Characterization of the Single-Stranded DNA Binding Protein Encoded by the Vaccinia Virus I3 Gene

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J Virol, April 1998, p. 2917-2926, Vol. 72, No. 4
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Characterization of the Single-Stranded DNA Binding Protein Encoded by the Vaccinia Virus I3 Gene

S. Craig Rochester¹ and Paula Traktman¹^,²^,^*

Departments of Cell Biology¹ and Microbiology,² Cornell University Medical College, New York, New York 10021

Received 24 September 1997/Accepted 10 December 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The 34-kDa protein encoded by the I3 gene of vaccinia virus is expressed at early and intermediate times postinfection andis phosphorylated on serine residues. Recombinant I3 has beenexpressed in Escherichia coli and purified to near homogeneity,as has the protein from infected cells. Both recombinant and endogenousI3 protein demonstrate a striking affinity for single-stranded,but not for double-stranded, DNA. The interaction with DNA isresistant to salt, exhibits low cooperativity, and appears toinvolve a binding site of approximately 10 nucleotides. Electrophoreticmobility shift assays indicate that numerous I3 molecules canbind to a template, reflecting the stoichiometric interactionof I3 with DNA. Sequence analysis reveals that a pattern of aromaticand charged amino acids common to many replicative single-strandedDNA binding proteins (SSBs) is conserved in I3. The inabilityto isolate viable virus containing an interrupted I3 allele providesstrong evidence that the I3 protein plays an essential role inthe viral life cycle. A likely role for I3 as an SSB involvedin DNA replication and/or repair is discussed.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Vaccinia virus, the prototypic member of the poxvirus family, replicates in the cytoplasm of the host cell and exhibits aremarkable degree of genetic autonomy. Compartmentalization ofthe infectious cycle within the cytoplasm implies that the virusmust supply all essential components of the transcription andreplication machinery. Indeed, vaccinia virus is known to encodemany DNA replicative functions, including a DNA polymerase withintrinsic 5'-3' polymerization and 3'-5' exonuclease activity,a processivity factor, a DNA ligase, a thymidine kinase, a thymidylatekinase, and a ribonucleotide reductase (46). Phenotypic analysesof temperature-sensitive (ts) DNA mutants has also revealed essential roles for the B1 kinase andthe D5 nucleoside triphosphatase in DNA replication. Finally,a virally encoded uracil DNA glycosylase (UDG) appears to participatein viral replication (5, 26, 44), with a viral dUTPaseplaying a supportive role in maintaining the integrity of thegenomic DNA.

Our understanding of the minimal functions required for vaccinia virus DNA replication remains incomplete, with several functionspostulated by analogy with other systems as yet unidentified.The viral and cellular processes of DNA replication, recombination,and repair share a general requirement for single-stranded DNA(ssDNA) binding proteins (SSBs). These accessory proteins formspecific complexes with ssDNA which render it resistant to nucleasesand remove barriers of intramolecular secondary structure. Thishelix-destabilizing activity, as well as the establishment ofspecific protein-protein interactions, serves to stimulate severalreplication enzymes. For example, both human replication proteinA (hRPA) and bacteriophage T4 gene 32 protein have been foundto interact with and stimulate their cognate DNA polymerases (15,17).

At the onset of these studies, no vaccinia virus SSB had been identified biochemically, genetically or by sequence analysisof the predicted open reading frames (ORFs) encoded by the genome.Nevertheless, the inability of the purified viral DNA polymeraseto pass through barriers of DNA secondary structure in vitro (3,24) suggested that an SSB would be essential for viral replication.Our search for a candidate SSB was guided by early reports inthe literature of various abundant DNA binding proteins foundwithin virosomes, the cytoplasmic foci of vaccinia replication.Initial efforts were directed at identifying the gene encodinga 34-kDa phosphoprotein referred to variously as polypeptide B(29, 32) or FP11 (30, 33). Fortuitously, these experimentsled us to the analysis of a distinct 34-kDa polypeptide encodedby the vaccinia I3 gene. Here we describe the characterizationof this protein and demonstrate that it is the best candidatefor a vaccinia virus-encoded SSB.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Materials. Restriction endonucleases and DNA-modifying enzymes were obtained from Boehringer Mannheim Biochemicals (Indianapolis, Ind.)or New England Biolabs, Inc. (Beverly, Mass.). [³⁵S]methionine, ³²P_i, and ³²P-labeled nucleoside triphosphates were obtained from Dupont/NewEngland Nuclear Corp. (Boston, Mass.). Proteins (unlabeled, prestained,and ¹⁴C labeled) for use as molecular weight (MW) standards were obtainedfrom GIBCO/Bethesda Research Laboratories, Inc. (Gaithersburg,Md.). HindIII-digested lambda phage DNA and HaeIII-digested phage $phi$ X174 DNA size markers were from New England Biolabs. ProteinA-Sepharose and antibiotics were purchased from Sigma ChemicalCo. (St. Louis, Mo.); nitrocellulose was obtained from Schleicher& Schuell (Keene, N.H.). Immunoblots were developed with reagentsobtained from Bio-Rad (Richmond, Calif.). Denatured DNA-cellulosewas obtained from Sigma. Phosphocellulose resin was obtained fromWhatman BioSystems, Ltd. (Kent, England).

Cells and virus. The WR strain of vaccinia virus and various derivatives were propagated in BSC40 cells maintained in Dulbecco's minimal essentialmedium (DMEM) supplemented with 5% fetal calf serum (FCS) (GIBCOLaboratories, Grand Island, N.Y.). For the purification of I3protein, HeLa cells grown in suspension culture (Joklik-modifiedDMEM, 2.5% calf serum, 2.5% horse serum) were infected with vacciniavirus.

Preparation of a bacterial overexpression clone. A 1,511-bp segment of the vaccinia virus HindIII I genome fragment was subcloned into pUC19, using HindIII and BamHI sitesin both the insert and vector. This sequence included about 500bp of additional sequence 5' of the I3 ORF and about 300 bp ofadditional sequence at the 3' end. The entire I3 ORF, from a BspHIsite at the 5' end of the gene (nucleotide [nt] $-$ 3) to an RsaIsite at the 3' end of the gene (nt +865), was excised from thisparental pUC-HindIII-BamHI vector, resolved by Tris acetate-EDTA-agarosegel electrophoresis, and purified on glass beads (49). Thisfragment was cloned into a glass-purified pET 3c backbone (45)prepared by restriction with NdeI followed by blunting with theKlenow fragment of Escherichia coli DNA polymerase I. This constructwas used to direct the synthesis of the authentic I3 protein aftertransformation into competent E. coli HMS174.

Overexpression of the I3 34-kDa protein. HMS174 cells transformed with the pET-I3 clone were grown to a density of 4 × 10⁸ cells per ml in the presence of maltose (0.2%) and ampicillin(50 µg/ml). Cultures were then induced by infection with $lambda$ CE6at a multiplicity of infection (MOI) of 10 PFU per cell; 20 minof adsorption at room temperature was followed by incubation at37°C with agitation for 25 min. Cultures were then shaken at roomtemperature for 3 h. Uninduced cultures were grown under the sameconditions but were not infected with $lambda$ CE6. Some cultures weremetabolically labeled for 5 min at the end of the induction period;labeling was performed in M9 minimal medium supplemented with[³⁵S]methionine (10 µCi/ml) and the remaining unlabeled amino acids.Bacteria were collected by centrifugation at 5,000 × g for 5 min.Pellets were solubilized by freeze-thawing in lysis buffer (1ml/10 ml of culture) (50 mM Tris [pH 7.5], 1.0 M NaCl, 10 mM EDTA,1 mM dithiothreitol [DTT], 10% sucrose) containing lysozyme (0.2mg/ml) followed by incubation on ice for 30 min. After the additionof Triton X-100 to 0.1%, the extract was clarified by centrifugation,and the supernatant was retained and stored at $-$ 20°C.

Preparation of a polyclonal anti-I3 serum. Recombinant I3, overexpressed in E. coli from the pET-I3 vector described above, was excised from a sodium dodecyl sulfate(SDS)-polyacrylamide gel and used as an antigen for the generationof a rabbit polyclonal antiserum. The serum was effective in bothimmunoprecipitation and immunoblot (used at a dilution of 1:500)assays.

Metabolic labeling of infected cells. The temporal profile of I3 protein synthesis during viral infections was assessed by immunoprecipitation of extracts preparedfrom metabolically labeled cells. BSC-40 cells (10⁷) were infected with wild-type (wt) virus at an MOI of 15 PFUper cell. After 30 min of adsorption, the inoculum was removedand the cells were rinsed and fed with DMEM-FCS. At selected times,the infected cultures were pulse labeled for 30 min with [³⁵S]methionine (0.1 mCi/ml) in methionine-free DMEM and subsequentlyharvested. Cultures were rinsed with ice-cold phosphate-bufferedsaline (PBS; 140 mM NaCl, 2.7 mM KCl, 10 mM Na₂HPO₄, 1.5 mM KH₂PO₄[pH 7.4]) and disrupted in phospholysis buffer (100 mM NaPO₄ [pH7.4], 100 mM NaCl, 1% Triton X-100, 0.1% SDS, 0.5% sodium deoxycholate).Lysates were clarified by microcentrifugation at 4°C and storedat $-$ 20°C. I3 phosphorylation was examined by immunoprecipitationof extracts prepared from cells metabolically labeled with ³²P_i (0.1 mCi/ml) for 2 h in phosphate-free DMEM.

Immunoprecipitation. Thawed lysates representing 1.2 × 10⁶ cells were clarified and incubated with 4 µl of preimmune or anti-I3 serum on ice for4 h. Immune complexes were recovered with protein A-Sepharose;bound antigen was liberated from the complex by boiling in proteinsample buffer (1% SDS, 1% 2-mercaptoethanol, 50 mM Tris [pH 6.8],10% glycerol) and then resolved by electrophoresis through SDS-12%polyacrylamide gels (19). Dried gels were visualized by fluorography(2).

Immunofluorescence. BSC40 cells were grown to confluence in Labtek eight-chamber slides (Nunc, Inc., Naperville, Ill.) and either left uninfectedor infected with wt vaccinia virus at an MOI of 15 in the presenceor absence of cytosine arabinoside (20 µg/ml). At designated timespostinfection, slides were chilled on ice and monolayers wererinsed with cold PBS and then fixed with 4% paraformaldehyde inPBS for 15 min at 4°C. Cells were then rinsed two times with coldPBS, permeabilized with 0.1% Triton X-100 in PBS for 5 min, andrinsed again. Clarified preimmune or anti-I3 immune serum wasthen applied for 1 h at a dilution of 1:50. Cells were washedthree times with cold PBS and then incubated with fluoresceinisothiocyanate-conjugated goat anti-rabbit immunoglobulin G (JacksonImmunoResearch Laboratories, Inc., West Grove, Pa.) at a dilutionof 1:100. When used in parallel to detect nucleic acids. Hoechst33258 (Polysciences, Inc., Warrington, Pa.) was applied at a concentrationof 0.5 µg/ml in PBS. Monolayers were rinsed four times with coldPBS, and then glass coverslips were mounted over Aquamount (LernerLabs, Pittsburgh, Pa.). Immunofluorescence was detected with aMicrophot EPI FL fluorescence microscope (Nikon, Inc., GardenCity, N.Y.). Photographic slides of these images were then scannedusing a Nikon Coolscan II scanner and Adobe Photoshop software(Adobe Systems, Inc., San Jose, Calif.). The figures were labeledby using Canvas software (Deneba Systems, Inc.), and final imageswere obtained with a Kodak dye sublimation printer.

One-dimensional phosphoamino acid analysis. ³²P-labeled vaccinia virus-infected cell extracts were subjected to immunoprecipitation as described above. Protein was elutedfrom protein A-Sepharose by boiling for 5 min in protein samplebuffer without dye. Proteins were precipitated by the additionof trichloroacetic acid to 10% followed by incubation on ice for60 min. Precipitates were collected by microcentrifugation at4°C for 15 min, rinsed with 100% ethanol ( $-$ 20°C), and air dried.Samples were resuspended in 50 µl of constant-boil HCl (Pierce,Rockford, Ill.) and heated at 110°C for 1 h; hydrolysates werecollected by lyophilization and resuspended in distilled H₂O.Hydrolyzed samples and phosphoamino acid markers (20 nmol) werespotted on thin-layer cellulose F chromatography plates (EM Separations,Gibbstown, N.J.). Electrophoresis was performed in pyridine-glacialacetic acid-water (1:10:189) at 2,000 V for 15 min. The plateswere dried, sprayed with ninhydrin (Sigma), developed at 65°Cfor 20 min, and exposed for autoradiography.

Purification of recombinant I3. Induced pET-I3 bacterial pellets from 2 liters of culture were frozen, thawed, resuspended in 200 ml of pET lysis buffer containing1 M NaCl and 0.2 mg of lysozyme per ml, and incubated for 30 minon ice. Triton X-100 was added to 0.1%; lysates were subjectedto vigorous vortexing and clarified by centrifugation at 14,000× g for 30 min. Lysates were then adjusted to contain 50 mM sodiumacetate, 12 mM MgCl₂, and 4 mM CaCl₂ and then treated with 20µl of DNase I (0.1 µg/ml) for 30 min at 25°C. The reaction wasstopped by adding EDTA to 6 mM and EGTA to 3 mM. The lysate wasthen dialyzed against 2 liters of buffer A (40 mM Tris [pH 7.4],50 mM NaCl, 6 mM EDTA, 3 mM EGTA, 1 mM $beta$ -mercaptoethanol, 10%glycerol). All purification steps were performed on a PharmaciaFPLC apparatus at 4°C. Gradient fractions (and I3 purificationprofiles) were typically monitored by immunoblot and silver-stainedSDS-polyacrylamide gel analysis. Protein concentrations were determinedby using the Bradford method and bovine serum albumin (BSA) asa standard. The dialysate (fraction I, 200 ml) was subjected toammonium sulfate precipitation. The 40 to 60% pellet fractionwas resuspended in 20 ml of buffer A and applied to a 15-ml ssDNA-cellulosecolumn that had been equilibrated with buffer A. The column wasdeveloped with an 80-ml linear gradient containing 50 mM to 2.5M NaCl. Peak I3 fractions were pooled and concentrated by reversedialysis using polyethylene glycol (fraction II). Fraction IIwas subsequently dialyzed against buffer B (50 mM Tris [pH 7.4],50 mM NaCl, 1 mM EDTA, 2 mM $beta$ -mercaptoethanol, 5% glycerol).

Purification of I3 from vaccinia virus-infected cells. HeLa cells (5 × 10⁹) in suspension culture were infected with wt vaccinia virus at an MOI of 15 in the presence of hydroxyurea(10 mM) and harvested at 5 h postinfection (hpi). Cytoplasmicextracts were prepared by hypotonic lysis as described previously(25), and fractionated by chromatography on a 25-ml DEAE-cellulosecolumn equilibrated in DEAE buffer (50 mM Tris [pH 7.4], 1 mMDTT, 1 mM EDTA, 10% glycerol)-50 mM NaCl, and developed with astepwise elution of NaCl in DEAE buffer. I3 was recovered in theflowthrough and applied to a 10-ml ssDNA-cellulose column (equilibratedin DEAE buffer-50 mM NaCl) that was then developed with a lineargradient of 50 mM to 2.5 M NaCl in DEAE buffer. Peak I3 fractionswere pooled, dialyzed against buffer B, and concentrated by polyethyleneglycol reverse dialysis. The purification yielded approximately0.5 mg of pure I3 from 5 × 10⁹ infected cells.

Gel filtration analysis of purified endogenous I3. A 200-µl sample containing 25 µg of I3 in 200 mM NaCl-20 mM Tris (pH 7.4)-1 mM DTT-1 mM EDTA-5% glycerol was injected ontoa 24-ml Superdex 75 column. The column was equilibrated and developedin the same buffer, and chromatography was performed at 0.25 ml/minon a Pharmacia FPLC apparatus at 4°C. Fractions of 0.5 ml werecollected. The profile of I3 within the fractions was determinedby SDS-polyacrylamide gel electrophoresis (PAGE) and immunoblotanalysis. Chromatography was also performed with the followingprotein standards of known Stokes radii in order to calibratethe column: BSA, 36.1 Å; chicken ovalbumin, 27.5 Å; and myoglobin,19 Å. Dextran blue and L-tryptophan were used to determine thecolumn's void and total volumes, respectively. The Stokes radiiand molecular weights of the I3 species observed were calculatedby the method of Siegel and Monty (43).

Electrophoretic mobility shift assays (EMSAs). Oligonucleotides were prepared with an Applied Biosystems (Foster City, Calif.) model 391 DNA synthesizer. Full-length oligonucleotideswere purified by using Poly-Pak cartridges (Glen Research, Sterling,Va.). The 5' terminus was radiolabeled with [ $gamma$ -³²P]ATP and T4 polynucleotide kinase. For the preparation of double-strandedoligonucleotides, complementary 5'-labeled oligonucleotides werehybridized as described previously (27). DNA probes and proteinsamples were mixed in reaction mixtures containing 250 µg of BSAper ml, 20 mM Tris (pH 7.4), 50 mM NaCl, 1 mM EDTA, and 5% glycerol.Then 15-µl reaction mixtures were incubated at 30°C for 15 min,added to 1 µl of 5× loading buffer, and analyzed by low-ionic-strength,nondenaturing, 15% polyacrylamide gel electrophoresis. Standardvertical gels were cast and run in 0.25× TBE (25 mM Tris, 21 mMboric acid, 0.25 mM EDTA); electrophoresis was performed at 200V for 4 h at 4°C. Gels were then dried and exposed for autoradiography.Bands were quantitated with a phosphorimager.

Denatured DNA-cellulose chromatography of vaccinia virus-infected cell extracts. BSC-40 cells (1.4 × 10⁸) were infected with wt vaccinia virus at an MOI of 15 PFU per cell. Adsorption was carried out for30 min, at which time monolayers were rinsed with either methionine-freeDME in the case of [³⁵S]methionine labeling or phosphate-free DME in the case of ³²P_i labeling. Cells were then immediately labeled with medium containingeither [³⁵S]methionine (0.1 mCi/ml) or ³²P_i (0.1 mCi/ml) for 5 h. Cytoplasmic extracts were prepared byhypotonic lysis (25) of labeled cells, and lysates were treatedwith DNase I as described above for recombinant protein purification.Each lysate was then dialyzed against buffer A and applied toa 5-ml ssDNA-cellulose column which had been equilibrated withbuffer A. The columns were developed with a 60-ml linear gradientof 50 mM-2.5 M NaCl. Resulting fractions were analyzed by SDS-PAGE(12% gel) and subjected to autoradiography, silver staining, andimmunoblot analysis.

Construction of an I3 null allele by replacing I3 with the Neo^r gene. The pUC HindIII-BamHI plasmid containing 1,511 bp of the HindIII I fragment was cleaved with XbaI and BglII to release a 383-bpfragment representing 46.5% of the I3 gene. The backbone was thentreated with phosphatase, made blunt with the Klenow fragmentof DNA polymerase I, resolved by Tris acetate-EDTA-agarose electrophoresis,and purified on glass beads. The neomycin resistance (Neo^r) gene under the direction of the vaccinia virus early/late p7.5promoter was excised from pVVNEO (8) by digestion with SalIand XbaI; the termini were then made blunt with the Klenow fragmentof DNA polymerase I. The Neo^r cassette was inserted into the XbaI-BglII site of the pUC HindIII-BamHIplasmid in place of the I3 sequence. Two pI3:NEO constructs, inwhich the Neo^r cassette was oriented in either direction relative to the flankingsequences, were selected. These plasmids retained 752 bp of viralsequence upstream of, and 376 bp downstream of, the Neo^r sequence to facilitate recombination into the vaccinia virusgenome. BSC-40 cells in 35-mm-diameter dishes were infected withwt vaccinia virus at an MOI of 0.03 PFU per cell; at 3 hpi thereplicate dishes were independently transfected with 3.5 µg ofa calcium phosphate precipitate of either supercoiled or linearizedpI3:NEO DNA. G418 (2 µg/ml) was added to the medium at 15 hpi;cultures were maintained at 37°C in the presence of drug until3 days postinfection. Monolayers were harvested and subjectedto two cycles of freeze-thawing to release cell-associated virus.Viral yields were then titrated, and each stock was independentlypassaged twice through BSC-40 cells at 37°C in the presence ofG418 to enrich for recombinant progeny. Two rounds of plaque purificationwere then performed to prepare Neo^r isolates from each of 16 original infections/transfections. Elevenof these had been transfected with supercoiled pI3:NEO (five inone orientation and six in the other); five had received linearizedpI3:NEO (two in one orientation and three in the other). Viralexpansions were then prepared from these isolates, and portionsof the stocks were applied to Zetaprobe (Bio-Rad) with a dot blotapparatus (Bio-Rad). Duplicate filters were then hybridized withone of four radioactive probes prepared by nick translation (38):(i) an 8.1-kb fragment derived from the vaccinia virus HindIIID genomic fragment, (ii) the excised Neo^r gene (without any vaccinia virus sequences), (iii) the 353-bpinternal fragment deleted from the I3 gene during the preparationof pI3:NEO (a probe for the wild-type I3 allele), and (iv) pUC19plasmid DNA.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

With the aim of identifying a viral SSB, we investigated the possibility that a protein previously described in the vacciniavirus literature and designated polypeptide B (29, 32) orFP11 (30, 33) might serve this function. This protein hadbeen described as an abundant DNA binding phosphoprotein of 34kDa which was a major component of virosomes (replication factories).

We set out to map the gene encoding this protein by using the technique of hybrid selection (7, 35, 37, 48). HindIIIrestriction fragments spanning the genome were used to selectearly viral mRNAs which were in turn translated in vitro; radiolabeledprotein products were resolved on SDS-12% polyacrylamide gels(data not shown) and compared to ³⁵S- and ³²P-labeled extracts prepared from infected cells. An abundant 34-kDaprotein whose mRNA was selected by the HindIII I fragment waschosen for further analysis and shown to be encoded by the I3ORF.

The I3 gene of vaccinia virus is predicted to encode a 267-amino-acid protein which exhibits no significant homology withother protein sequences (9, 16, 39). Transcriptional analysishas shown that I3 mRNA is synthesized at both early and intermediatetimes postinfection. Indeed, the sequences upstream of the I3gene contain characteristic promoter elements for both early andintermediate vaccinia virus gene expression (14). From the outsetwe wished to characterize those properties of the I3 protein whichmight bear on its potential as an SSB. We began by cloning theauthentic ORF into expression vectors which would enable us toobtain large quantities of recombinant protein for both antibodyproduction and biochemical characterization.

Characterization of the temporal expression pattern of I3 during vaccinia virus infection. Authentic I3 protein was expressed in E. coli through the use of the pET vector system (45). Upon induction of the T7 promoterby infection with a bacteriophage carrying the T7 RNA polymerasegene, the I3 protein accumulated to significant levels (Fig. 1A,lanes 1 and 2). This protein was used in the preparation of apolyclonal anti-I3 serum as described in Materials and Methods.This antiserum was used to examine the temporal regulation ofI3 protein synthesis and to look at I3 protein localization withinvaccinia virus-infected cells by immunofluorescence.

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FIG. 1. Analysis of I3 expression in E. coli and in vaccinia virus-infected cells. (A) Synthesis of recombinant I3 in E. coli transformants containing plasmid pET-I3. Extracts from uninduced (U) or induced (I) bacteria are shown in lanes 1 and 2, respectively; the 34-kDa I3 protein is apparent in induced extracts. Cultures were metabolically labeled with [³⁵S]methionine as described in Materials and Methods prior to being harvested and analyzed by SDS-PAGE and fluorography. (B) Temporal profile of I3 synthesis. Parallel cultures were left uninfected (M), infected with wt vaccinia virus (MOI of 15), and harvested at 2, 3, 4, 6, or 8 hpi or were infected with wt vaccinia virus (MOI of 15) in the presence of cytosine arabinoside and harvested at 4 hpi (C). Cells were metabolically labeled with [³⁵S]methionine for 45 min prior to being harvested. Aliquots of total cellular lysates (lanes 1 to 7) as well as the species recovered after immunoprecipitation with anti-I3 serum (lanes 8 to 14) were analyzed by SDS-PAGE and fluorography. (C) I3 is phosphorylated in vivo. Cells infected with wt vaccinia virus (MOI of 15) were metabolically labeled with ³²P_i from 1 to 3 or 3 to 5 hpi and harvested at the end of the labeling period. The time of harvest is shown above the lanes. Lysates were subjected to immunoprecipitation with preimmune serum (P.I.) or anti-I3 serum and subjected to SDS-PAGE and fluorography. ¹⁴C-labeled protein standards are shown at the far left in the lane marked MW, with their molecular masses indicated. The arrow at the far right shows the position of electrophoretic migration of both recombinant and authentic I3 protein.

To determine the temporal profile of I3 synthesis, BSC-40 cells were infected with wt virus at an MOI of 15 PFU per cell at37°C, radiolabeled with [³⁵S]methionine for 30 min at various times postinfection, and harvestedimmediately. Extracts were subjected to immunoprecipitation analysiswith the anti-I3 serum; the recovered immune complexes were fractionatedby SDS-PAGE and visualized by fluorography. The fluorographs (Fig.1B) reveal that the temporal pattern of I3 expression is thatof both an early and an intermediate vaccinia virus protein. Synthesisof I3 in the presence of cytosine arabinoside verifies that itis indeed an early gene (Fig. 1B, lane 14). That it is also anintermediate gene is demonstrated by the observation that althoughI3 synthesis is initiated by 2 hpi (lane 9), it reaches maximallevels at 3 to 4 hpi (lanes 10 and 11). That I3 is not a lategene is evident by the fact that synthesis begins to decline by6 hpi and is minimal by 8 hpi (lanes 12 and 13). This profileof protein synthesis is mirrored in immunoblot analyses of I3accumulation (data not shown), which show that I3 levels havereached a plateau by 8 hpi. This temporal profile would ensurethat I3 was present at the onset of DNA replication and throughoutits duration but suggests that I3 is unlikely to be a major componentof newly assembled virions.

Immunoprecipitation analysis was also used to assess the phosphorylation of I3 in vaccinia virus-infected cell extracts (Fig.1C). BSC-40 cells were infected with wt vaccinia virus at an MOIof 15 PFU per cell at 37°C and radiolabeled with ³²P_i at various times postinfection. Extracts were subjected toimmunoprecipitation with anti-I3 serum. Substantial levels ofI3 phosphorylation were seen in extracts labeled from 1 to 3 or3 to 5 hpi (Fig. 1C, lanes 2 and 3). No such radiolabeled specieswas recovered when preimmune serum was used instead (Fig. 1C,lane 1).

I3 is phosphorylated on serine residues. ³²P-labeled I3 immunoprecipitates were used as substrates for phosphoamino acid analysis. Briefly, liberated I3 immunocomplexeswere precipitated, resuspended in concentrated HCl, and subjectedto partial hydrolysis by heating at 110°C for 1 h. Lyophilizedamino acids were then analyzed by one-dimensional high-voltagethin-layer electrophoresis. As shown in Fig. 2, in which identicalsamples were mixed with unlabeled phosphoamino acid standardsindividually (lanes 1 to 3) or together (lane 4), I3 is phosphorylatedexclusively on serine residues. Since similar studies on polypeptideB have shown it to be phosphorylated on threonine residues (29),our data suggest that I3 and polypeptide B are not the same protein.

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FIG. 2. I3 is phosphorylated on serine residues. Cells were infected with wt virus (MOI of 15) and metabolically labeled with ³²P_i. Lysates were prepared and subjected to immunoprecipitation with anti-I3 serum. Liberated immune complexes were subjected to trichloroacetic acid precipitation and then to hydrolysis with HCl. The hydrolysates were mixed with phosphoamino acid markers either individually (lanes 1 through 3) or as a mixture (lane 4). Samples were then applied to thin-layer cellulose plates and resolved by high-voltage electrophoresis. Markers were visualized by color development with ninhydrin; radiolabeled phosphoamino acids derived from I3 were visualized by autoradiography. The dotted wickets indicate the positions of migration of the phosphoserine (pSerine), phosphothreonine (pThreonine), and phosphotyrosine (pTyrosine) markers. The position of migration of free phosphate is indicated, as is the application origin.

Localization of I3 within vaccinia virus-infected cells by immunofluorescence. A presumed role for I3 as a viral SSB would place it in the virosome during infection, perhaps with this localization dependenton ongoing DNA synthesis. We used immunofluorescence microscopyto address the issue of intracellular localization of I3 duringvaccinia virus infection. As shown in Fig. 3A, BSC cells infectedwith vaccinia virus and fixed at 4 hpi display large discretecytoplasmic foci of fluorescence only when incubated with anti-I3immune serum. Mock-infected cells incubated with immune serum(Fig. 3F) or infected cells incubated with preimmune serum (Fig.3G) exhibited no fluorescence. To control for the possibilitythat the observed foci represented nonspecific aggregates of I3,monolayers were infected in the presence of the DNA replicationinhibitor cytosine arabinoside. These infections showed a morediffuse pattern of cytoplasmic staining with some small punctatefoci, as seen in Fig. 3B and C. This result indicates that I3localization is in fact dependent on DNA replication and accumulationwithin virosomal structures. Indeed, analysis of infected cellsdoubly labeled with anti-I3 serum and Hoechst 33258 show an equivalencebetween cytoplasmic nucleic acid (virosomal) staining (Fig. 3D)and I3 staining (Fig. 3E).

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FIG. 3. I3 protein localizes to discrete cytoplasmic foci that are coincident with virosomes. Mock- or virus-infected BSC-40 cells were processed for immunofluorescence as described in Materials and Methods. The panels represent the following treatments: (A) vaccinia virus infected, anti-I3 serum; (B and C) vaccinia virus infected in the presence of cytosine arabinoside (20 µg/ml), anti-I3 serum; (D and E) vaccinia virus infected, anti-I3 serum plus Hoechst 33258; (F) mock infected, anti-I3 serum; (G) vaccinia virus infected, preimmune serum. Panels D and E represent the same field.

Purification of recombinant and endogenous I3. To begin analyses of the biochemical properties of the I3 protein, we purified both the recombinant protein from E. coli andthe endogenous protein from vaccinia virus-infected cells. Althoughseveral chromatographic strategies were attempted, the followingprotocols were especially effective and capitalized on the obviousaffinity of I3 for ssDNA.

(i) Recombinant I3. Recombinant I3 protein was purified to near homogeneity from soluble extracts generated by induction of bacteria containingplasmid pET-I3 with $lambda$ CE6 at 25°C. Cell lysis was performed underhigh-salt conditions to maximize protein solubility and to dissociateprotein-DNA complexes. Lysates were then treated with DNase Ito digest endogenous DNA which might compete with immobilizedssDNA-cellulose for I3 binding. Lysates were subjected to ammoniumsulfate precipitation, and the 40 to 60% pellet fraction was appliedto an ssDNA-cellulose column which was developed with increasingconcentrations of NaCl. I3 eluted in a broad peak between 1.0and 2.0 M NaCl and was purified to near homogeneity by this procedure,as assessed by SDS-PAGE and silver stain (Fig. 4A) and immunoblot(not shown) analyses. This source of I3 is especially useful becauseit is free of other viral proteins and is presumably not phosphorylated.

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FIG. 4. Purification of recombinant and authentic I3. (A) Purification of I3 from E. coli transformants containing pET-I3. Expression of I3 was induced as described in Materials and Methods, and I3 was purified by ammonium sulfate precipitation and chromatography on ssDNA-cellulose. Aliquots of uninduced cultures (lane 2), of induced cultures (17 µg of protein; lane 3), and of each purification step (lanes 4 [29 µg of protein] and 5 [0.6 µg of protein] are shown. Positions of MW markers (lane 1) are shown in kilodaltons at the left. Proteins were resolved by SDS-PAGE and visualized by silver staining. (B) Purification of endogenous I3. I3 was purified from cells infected with wt vaccinia virus as described in Materials and Methods. Aliquots of the unfractionated lysate and peak fractions from the DEAE-cellulose and ssDNA-cellulose columns were analyzed by SDS-PAGE and silver staining. Amounts of protein analyzed: lane 2, 50 µg; lane 3, 20 µg; lane 4, 1.2 µg. Protein MW standards were resolved in lane 1; the corresponding molecular masses are indicated in kilodaltons at the left.

(ii) I3 from vaccinia virus-infected cells. Eight liters of a suspension culture of HeLa cells was infected with vaccinia virus at a high MOI in the presence of hydroxyurea.Cytoplasmic extracts were subjected to DEAE-cellulose chromatography,and the protein pool eluting with 50 mM NaCl was applied to anssDNA-cellulose column. The column was developed with a lineargradient of 50 mM to 2.75 M NaCl. A broad peak of I3 protein elutedbetween 1.0 and 2.0 M NaCl and was shown to be purified to nearhomogeneity, as assessed after SDS-PAGE by silver staining (Fig.4B) and immunoblot (not shown) analyses. This purification yielded0.5 mg of pure protein from 5 × 10⁹ infected cells. Compared with the purification of 0.2 mg of overexpressedD5 (6) and 0.3 mg of overexpressed DNA polymerase (25) from2 × 10⁸ and 1 × 10⁹ infected BSC-40 cells, respectively, this yield indicates thatI3 is expressed at high levels during the early phase of wt infections.

Determination of the native MW of the I3 protein. Gel filtration chromatography was performed on both recombinant and endogenous forms of I3 to examine their native MW in solution.Elution profiles of I3 from a Superdex 75 FPLC column were comparedto those of known standards; I3 eluted just after the peak ofovalbumin (MW, 44,000) (not shown). A Stokes radius of 24.7 Åwas calculated by the method of Siegel and Monty (43). An MWof 34,000 was extrapolated for I3 based on a plot of MW versusStokes radius for protein standards, indicating that I3 existsas a monomer in solution.

Recombinant I3 binds specifically to single-stranded oligonucleotides. The chromatographic properties of I3 suggested that it did indeed have a high affinity for ssDNA (Fig. 4A). To explore theDNA binding character of I3 protein in more detail, we performedEMSAs. As shown in Fig. 5A, purified recombinant I3 formed a specificprotein-DNA complex with a 5'-labeled single-stranded 24-nt probein a concentration-dependent manner. In contrast, virtually noDNA binding was seen if a double-stranded oligonucleotide of thesame sequence was used as the probe (Fig. 5B). The plot of thesedata shown in Fig. 5C illustrates the striking specificity ofI3 for ssDNA.

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FIG. 5. EMSAs show that I3 binds specifically to ssDNA. (A) Analysis of complex formation between purified, recombinant I3 and ssDNA oligonucleotides. Reaction mixtures contained 0.2 pmol of a single-stranded, terminally ³²P-labeled 24-mer oligonucleotide and various amounts of I3. Amounts of I3 used: lane 1, 0 pmol; lane 2, 0.3 pmol; lane 3, 0.6 pmol; lane 4, 1.3 pmol; lane 5, 2.0 pmol; lane 6, 2.6 pmol; lane 7, 3.2 pmol; lane 8, 3.9 pmol; lane 9, 4.6 pmol; lane 10, 5.2 pmol. After incubation for 15 min at 30°C, samples were fractionated on a 15% nondenaturing polyacrylamide gel at 4°C and visualized by autoradiography. (B) Analysis of complex formation between purified, recombinant I3 and double-stranded DNA oligonucleotides. Reactions were carried out and analyzed as for panel A except that protein samples were mixed with 0.2 pmol of a terminally radiolabeled double-stranded 24-mer oligonucleotide identical in sequence to that used for panel A. (C) Graphic representation of I3-DNA complex formation. The data in panels A and B were quantitated by phosphorimaging and plotted as shown. The ordinate represents the picomoles of DNA bound, as determined by measuring the decrease in the levels of free probe remaining; the abscissa represents the amount of I3 in the reaction. ds, double-stranded.

I3-ssDNA complexes are highly salt resistant. The elution profile of I3 from ssDNA-cellulose had suggested to us that the I3-DNA interaction was a strong one. Those experimentsmonitored the salt sensitivity of I3-DNA interactions in the presenceof multiple other proteins. To examine the salt sensitivity ofthe binding of purified recombinant I3 to DNA, EMSAs were performedin the presence of various concentrations of NaCl. As shown inFig. 6A, no diminution of complex formation was seen until theNaCl concentration reached 0.5 M, and significant binding remainedeven in the presence of 1 M NaCl. The observation that the additionof increasing amounts of unlabeled single-stranded 24-mer midwaythrough a 30-min incubation could fully compete for I3 binding(Fig. 6B), displacing it from the radiolabeled probe, confirmsthat our assays are detecting a classic, noncovalent equilibriuminteraction between protein and DNA.

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FIG. 6. I3-DNA interaction: NaCl titration and competition analyses. (A) The interaction of I3 with ssDNA is salt resistant. Reaction mixtures containing 3.3 pmol of recombinant I3 and 0.2 pmol of radiolabeled single-stranded 24-mer were incubated at 30°C for 15 min in buffer containing the indicated concentration of NaCl. Samples were fractionated on a 15% nondenaturing polyacrylamide gel at 4°C and visualized by autoradiography. (B) The interaction of I3 with ssDNA can be reversed by the addition of unlabeled competitor DNA. Reaction mixtures containing 3.3 pmol of recombinant I3 and 0.2 pmol radiolabeled single-stranded 24-mer were incubated at 30°C for 15 min. Unlabeled single-stranded 24-mer was then added to the levels indicated, and reaction mixtures were incubated for an additional 15 min at 30°C. Samples were then fractionated on a 15% nondenaturing polyacrylamide gel at 4°C and visualized by autoradiography.

I3 forms distinct complexes on longer oligonucleotides. To assess the topology of I3's interaction with DNA, EMSAs were performed with single-stranded oligonucleotides of increasinglength. I3 was shown to form a ladder of discrete complexes onlonger probes. As shown in Fig. 7 in an autoradiograph of a 5to 20% gradient acrylamide gel, the number of complexes seen increasesas probe length is increased. This is seen most clearly at limitingprotein concentrations, since complexes are chased to saturated,lower-mobility species at high I3 concentrations. From the numberof complexes seen with each oligonucleotide used, we can estimatethe binding site size to be approximately 10 nt per I3 molecule(seven complexes are seen with the 73-mer, five are seen withthe 53-mer, three are seen with the 34-mer etc.). However, wefind that I3 will not bind to a 12-mer in this assay (not shown),indicating that the minimum length for binding is between 13 and18 nt. The ability to detect the full array of different complexesunder conditions in which most of the probe remains free stronglysuggests that I3 binds to DNA in a noncooperative manner.

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FIG. 7. Analysis of the binding site size of I3 on ssDNA. Reaction mixtures contained either 10.5, 1.5, or 0 pmol of purified recombinant I3 and 0.2 pmol of a terminally radiolabeled oligonucleotide of 18, 24, 34, 53, or 73 nt in length. After 15 min of incubation at 30°C, samples were fractionated on a nondenaturing, 5 to 20% polyacrylamide gradient gel at 4°C and visualized by autoradiography.

Endogenous I3 also shows a strong preference for ssDNA. A comparison of the DNA binding properties of recombinant and endogenous I3 is shown in Fig. 8. The two proteins show comparablebinding to the radiolabeled 24-nt probe, although the mobilitiesof the complexes formed are somewhat different in this particularexperiment (Fig. 8A). Recombinant I3 appears to form two complexes,whereas endogenous I3 forms only the more slowly migrating ofthese two species. As shown in Fig. 8B, the endogenous I3 alsohas a very strong preference for ssDNA.

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FIG. 8. Endogenous I3 binds specifically to ssDNA. (A) Comparison of the binding of endogenous and recombinant I3 to ssDNA. Reaction mixtures containing 0.2 pmol of radiolabeled single-stranded 24-mer oligonucleotide and the indicated amounts of either endogenous I3 (VV I3) (lanes 1 to 5) or recombinant I3 (Rec I3) (lanes 6 to 11) were incubated at 30°C for 15 min, fractionated on a 15% nondenaturing polyacrylamide gel at 4°C, and visualized by autoradiography. (B) Comparison of the binding of endogenous I3 to single-stranded and double-stranded DNA. Reaction mixtures contained 0.2 pmol of radiolabeled single-stranded 24-mer oligonucleotide (lanes 1 to 3) or 0.2 pmol radiolabeled double-stranded (ds) 24-mer oligonucleotide (of identical sequence) (lanes 4 to 6) and the indicated amounts of purified endogenous I3. After incubation for 15 min at 30°C, samples were fractionated on a 15% nondenaturing polyacrylamide gel at 4°C and visualized by autoradiography.

I3 saturates M13 ssDNA with low cooperativity. The issue of whether recombinant and/or endogenous I3 bind ssDNA in a cooperative fashion was also addressed in assays usingsingle-stranded, circular M13 DNA and increasing concentrationsof I3 (23). Under conditions of DNA excess, highly cooperativebinding would result in two bands after electrophoretic fractionthrough agarose: one representing fully saturated DNA, and onerepresenting free DNA. As protein concentration increased, theintensity of the saturated DNA band would increase. In the absenceof cooperativity, one would expect to see a random distributionof protein-DNA complexes, manifested in a diffuse band whose mobilitywould decrease as protein concentration increased. I3 bindingto the 7.2-kbp M13 ssDNA clearly progressed through the formationof a random population of protein-DNA complexes which were ofdecreasing mobility with increasing protein concentration (Fig.9). Equivalent titrations are presented for recombinant I3 andfor endogenous I3; again, although the profiles are similar, themobilities of the complexes seen are somewhat different. Elevationof the NaCl concentration in these reactions to 100 or 250 mMhad no effect on the distribution of the shifted species (datanot shown). Therefore, we do not observe a qualitative salt-dependentchange in the cooperativity of DNA binding.

Chromatographic profile of I3 on ssDNA cellulose: phosphorylation does not appear to affect affinity. In our comparisons of the interactions of recombinant and endogenous I3 with DNA, we found similarities in preference forssDNA (Fig. 5 and 8), stoichiometry of binding (Fig. 8), and lackof cooperativity (Fig. 9). These results suggested that the phosphorylationof endogenous I3 probably had little effect on the DNA bindingproperties of the protein. During the course of these studies,however, data from another laboratory suggested that this mightnot be so. Davis and Mathews (4) identified I3 as a proteinlikely to interact with the vaccinia virus-encoded ribonucleotidereductase by screening vaccinia virus expression libraries withan anti-idiotype antibody raised against anti-ribonucleotide reductase(small subunit). Their studies suggested that whereas ³⁵S-labeled I3 could be coprecipitated with nascent viral DNA metabolicallylabeled with bromodeoxyuridine, ³²P-labeled I3 could not.

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FIG. 9. I3 binds to ssDNA with low cooperativity. Reaction mixtures containing 0.316 pmol of M13mp18 single-stranded circular DNA (7,249 bases) and various amounts (0, 20, 40, 60, 80, 100, and 120 pmol) of either recombinant (lanes 1 to 7) or endogenous (lanes 8 to 14) I3 protein were incubated at 30°C for 15 min. Reaction mixtures were then fractionated by electrophoresis through a 0.5% agarose gel; the gel was stained in 2 M NaCl-ethidium bromide, and DNA bands were visualized by UV illumination.

We addressed this issue further by looking at the association of I3 with ssDNA-cellulose either [³⁵S]methionine-labeled (Fig. 10A) or ³²P_i-labeled (Fig. 10B) cytoplasmic extracts. Fractions eluted fromthe column were analyzed by SDS-PAGE (12% gel) and visualizedby silver staining (data not shown), immunoblot analysis, andautoradiography. As assessed by silver staining and immunoblotanalysis, I3 elutes from ssDNA-cellulose as a broad peak from0.5 to 2 M NaCl. These gels also show that I3 is by far the mostabundant (silver stain analysis) and highly synthesized (autoradiography)protein retained on the ssDNA matrix under stringent wash conditions.³²P-labeled I3 also elutes as a broad peak that extends until thehighest salt concentrations, indicating that phosphorylated I3does not have a reduced affinity for ssDNA. (The highly radiolabeledspecies of approximately 34 kDa that appears to elute prior toimmunoreactive I3 does not comigrate precisely with I3 and probablyrepresents the H5 protein.) In support of this conclusion, wehave also shown that recombinant I3, which is almost certainlynot phosphorylated, exhibits the same affinity for ssDNA-celluloseseen with endogenous I3.

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FIG. 10. Chromatographic profile of [³⁵S]methionine-labeled and ³²P_i-labeled I3 on denatured DNA-cellulose. (A) BSC-40 cells were infected for 5 h with wt virus (MOI of 15) at 37°C and metabolically labeled with [³⁵S]methionine throughout. Cytoplasmic extracts were prepared as described in Materials and Methods and applied to a 5-ml denatured DNA-cellulose column. The column was developed with a 60-ml linear gradient of 50 mM to 2.5 M NaCl. Fractions were analyzed by SDS-PAGE (12% gel), and the gel was subjected to autoradiography. Lanes: M, ¹⁴C-labeled protein standards (molecular masses are shown in kilodaltons at the left); Load, total cytoplasmic lysate; FT, flowthrough; Wash, material eluting in a 10-ml 50 mM NaCl wash. The remaining lanes contain the samples eluting during development with the NaCl gradient. The majority of the fractions were also subjected to immunoblot analysis using the I3 antiserum; the relevant portion of the blot is positioned below the autoradiograph. (B) BSC-40 cells were infected for 5 h with wt virus (MOI of 15) at 37°C and metabolically labeled with ³²P_i throughout. Cytoplasmic extracts were prepared and analyzed as described above for panel A.

Attempted generation of an I3 null mutant virus. The data presented above demonstrate that I3 is the best candidate for a viral SSB $---$ it is one of the most abundant viral proteinssynthesized prior to and during DNA replication and exhibits thestrongest and most specific affinity for ssDNA. A role as an SSBwould almost certainly require that I3 be an essential viral function.To determine whether I3 was in fact essential for viral replication,we attempted to isolate a viral recombinant in which the I3 allelehad been inactivated by insertion of a selectable marker. BSC-40cells infected with wt vaccinia virus were transfected with aplasmid construct containing modified HindIII I sequences; 46.5%of the I3 gene was deleted and replaced with the Neo^r gene under the control of a constitutive vaccinia virus promoter.Infected cells were transfected with either supercoiled or linearizedplasmid DNA and maintained at 37°C under G418 selection until3 days postinfection. Under these conditions, recombination betweenhomologous sequences on the plasmid and viral genome should occur.Homologous recombination between the linearized plasmid and thegenome should replace the endogenous allele with the interruptedallele containing the neo^r cassette. If the I3 allele is essential, then acquisition ofNeo^r will come only from illegitimate, nonhomologous recombinationevents. When circular plasmid is used in the transfections, homologousrecombination with the genome will generate two tandem copiesof the I3 gene, one of which is intact and one of which is internallydeleted and contains the Neo^r gene. These intermediate viruses are then subjected to two roundsof plaque purification in the absence of G418. It has been shownpreviously that tandemly repeated sequences are unstable withinthe vaccinia virus genome; if the I3 gene is not essential, recombinationbetween the I3 alleles will lead to excision of the Neo^r gene with the concomitant retention of only a deleted I3 allele.When the final viral stocks were analyzed, isolates obtained fromall 16 independent infections/transfections retained the Neo^r gene and an intact I3 gene. These data provide compelling evidence(21, 35, 42) that the I3 gene product plays an essentialrole during the vaccinia virus infectious cycle.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Our study has identified an essential vaccinia virus gene which encodes a protein with virtually all of the characteristicsof replicative SSBs. These include abundant expression beforeand during DNA replication, localization to sites of viral DNAreplication, and sequence-nonspecific, high-affinity binding tossDNA. Our observation that I3 binds approximately 10 nt is alsocomparable to results obtained for several other SSBs (15, 17).The binding of I3 to ssDNA appears to lack significant cooperativity;the cooperativity of SSBs from different organisms has been reportedto differ substantially (17, 22). Low cooperativity may infact be an intrinsic feature of I3, but it is also possible thatour experimental conditions (for example, the lack of an appropriatecation or cofactor) are not optimized for cooperative bindingor that cooperativity requires an additional protein partner.

Although SSBs do not have a high degree of primary sequence similarity, there are common sequence motifs that have emergedfrom comparative analyses. A domain containing conserved aromaticand charged residues thought to mediate DNA binding is presentin many SSBs and appears to be present in the I3 protein as well(11, 34, 51) (Fig. 11A). Support for the importance of thisloosely defined motif has come from the direct demonstration thatfor several of these proteins, these aromatic residues are importantfor DNA binding. Interestingly, this motif is retained in theI3 homolog of molluscum contagiosum virus (MCV), a poxvirus whosegenomic sequence differs significantly from that of vaccinia virus(40, 41) (Fig. 11B). Overall, the identity of the MCV proteinto the vaccinia protein is only 39.1%, suggesting that those regionsthat are conserved are likely to be of functional importance inthe context of viral infection.

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FIG. 11. Conservation of sequence motifs within SSBs. (A) A common motif is found in diverse SSBs. Partial protein sequences from various SSBs were aligned with that portion of the gene 5 protein (fd bacteriophage) involved in DNA binding (modified from references 11, 34, and 51). This analysis yielded a region in all of the sequences which consists of conserved aromatic and basic amino acids (indicated by single-letter abbreviations) separated by variable numbers of unrelated residues. These spacer regions are designated by X, with a subscript indicating the number of residues in each case. The proteins shown are the I3 protein (39) of vaccinia virus strain WR (VV), gene 5 protein of bacteriophage fd (GP5), gene 32 protein of bacteriophage T4 (GP32), SSB of E. coli (SSB), and DNA binding proteins from bacteriophage ike (PIKE), herpes simplex virus type 1 (HSV-1), varicella-zoster virus (VZV), Epstein-Barr virus (EBV), and adenovirus type 5 (AD-5). Numbers indicate the residue numbers for each sequence shown in the alignment. (B) Sequence comparison of the vaccinia virus I3 protein and the homolog encoded by MCV. The sequence of the I3 protein encoded by the WR strain of vaccinia virus protein was aligned with the sequence of the MCV homolog (ORF MC046L, accession no. U60315). Residues common to both proteins are shaded and boxed; circles are above the residues corresponding to the motif shown in panel A.

We have also shown that the I3 protein is phosphorylated on a serine residue(s). This property suggests that I3 is distinctfrom the phosphoprotein described earlier in the literature asa possible SSB (polypeptide B or FP11), which was shown to bephosphorylated on threonine residues. I3 also shows a far strongerand more specific affinity for ssDNA than was described for thisprotein, which is instead more likely to be the recently describedproduct of the H5 gene (1), a 25-kDa protein which migratesanomolously in SDS-PAGE with an apparent MW of 35,000 (1, 10,18, 38e)).

Our investigation of the elution profiles of ³⁵S- or ³²P-labeled extracts from ssDNA-cellulose revealed a single binding modefor phosphorylated and total I3, suggesting that phosphorylationdoes not alter the ssDNA binding properties on the protein underthese conditions. This interpretation, of course, rests on theassumption that both phosphorylated and unphosphorylated I3 arepresent intracellularly. In support of our conclusion, we alsosee no appreciable difference in the DNA binding properties ofendogenous I3 and recombinant I3 purified from E. coli. Nevertheless,Davis and Mathews previously reported that antibromodeoxyuridineantibody coprecipitated ³⁵S-labeled but not ³²P-labeled I3 (4). Our data suggest that their observationsmay reflect technical considerations (such as differences in thelevels of the phosphorylated and unphosphorylated species) ormay indicate that phosphorylation of I3 does modulate its interactionwith DNA in vivo. We would propose that this modulation is indirect,perhaps by regulating I3's interactions with other proteins, ratherthan through a direct effect on its inherent DNA binding properties.

The role of I3's phosphorylation, therefore, warrants further study, especially since several eukaryotic SSBs are known tobe phosphorylated (15, 52). The 34-kDa middle subunit of hRPAis phosphorylated in a cell cycle-specific manner, suggestingthat hRPA-mediated events, including DNA replication, may be regulatedthrough modulation of hRPA activity. The major SSB of adenovirus,DBP, is phosphorylated on several serine and threonine residuesin its N-terminal domain, which is not its DNA binding domain.The significance of this phosphorylation is also unknown. Studiesfrom our laboratory suggest that recombinant I3 cannot be phosphorylatedin vitro by either purified B1 kinase (35, 38a) or F10 kinase(38b, 47). In addition, the phosphorylation of I3 is not compromisedin vivo during nonpermissive infections performed with mutantscarrying lesions in the B1 (ts2 or ts25) (35, 36, 38c) orF10 (ts28) (38d, 47, 50) kinase. It appears, therefore, thatI3 is phosphorylated by cellular kinases. If phosphorylation ofI3 is meaningful and not fortuitous, we suggest again that themost obvious hypothesis is that phosphorylation mediates protein-proteininteractions central to I3's role(s) in vivo.

Our characterization of I3's DNA binding properties prompted us to test whether purified recombinant I3 could substitute forE. coli SSB in permitting recombinant vaccinia virus DNA polymeraseto replicate a singly primed M13 template in vitro (24). Itcould not; moreover, addition of I3 to reactions containing E.coli SSB inhibited RFII formation in a dose-dependent manner (notshown). As more I3 was added, the length of the products formeddecreased in a uniform manner, suggesting that I3 was slowingthe apparent rate of polymerase elongation. These data could beexplained by the presence of an inhibitor of the polymerase inour preparations; the observation that some, but not all, methodsof purifying the herpes simplex virus-encoded SSB gave resultssimilar to ours provides a precedent for this interpretation (13,31). Alternatively, our data might suggest that the functionof I3 as an SSB relies on appropriate phosphorylation and/or oninteractions with molecules other than the catalytic DNA polymerase.Candidates for such partners could include an additional componentof an SSB multimer, a processivity factor, or a replicative helicase.Moreover, the earlier studies of Davis and Matthews indicatedthat an anti-idiotypic antibody raised against the ribonucleotidereductase bound to the I3 protein; this finding, as well as theirsupporting data, suggests strongly that I3 could interact withthe nucleotide synthetic machinery at the replication fork (4).By analogy to the cellular RPA, which interacts with componentsof the repair machinery as well as the replication machinery (12,20, 28), I3 might also associate with such viral enzymes asthe UDG. Identification of such a complex might clarify the surprisingobservation that the vaccinia virus UDG is essential for DNA replication(5, 26, 44). Davis and Mathews noted that both I3 and theSSB of bacteriophage of T4 (gene 32 protein) have a highly acidicC terminus (4). This region of the gene 32 protein has beenshown to mediate interactions with other proteins. Assessing theimpact of mutations within this and other regions of I3 on theviral life cycle, as well as pursuing biochemical and geneticstrategies aimed at identifying I3-interacting proteins, shouldprovide insight into the regulation of viral DNA metabolism.

	ACKNOWLEDGMENTS

We thank B. Peabody for technical support and Lori Van Houten for invaluable help with the photography. We also thank NancyKlemperer, Ke Liu, Bill McDonald, and Joel Pardee for many helpfuldiscussions.

This work was supported by a grant to P.T. from the NIH (AI 21758) and by a generous group of donors from the Dorothy RodbellCohen Foundation.

	FOOTNOTES

^* Corresponding author. Present address: Department of Microbiology and Molecular Genetics, Medical College of Wisconsin, 8701Watertown Plank Rd., Milwaukee, WI 53226. Phone: (414) 456-8253.Fax: (414) 456-6535. E-mail: ptrakt{at}mcw.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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33. Polisky, B., and J. Kates. 1975. Viral-specific polypeptides associated with newly replicated vaccinia DNA. Virology 66:128-139[Medline].

34. Prasad, B. V. V., and W. Chiu. 1987. Sequence comparison of single-stranded DNA binding proteins and its structural implications. J. Mol. Biol. 193:579-584[Medline].

35. Rempel, R., and P. Traktman. 1992. Vaccinia virus B1 kinase: phenotypic analysis of temperature-sensitive mutants and enzymatic characterization of recombinant proteins. J. Virol. 66:4413-4426[Abstract/Free Full Text].

36. Rempel, R. E., M. K. Anderson, E. Evans, and P. Traktman. 1990. Temperature-sensitive vaccinia virus mutants identify a gene with an essential role in viral replication. J. Virol. 64:574-583[Abstract/Free Full Text].

37. Ricciardi, R. P., J. S. Miller, and B. E. Roberts. 1979. Purification and mapping of specific mRNAs by hybridization-selection and cell-free translation. Proc. Natl. Acad. Sci. USA 76:4927-4931[Abstract/Free Full Text].

38. Rigby, P. W. J., M. Dieckmann, C. Rhodes, and P. Berg. 1977. Labeling deoxyribonucleic acid to high specific activity in vitro by nick translation with DNA polymerase I. J. Mol. Biol. 113:237-251[Medline].

38a. Rochester, C. R., and U. Sankar. Unpublished data.

38b. Rochester, C. R., and S. Jesty. Unpublished data.

38c. Sankar, U. Personal communication.

38d. Sankar, U., and P. Traktman. Unpublished data.

38e. Sankar, U., M. Derrien, and P. Traktman. Unpublished data.

39. Schmitt, J. F. C., and H. G. Stunnenberg. 1988. Sequence and transcriptional analysis of the vaccinia virus HindIII I fragment. J. Virol. 62:1889-1897[Abstract/Free Full Text].

40. Senkevich, T. G., J. J. Bugert, J. R. Sisler, E. V. Koonin, G. Darai, and B. Moss. 1996. Genome sequence of a human tumorigenic poxvirus: Prediction of specific host responses $---$ evasion genes. Science 273:813-816[Abstract].

41. Senkevich, T. G., E. V. Koonin, J. J. Bugert, G. Darai, and B. Moss. 1997. The genome of molluscum contagiosum virus: analysis and comparison with other poxviruses. Virology 233:19-42[Medline].

42. Shuman, S., M. Golder, and B. Moss. 1989. Insertional mutagenesis of the vaccinia virus gene encoding a type I topoisomerase: evidence that the gene is essential for virus growth. Virology 170:302-306

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38b.	Rochester, C. R., and S. Jesty. Unpublished data.
38c.	Sankar, U. Personal communication.
38d.	Sankar, U., and P. Traktman. Unpublished data.
38e.	Sankar, U., M. Derrien, and P. Traktman. Unpublished data.
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41.	Senkevich, T. G., E. V. Koonin, J. J. Bugert, G. Darai, and B. Moss. 1997. The genome of molluscum contagiosum virus: analysis and comparison with other poxviruses. Virology 233:19-42[Medline].
42.	Shuman, S., M. Golder, and B. Moss. 1989. Insertional mutagenesis of the vaccinia virus gene encoding a type I topoisomerase: evidence that the gene is essential for virus growth. Virology 170:302-306