1 in the absence of viral DNA. In enhancer-dependent transactivation by IE1, the 28-mer palindromic repeats comprising the hr enhancer elements interactwith dimeric IE1 (11, 18, 20, 22, 37, 38). Thus, IE1oligomerization has been implicated as a required step in DNA-dependenttransactivation (6, 37, 38). To investigate the role ofIE1 oligomerization and to determine whether homophilic associationis DNA dependent, we tested IE1 interactions by first using apull-down assay involving GST fusionproteins.

GST-IE1, which consists of full-length IE1 (residues 1 to 582) fused to the C terminus of GST (Fig. 1B), was overproducedin E. coli and loaded onto glutathione-Sepharose beads. Afterincubation with in vitro-synthesized, [³⁵S]methionine-labeled IE1, the GST-IE1 beads were washed extensivelyand protein was eluted. Significant binding of wild-type IE1 toGST-IE1 was detected (Fig. 2A, lane 3). In contrast, little, ifany, binding of IE1 to GST alone occurred (Fig. 2A, lane 2). Thespecificity of IE1 binding to GST-IE1 was confirmed by testingfor interaction with unrelated AcMNPV protein P35 (1, 10).In vitro-synthesized P35 failed to interact with GST or GST-IE1(data not shown). We concluded that independently synthesizedIE1 molecules have the capacity to oligomerize in the absenceof hr enhancer DNA.

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FIG. 2. In vitro association of GST-IE1 with IE1. (A) GST-IE1 binding assay. In vitro-synthesized, ³⁵S-labeled IE1 was mixed with glutathione-beads containing GST alone (lane 2) or GST-IE1 (lane 3). After washing, bound protein was eluted, subjected to SDS-PAGE, and imaged. (B) GST-IE1 association with IE1 insertions. ³⁵S-labeled IE1 insertions were assayed for binding to GST alone and GST-IE1 as described for panel A. Mutated IE1s are designated by the amino acid residue preceding the insertion (38). (C) Wild-type (wt) IE1 association with GST-IE1 insertions. ³⁵S-labeled IE1 was assayed for binding to GST alone (lane 2), GST-IE1 (lane 3), or GST-IE1 insertions (lanes 4 to 6) as described for panel A. For each binding assay (A to C), 1% of the ³⁵S-labeled input protein (Input) was included.

Identification of IE1 domains required for in vitro oligomerization. To map the domains required for IE1 oligomerization, we tested the effects of site-specific mutations on the ability of IE1to interact with GST-IE1. We first screened a panel of 14 IE1mutations containing three- to eight-residue insertions spanningthe full-length protein (38). The mutated IE1s were synthesizedin vitro and tested for oligomerization by using the GST-IE1 pull-downassay. A majority of the IE1 insertion mutations tested, includingIE1^I70, IE1^I118, IE1^I143, IE1^I156, IE1^I243, IE1^I311, IE1^I418, IE1^I513, and IE1^I579, associated with GST-IE1 at levels comparable to that of wild-typeIE1 (Fig. 2B), suggesting that oligomerization was unaffected.In contrast, insertions IE1^I391, IE1^I414, IE1^I425, IE1^I462, and IE1^I553 exhibited reduced levels of interaction, as judged by subtractingthe level of ³⁵S-labeled IE1 bound nonspecifically to GST alone from that boundspecifically to GST-IE1. Of these insertions, IE1^I425 and IE1^I553 were the most impaired for GST-IE1 binding (Fig. 2B), which suggestedthat domains contributing to IE1 oligomerization were compromisedby thesemutations.

To verify these IE1 interactions, we used reciprocal binding assays. GST was fused to selected IE1 insertion mutations andsubsequently tested for association with ³⁵S-labeled wild-type IE1. As expected, GST-IE1^I243 interacted with wild-type IE1 at levels comparable to that ofGST-IE1 (Fig. 2C, lanes 3 and 4). Under these conditions, wild-typeIE1 also interacted with GST-IE1^I391 and GST-IE1^I425 but at reduced levels (Fig. 2C, lanes 5 and 6). Although notanalyzed here, the domain including residue 553 was characterizedfurther by substitution mutagenesis (see below). Collectively,these in vitro data indicated that domains encompassing residues391, 425, and 553 contribute directly or indirectly to IE1 intermolecularinteractions.

Identification of IE1 domains required for in vivo oligomerization. To verify that IE1 oligomerizes within the cell, we investigated IE1 interactions in vivo. To this end, we tagged IE1 at residue579 with the influenza virus HA epitope (IE1^HA) or the FLAG epitope (IE1^FLAG). Transactivation by IE1^HA was indistinguishable from that by wild-type, untagged IE1 (datanot shown). DNA-binding activity was verified by EMSAs. Underthese conditions, both IE1^HA and IE1^FLAG bound a DNA probe containing the 28-mer of the hr5 enhancer withan efficiency comparable to that of untagged IE1 (Fig. 3A, lanes2 and 4, and B, lane 1). The presence of each epitope-tagged proteinin the DNA complex was confirmed by using specific antiserum.HA-specific monoclonal antiserum $alpha$ -HA yielded two supershiftedIE1^HA-containing complexes (Fig. 3A, lane 5). $alpha$ -FLAG antiserum alsodetected two supershifted IE1^FLAG-containing complexes. The proportion of the largest complex increasedwith increasing $alpha$ -FLAG (Fig. 3B, lanes 2 to 4) and thus indicatedthe presence of two IE1^FLAG molecules. These data demonstrated that dimeric IE1 binds tothe single 28-mer, as expected (37, 38).

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FIG. 3. DNA binding by C-terminally epitope-tagged IE1. (A) EMSA using IE1^HA. In vitro-synthesized, untagged IE1 (lanes 2 and 3) and IE1^HA (lanes 4 and 5) were incubated with a ³²P-labeled 28-mer DNA probe in the presence (+) or absence ( $-$ ) of monoclonal antiserum $alpha$ -HA. Complexes were subjected to nondenaturing PAGE and autoradiography. IE1-DNA complexes, alone (IE1) or bound by one (*) or two (**) antibodies, are indicated. In the absence of IE1 (lane 1), no DNA probe was bound. (B) EMSA using IE1^FLAG. In vitro-synthesized IE1^FLAG was incubated with a 28-mer DNA probe in the absence ( $-$ ) (lane 1) or presence of increasing amounts of $alpha$ -FLAG antiserum (lanes 2 to 4) and subjected to EMSA as described for panel A. wt, wild type.

To test for intracellular IE1 oligomerization, we used IE1^HA in $alpha$ -HA immunoprecipitation assays. SF21 cells were transfectedwith plasmids encoding IE1^HA and untagged, wild-type IE1. The ie-1 promoter lacking hr enhancersequences was used to direct ie-1 expression (Fig. 1C). $alpha$ -HA immunoprecipitationof nonionic detergent lysates of transfected cells detected acomplex containing both IE1 proteins, as shown by immunoblot analysisusing $alpha$ -IE1 antiserum (Fig. 4C, lane 3). Although untagged IE1was readily detected in whole-cell lysates (Fig. 4B, lane 1),it was not immunoprecipitated by $alpha$ -HA (Fig. 4C, lane 1). Thus,detection of untagged IE1 in immunoprecipitates was indicativeof its capacity to complex directly or indirectly with IE1^HA.

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FIG. 4. In vivo association of IE1 and IE1^HA insertions. (A) IE1 insertions. The position of each insertion mutation within IE1^HA is depicted. The ability (+) (see below) or inability ( $-$ ) to oligomerize in vitro and in vivo is shown. (B) Intracellular levels of wild-type (wt) IE1 and IE1^HA insertions. SF21 cells were transfected with plasmids encoding wild-type, untagged IE1 and wild-type IE1^HA or the indicated IE1^HA insertions. Plasmid levels were adjusted to provide comparable levels of protein, maintaining a constant plasmid level by supplementation with ie-1 promoter-containing plasmid pIE1-lacZ (3). Nonionic detergent extracts of cells were prepared 24 h after transfection. Samples (10⁵ cell equivalents) representing 10% of that used for immunoprecipitation (see below) were subjected to immunoblot analysis by using IE1-specific ( $alpha$ -IE1) serum. (C) Immunoprecipitations. HA-tagged proteins from transfected-cell extracts (10⁶ cell equivalents) were immunoprecipitated (immuno-ppt) with HA-specific monoclonal antibody $alpha$ -HA and subjected to immunoblot analysis by using $alpha$ -IE1. IE1^HA and wild-type IE1 proteins are indicated.

We therefore used immunoprecipitation assays of IE1 insertion mutations to define the residues required for in vivo IE1 oligomerization.Immunoblot analysis demonstrated that all IE1 insertion mutationswere synthesized in plasmid-transfected cells (Fig. 4B). However,the levels of IE1^I553 were the lowest (Fig. 4B, lane 14), suggesting that its stabilitywas reduced (see below). The IE1 insertion mutations capable ofin vitro oligomerization, IE1^I70, IE1^I118, IE1^I143, IE1^I156, IE1^I243, IE1^I311, IE1^I418, and IE1^I462, complexed with untagged wild-type IE1 (Fig. 4C). IE1^I391 and IE1^I425 also maintained the capacity to oligomerize. Only IE1^I553 failed to interact, despite the presence of excess wild-typeIE1 (Fig. 4C, lane 14). Thus, of the insertion mutations tested,only IE1^I553 was defective for oligomerization, both in vitro and in vivo.These data indicated that the domain encompassing residue 553is a principal determinant of IE1oligomerization.

Requirement of a helix-loop-helix-like domain for IE1 oligomerization in vitro. HLH domains are commonly required for oligomerization of transcription activators and often serve as the protein-protein interface(24, 27, 31, 35). IE1 residue 553 lies within a C-terminalregion (Fig. 5A) predicted to contain two amphipathic $alpha$ -helicespreceded by a cluster of basic residues (18, 38). The highdegree of conservation of this region among baculovirus IE1 proteins(Fig. 5A) is indicative of its relative importance for IE1 function.To define the function of this HLH-like domain, we determinedthe effects of selective amino acid substitutions on IE1 interactionsin vitro. IE1 mutations were synthesized and tested for the capacityto interact by using the GST-IE1 pull-down assay. As shown previously(Fig. 2A), wild-type IE1 bound efficiently to GST-IE1 (data notshown). Replacement of pairs of hydrophobic residues with chargedresidues within the putative HLH (L⁵⁴³D-L⁵⁴⁷E, L⁵⁵⁰D-I⁵⁵⁴E, L⁵⁶¹D-A⁵⁶⁴E, and I⁵⁶⁵D-A⁵⁶⁸E) diminished IE1's interaction with GST-IE1 to levels comparableto that with GST alone (Fig. 5B). Although replacement of adjacentarginines with alanine (R⁵³⁷A-R⁵³⁸A) also eliminated IE1 interaction, replacement of a nearby arginine-lysinepair (R⁵²⁴A-K⁵²⁶A) did not (Fig. 5B). Reciprocal GST-IE1 binding assays confirmedthe binding differences between substitution R⁵²⁴A-K⁵²⁶A and the mutations within the HLH. GST-IE1^R524A-K526A interacted with wild-type IE1 at levels comparable to that ofGST-IE1 (Fig. 5C, lanes 3 and 4). In contrast, only backgroundlevels of wild-type IE1 bound to substituted GST-IE1^L550D-I554E, GST-IE1^L561D-A564E, and GST-IE1^I565D-A568E (Fig. 5C, lanes 5, 6, and 7). On the basis of these in vitrodata, we concluded that hydrophobic residues within the putativehelices contribute to oligomerization. R⁵³⁷ and R⁵³⁸ also contributed to IE1 in vitro interactions, but subsequentstudies indicated that they were less important in vivo (see below).

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FIG. 5. In vitro association of GST-IE1 with HLH substitutions. (A) HLH-like domain of IE1. AcMNPV IE1 residues 521 to 570 were aligned with the corresponding IE1 residues from the indicated baculoviruses. Conserved basic (+) and hydrophobic ( $Psi$ ) residues (shaded) are depicted. Pairwise substitutions (underlined) are designated by position. (B) Binding to GST-IE1. The indicated IE1 mutations were synthesized in vitro with [³⁵S]methionine and assayed for binding to GST alone and GST-IE1 as described in the legend to Fig. 2. (C) Binding to GST-IE1 substitutions. ³⁵S-labeled wild-type (wt) IE1 was tested for binding to GST alone (lane 2), GST-IE1 (lane 3), or the indicated GST-IE1 substitutions (lanes 4 to 7). For each binding assay, 1% of the ³⁵S-labeled input protein (Input) was included.

Requirement of the C-terminal HLH-like domain for IE1 oligomerization in vivo. To verify that the HLH-like domain is required for intracellular IE1 oligomerization, we tested the effects of HLH substitutionson in vivo IE1 interactions as assayed by immunoprecipitationof extracts from plasmid-transfected cells (Fig. 6B). The steadystate levels of all HLH substitution mutations were reduced comparedto that of wild-type IE1, suggesting that defects within the HLH-likedomain reduce IE1 stability. The least stable was IE1^L561D-A564E (Fig. 6B, lane 8). Complexes containing IE1^HA were precipitated with $alpha$ -HA and subjected to immunoblot analysiswith $alpha$ -IE1 (Fig. 6C). Both IE1^R524A-K526A and IE1^R537A-R538A interacted with wild-type IE1 (Fig. 6C, lanes 4 and 5). Thus,replacement of R⁵³⁷ and R⁵³⁸ had less of an effect on IE1 oligomerization in vivo than invitro. Despite the presence of excess wild-type IE1, mutationsIE1^L543D-L547E, IE1^L550D-I554E, IE1^L561D-A564E, and IE1^I565D-A568E failed to complex with IE1 (Fig. 6C, lanes 6 to 9). Thus, allsubstitution mutations within the HLH-like domain abrogated invivo IE1 oligomerization. Collectively, the in vivo and in vitroassays indicated that the hydrophobic residues within the HLHare required for IE1 oligomerization and contribute to IE1 stability.

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FIG. 6. In vivo association of IE1 and HLH substitutions. (A) IE1 substitution mutations. Pairs of residue substitutions designated by their positions are indicated below IE1 residues 521 to 570. The ability (+) or inability ( $-$ ) of each IE1^HA mutation to oligomerize in vitro and in vivo is shown. (B) Intracellular levels of wild-type (wt) IE1 and IE1^HA mutations. SF21 cell extracts were prepared 24 h after transfection with plasmids encoding untagged wild-type IE1 and wild-type IE1^HA or the indicated IE1^HA substitutions as described in the legend to Fig. 4. Samples (10⁵ cell equivalents) representing 10% of the amount used for immunoprecipitation (see below) were subjected to immunoblot analysis by using $alpha$ -IE1. (C) Immunoprecipitations. HA-tagged proteins from cell extracts (10⁶ cell equivalents) were immunoprecipitated (immuno-ppt) with $alpha$ -HA and subjected to immunoblot analysis by using $alpha$ -IE1. IE1^HA and wild-type IE1 proteins are indicated.

Requirement of oligomerization for transactivation by IE1. IE1 mutations that disrupt binding to hr enhancer elements eliminate hr-dependent transactivation (18, 37). Since oligomerizationshould enhance the stability of the IE1 interaction with the palindromic28-mer response elements within the hr enhancer (38), we predictedthat oligomerization contributes to IE1 transactivation. To testthis hypothesis, we compared the capacity of IE1 oligomerization-defectivemutations to transactivate an hr-dependent promoter. To this end,we constructed a reporter plasmid (Fig. 7A) encoding the luciferasegene under control of the basal promoter of the AcMNPV p35 gene,which was linked to an upstream palindromic 28-mer of the hr5enhancer. The minimal p35 basal promoter contains a TATA elementand early RNA start site (+1) but lacks its viral upstream activatingregion (UAR) (9, 33, 36, 38). cis linkage of a single28-mer in either orientation yields 40-fold stimulation of thep35 basal promoter by IE1 (37).

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FIG. 7. Transactivation by IE1^HA mutations. (A) Luciferase reporters. For hr-dependent transcription, the luciferase gene under the control of the p35 basal promoter (prm; TATA element and RNA start site, +1) was linked to a single copy of the palindromic 28-mer from hr5, which is sufficient for enhancer activity. For UAR-dependent transcription, the luciferase gene was placed under the control of the full-length p35 promoter with UAR sequences $-$ 110 to $-$ 30 upstream from the TATA element. (B) IE1^HA insertions. SF21 cells (2 × 10⁶/plate) were transfected with reporter plasmid DNA (2 µg) alone or with reporter plasmid DNA and plasmid DNA (0.5 µg) encoding the indicated IE1^HA. Cell lysates were prepared 48 h later and assayed for luciferase. The values for hr-dependent (solid bar) and UAR-dependent (striped bar) transactivation are averages ± standard deviations of triplicate transfections and are reported as relative light units (RLU). IE1^HA levels were determined by immunoblot analysis of total cell lysates (2.4 × 10⁵ cell equivalents) using $alpha$ -HA. (C) IE1^HA substitutions. Plasmid transfection assays were conducted by using hr-dependent (solid bar) and UAR-dependent (striped bar) reporters and the indicated IE1^HA substitutions as described for panel B. IE1^HA levels were also determined as described for panel B. wt, wild type.

Levels of transactivation by IE1^HA mutations were determined by plasmid transfection assays. IE1^HA synthesis in transfected cells was confirmed by immunoblot analysisof whole-cell lysates (Fig. 7B and C). Several mutated IE1s wereproduced at lower levels, including oligomerization-defectiveIE1^I553, IE1^L543D-L547E, IE1^L550D-I554E, IE1^L561D-A564E, and IE1^I565D-A568E. Transactivation of the hr-dependent reporter by oligomerization-competentinsertion mutations IE1^I70, IE1^I118, and IE1^I143 was greater than or equal to that of wild-type IE1^HA (Fig. 7B, solid bar). Oligomerization-competent IE1^I156 and IE1^I418 showed reduced transactivation, whereas oligomerization-competentIE1^I243, IE1^I391, IE1^I425, and IE1^I462 were transactivation defective (Fig. 7B, solid bar). Likewise,oligomerization-defective IE1^I553 failed to transactivate. Of the oligomerization-competent substitutionmutations, IE1^R524A-K526A exhibited 40% of wild-type transactivation but IE1^R537A-R538A was inactive (Fig. 7C, solid bar). Oligomerization-defectiveHLH mutations IE1^L543D-L547E, IE1^L550D-I554E, IE1^L561D-A564E, and IE1^I565D-A568E failed to transactivate (Fig. 7C, solidbar).

To determine whether the observed instability of oligomerization-defective IE1 was solely responsible for the loss of function,we tested for transactivation by IE1 mutations in dose-dependenttransfection assays by using the hr-dependent luciferase reporter(Fig. 8A, inset). As expected, increased levels of plasmid DNAencoding wild-type IE1^HA yielded a proportional increase in reporter activation (Fig.8A) and IE1^HA synthesis (Fig. 8B). With the exception of IE1^L561D-A564E, all oligomerization-defective mutations, including IE1^I553, IE1^L543D-L547E, IE1^L550D-I554E, and IE1^I565D-A568E, were produced at levels greater than the lowest level of wild-typeIE1 (Fig. 8B). Despite increased intracellular levels, none ofthese IE1 mutations transactivated the hr-dependent reporter (Fig.8A). Thus, although loss of oligomerization reduced IE1 levels,this instability was not exclusively responsible for loss of IE1function. We concluded that IE1 oligomerization is required forhr enhancer-dependent transactivation.

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FIG. 8. Dose response of transactivation by oligomerization-defective IE1^HA. (A) hr-dependent luciferase reporter activity. SF21 cells (2 × 10⁶/plate) were transfected with 2 µg of the hr-dependent reporter plasmid (inset) and increasing amounts (micrograms) of the indicated IE1^HA plasmids. A constant level of plasmid DNA was maintained by supplementation with ie-1 promoter (prm)-containing plasmid pIE1-lacZ (3). Luciferase reporter activity was determined 48 h after transfection as described in the legend to Fig. 7. (B) Immunoblots. IE1^HA levels were determined by immunoblot analysis of total cell lysates (2 × 10⁵ cell equivalents) by using $alpha$ -HA. (C) UAR-dependent luciferase reporter activity. SF21 cells (2 × 10⁶/plate) were transfected with 2 µg of the UAR-dependent reporter plasmid (inset) and increasing amounts (micrograms) of the indicated IE1^HA plasmids and then assayed for luciferase activity as described for panel A. wt, wild type.

IE1 oligomerization is required for transactivation of non-hr promoters. Certain AcMNPV early promoters are highly responsive to IE1 transactivation in the absence of cis-linked hr elements (2,13, 18, 19, 25, 28, 33). For example, the AcMNPV p35promoter is stimulated more than 1,000-fold by IE1 (28, 33).There is no evidence that IE1 binds to this promoter or its UAR(37). Thus, to ascertain whether IE1 oligomerization is alsonecessary for non-hr transactivation, we tested IE1 mutationsfor stimulation of the luciferase gene placed under the controlof the full-length p35 promoter (Fig. 7A). Levels of IE1^HA in transfected SF21 cells (not shown) were comparable to thoseobserved in hr-reporter transfections (Fig. 7B andC).

The UAR-dependent p35 promoter was transactivated by oligomerization-competent IE1^I70 and IE1^I118 at or above the level of transactivation by wild-type IE1^HA. Mutated IE1^I143, IE1^I156, and IE1^I418 transactivated at levels that were >40% of the wild-type IE1level (Fig. 7B, striped bars). In contrast, oligomerization-competentIE1^I243, IE1^I391, IE1^I425, and IE1^I462 failed to transactivate the UAR-dependent promoter (Fig. 7B,striped bars). Oligomerization-defective IE1^I553 also failed to transactivate. Likewise, oligomerization-defectiveHLH substitutions IE1^L543D-L547E, IE1^L550D-I554E, IE1^L561D-A564E, and IE1^I565D-A568E were transactivation defective (Fig. 7C, striped bars). Of theoligomerization-competent mutations, IE1^R524A-K526A exhibited 50% of wild-type activity but IE1^R537AR538A was inactive (Fig. 7C, stripedbars).

To rule out the possibility that the instability of oligomerization-defective IE1 caused loss of non-hr transactivation, wealso tested the activity of the IE1 mutations in dose-dependenttransfection assays by using the UAR-dependent p35 reporter (Fig.8C, inset). The intracellular levels (not shown) of the oligomerization-defectiveIE1 mutations were indistinguishable from those in the hr-dependentreporter assays (Fig. 8B). All IE1 mutations, excluding IE1^L561DA564E, were produced at levels greater than the lowest level of wild-typeIE1. Despite increased intracellular levels, none of these IE1mutations transactivated the UAR-dependent reporter (Fig. 8C).We concluded that oligomerization is also necessary for non-hrtransactivation by IE1. Thus, proper homophilic interactions byIE1 are necessary for transcriptional stimulation of distinctearlypromoters.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The activity of transcriptional activators is often regulated by homophilic interactions. Many HLH-containing transcriptionalactivators homo-oligomerize through HLH interactions to form anactive dimer capable of binding to palindromic DNA recognitionsites (reviewed in references 24, 27, 31, and 35). Similarly,baculovirus IE1 binds as a dimer to the palindromic 28-mer enhancerelement of the hrs (11, 37). We report here that hr-dependenttransactivation by IE1 requires IE1 homo-oligomerization, whichoccurs in a DNA-independent manner. Our data build a model (Fig.9) in which IE1 dimers assemble upon synthesis and interact directlywith symmetrical recognition sites comprising the 28-mer as aprerequisite to enhancer-dependent transcriptional activation.

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FIG. 9. Role of oligomerization in IE1 transactivation. (A) Summary of IE1 mutations. The capacity of each IE1^HA mutation to oligomerize in vivo (+ or $-$ ) and to transactivate hr-dependent promoters (+ or $-$ ) is shown. ND, not determined. Residues comprising the transactivation and HLH-like domains are indicated (overlined). Residues constituting the DNA-binding domain(s) remain undefined. (B) Model of dimeric IE1 binding to the 28-mer of hr5. The imperfect palindrome of the 28-mer is bisected by an EcoRI site. Each IE1 monomer interacts with a half site (hs) by contacting the top strand of hs^L and the bottom strand of hs^R (striped boxes) (23). The monomers interact across the EcoRI site through their HLH-like domains. IE1 is depicted with separable transactivation (upper orb) and DNA-binding (lower orb) domains.

IE1 oligomerization mediated by an HLH interface. The C terminus of IE1, which contains an HLH-like domain, was previously implicated in IE1 homophilic interactions (18,38). Our mutational analyses described here indicated that multipledomains contribute to the capacity of IE1 to oligomerize in vitro(Fig. 2 and 5). However, only mutations that disrupted the HLH-likedomain (residues 543 to 568) caused loss of oligomerization bothin vitro and in vivo (Fig. 4 and 6). Thus, the HLH motif is theprincipal contributor to IE1 oligomerization. This conclusionis supported by the previous finding that IE1 binding to 28-merDNA as a heterodimer with wild-type IE1 was selectively compromisedby mutations in the HLH domain (38). As predicted from studieson the oligomerization domains of known HLH-containing transcriptionalactivators (24, 27, 31), replacement of the hydrophobicresidues comprising the HLH-like domain of IE1 eliminated oligomerization(Fig. 6). By analogy, it is likely that the hydrophobic face ofthe amphipathic helices participates directly in these homophilicinteractions. Under the conditions we used, IE1-IE1 interactionwas sufficiently strong that oligomerization was readily detectedin the absence of DNA binding, suggesting that IE1 oligomerizationoccurs prior to hr binding. It is unknown whether the HLH-likedomain is sufficient to mediate oligomerization. The finding thatdomains centered at residues 391 and 425 (Fig. 2) also affectedin vitro oligomerization suggests that other regions contributeindirectly to IE1 homophilicinteractions.

Oligomerization-dependent transactivation by IE1. Of 11 IE1 insertion mutations, 5 failed to transactivate an hr-dependent promoter (Fig. 9A). However, all of these mutatedIE1s retained the capacity to homo-oligomerize, with the exceptionof the insertion at residue 553. On the basis that all oligomerization-defectivemutations, including substitutions within the HLH, caused lossof IE1 transactivation (Fig. 9A), we concluded that oligomerizationis required for hr-dependent transactivation. Since transactivationis directly correlated with the capacity of IE1 to bind the palindromic28-mer of the hr element (11, 20, 22, 37), it is likelythat oligomerization contributes directly to DNA binding (seebelow). Consistent with this conclusion, in vitro biochemicalstudies indicated that each of the oligomerization-defective IE1sanalyzed here failed to bind 28-mer DNA (38). Nonetheless, ourstudies indicated that oligomerization-defective IE1 also failedto transactivate IE1-responsive promoters that lack obvious hr-relatedsequences, including the full-length p35 promoter (Fig. 7 and8). Thus, oligomerization also contributes to transactivationfunctions other than DNA binding. Possibilities include oligomerization-dependentconformational changes in IE1 that facilitate interaction withor recruitment of cellular factors contributing to RNA polymeraseII transcription at early promoters. Consistent with oligomerization-inducedconformational changes, oligomerization-defective IE1 exhibitedmarked instability compared to oligomerization-competent IE1,as suggested by the reduced steady-state levels of these IE1 mutations(Fig. 7 and 8). In particular, the substitution mutations withinthe HLH-like domain, which were expected to have minor effectson overall IE1 conformations, exhibited the greatest instability.These findings suggested that oligomerization contributes to properproteinfolding.

Model for DNA binding by IE1: role of oligomerization. Our data reported here, combined with previous studies (20, 23, 37, 38), suggest that IE1 oligomerization orientseach IE1 subunit for proper interaction with the two half sitesof the 28-mer. In this model (Fig. 9B), the preassembled IE1 dimerinteracts across the 28-mer axis of symmetry to make simultaneouscontact with both half sites in order to achieve transcriptionalenhancement. The demonstration here of two supershifted DNA-proteinspecies (Fig. 3) and the detection of discrete heterodimers (37,38) by EMSA verified that the IE1-28-mer complex contains twomolecules of IE1. The requirement for a critical spacing of the28-mer half sites suggests that simultaneous interaction withboth half sites is needed for enhancer activation (37). Bothhalf sites are also required for optimal IE1 interaction in vitro(37). Moreover, since a single half site is sufficient to bindIE1 but insufficient to stimulate transcription, it is likelythat interaction with dual half sites induces an uncharacterizedchange in IE1 or the interacting DNA which promotes enhancer activity.Thus, the binding of preformed IE1 dimers likely facilitates propercontact with the 28-mer halfsites.

DNA binding by IE1. In many basic-HLH domain-containing transactivators, the consequence of dimerization is the juxtaposition of two regions richin basic residues that form a DNA-binding interface (24, 27,31, 35). By analogy, the basic residues preceding the HLH-likedomain of IE1 (Fig. 5) were predicted to be involved in hr binding.Replacement of R⁵²⁴ and K⁵²⁶ with alanine had little effect on IE1 oligomerization (Fig. 5and 6) or in vitro DNA binding (38). In contrast, replacementof residues R⁵³⁷ and R⁵³⁸, located immediately adjacent to the predicted HLH, caused lossof in vitro DNA binding as homo- and heterodimers (38) and eliminatedIE1 transactivation (Fig. 7C). Subsequent studies indicated thatIE1 nuclear localization was compromised by R⁵³⁷-R⁵³⁸ substitutions, possibly explaining the loss of transactivation(V. A. Olson, unpublished data). Although direct participationin DNA interactions by the these basic residues has not been resolved,other IE1 domains contribute to DNA binding. Mutagenesis of theconserved basic region centered at residue 156 also caused lossof in vitro DNA binding (38). Our studies reported here haveshown that IE1^I156 is impaired in hr-dependent transactivation but not non-hr-dependenttransactivation (Fig. 7). Since IE1^I156 is oligomerization competent (Fig. 2 and 4), its loss of DNAbinding may be due to the disruption of a DNA (hr)-binding domain.These results imply that IE1 differs from other basic-HLH transcriptionalactivators by possessing multiple DNA-binding domains. Furtherstudies are required to identify the regions of IE1 involved inhrbinding.

	ACKNOWLEDGMENTS

We thank Bob Liu for the construction of several of the plasmids used in this study and for helpful discussions. Steve Rodemsand Steve Pullen also provided plasmids andinsight.

This work was supported in part by Public Health Service grant AI25557 from the National Institute of Allergy and InfectiousDiseases.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute for Molecular Virology, Bock Laboratories, University of Wisconsin $---$ Madison,1525 Linden Dr., Madison, WI 53706-1596. Phone: (608) 262-7774.Fax: (608) 262-7414. E-mail: pfriesen{at}facstaff.wisc.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Hartlieb, B., Modrof, J., Muhlberger, E., Klenk, H.-D., Becker, S. (2003). Oligomerization of Ebola Virus VP30 Is Essential for Viral Transcription and Can Be Inhibited by a Synthetic Peptide. J. Biol. Chem. 278: 41830-41836 [Abstract] [Full Text]
Olson, V. A., Wetter, J. A., Friesen, P. D. (2003). The Highly Conserved Basic Domain I of Baculovirus IE1 Is Required for hr Enhancer DNA Binding and hr-Dependent Transactivation. J. Virol. 77: 5668-5677 [Abstract] [Full Text]
Olson, V. A., Wetter, J. A., Friesen, P. D. (2002). Baculovirus Transregulator IE1 Requires a Dimeric Nuclear Localization Element for Nuclear Import and Promoter Activation. J. Virol. 76: 9505-9515 [Abstract] [Full Text]

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