Persistence and Expression of the Herpes Simplex Virus Genome in the Absence of Immediate-Early Proteins

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J Virol, April 1998, p. 3307-3320, Vol. 72, No. 4
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Persistence and Expression of the Herpes Simplex Virus Genome in the Absence of Immediate-Early Proteins

Lorna A. Samaniego, Lisa Neiderhiser, and Neal A. DeLuca^*

Department of Molecular Genetics and Biochemistry, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania 15261

Received 21 November 1997/Accepted 7 January 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The immediate-early (IE) proteins of herpes simplex virus (HSV) function on input genomes and affect many aspects of hostcell metabolism to ensure the efficient expression and regulationof the remainder of the genome and, subsequently, the productionof progeny virions. Due to the many and varied effects of IE proteinson host cell metabolism, their expression is not conducive tonormal cell function and viability. This presents a major impedimentto the use of HSV as a vector system. In this study, we describea series of ICP4 mutants that are defective in different subsetsof the remaining IE genes. One mutant, d109, does not expressany of the IE proteins and carries a green fluorescent protein(GFP) transgene under the control of the human cytomegalovirusIE promoter (HCMVIEp). d109 was nontoxic to Vero and human embryoniclung (HEL) cells at all multiplicities of infection tested andwas capable of establishing persistent infections in both of thesecell types. Paradoxically, the genetic manipulations that wererequired to eliminate toxicity and allow the genome to persistin cells for long periods of time also dramatically lowered thelevel of transgene expression. Efficient expression of the HCMVIEp-GFPtransgene in the absence of ICP4 was dependent on the ICP0 protein.In d109-infected cells, the level of transgene expression wasvery low in most cells but abundant in a small subpopulation ofcells. However, expression of the transgene could be induced incells containing quiescent d109 genomes weeks after the initialinfection, demonstrating the functionality of the persisting genomes.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The temporal regulation of herpes simplex virus type 1 (HSV-1) gene expression during permissive infection commences withthe induction of the immediate-early (IE) genes by the virionprotein VP16 (3, 8). VP16 activates transcription by binding,along with the cellular factors Oct1 and host cell factor (HCF),to the TAATGARAT elements present in all IE promoters (56, 57,80, 113, 116a). The virus encodes five IE proteins, designatedinfected cell polypeptides (ICP) 0, 4, 22, 27, and 47 (13, 43,84). With the exception of ICP47, these IE proteins are knownto have regulatory functions demonstrated to affect the coordinatedexpression of the HSV genome. ICP4 and ICP27 are absolutely essentialfor virus replication (18, 24, 71, 87, 96, 115), whilethe growth of ICP0 mutants is significantly impaired (97, 110).These three IE proteins have the most profound effects on subsequentviral gene expression.

ICP4 is the major regulatory protein of the virus, and it is necessary for the transition of viral gene transcription fromthe IE to the E phase (24, 87, 115). It functions as a repressor(19, 38, 76, 82) or activator (19, 27, 33, 81,90) of transcription by forming multiple contacts with basaltranscription factors (9, 37, 38, 105).

ICP0 is a potent transactivator of viral and cellular promoters in transient assays (27, 33, 81, 90), and it providesfor efficient viral gene expression and growth, in vitro and invivo (5, 7, 62). ICP0 enhances gene expression, in partby increasing the transcription rates of viral genes (50, 99),although the exact mechanism by which ICP0 accomplishes this isnot yet clear. These functions most likely underlie the requirementfor ICP0 in lytic viral growth and the efficient reactivationof the virus from latent infections as shown in the mouse andrabbit models (5, 14, 28, 35, 62, 95). ICP0 has alsobeen shown to interact with ND10 nuclear structures (29, 67)and components of the transcription (61), translation (51),cell cycle (52), and proteolytic (30) machinery of the cell.Therefore, it has the potential to affect many aspects of hostcell metabolism.

ICP27 regulates the processing of viral and cellular mRNAs (39, 73, 74, 102, 106). It may also act by modulating theactivities of ICP4 and ICP0 (75, 104), as well as the modificationstate of ICP4 (75, 92, 112). The combined activities of ICP27contribute to efficient late-gene expression (71, 96). Recentstudies have shown that ICP27 also significantly contributes toelevated levels of early-gene expression, explaining the requirementfor ICP27 in viral DNA synthesis (98, 114).

ICP22 and ICP47 can be deleted from the genome without greatly affecting viral growth and viability in most cell types (70,86, 103). ICP22 promotes efficient late-gene expression ina cell type-dependent manner (103). It has been reported to giverise to a novel phosphorylated form of RNA polymerase II (polII) (93) as well as to regulate the stability and splicing patternof the ICP0 mRNA (10). Its regulatory effects may thus be mediatedthrough these activities. The function of ICP47 may be more relevantin vivo, where it may help the virus escape immune surveillanceon the basis of its ability to block the presentation of antigenicpeptides to CD8⁺ cells (118).

In ICP4 mutant backgrounds, expression of viral early and late genes is dramatically reduced. This has led to the considerationof such backgrounds as starting points for the construction ofgene transfer vehicles. However, despite the limited expressionof the HSV genome in ICP4 mutant backgrounds, such mutants arevery toxic to cells. This is most likely because of the overexpressionof the remaining IE proteins in the absence of ICP4. Several ofthe IE genes reduce the transformation of cells when cotransfectedwith a selectable marker, implying that the protein products ofthe transfected IE genes are not conducive to cell survival (48).Given this observation, and the findings of numerous groups onthe effects of IE proteins on different aspects of host cell metabolism,it seems reasonable that the elimination of IE protein activityis essential for the efficient and safe use of HSV as a gene transfervehicle. Lending support to this hypothesis are the observationsthat elimination of the VP16 activation function in an ICP4 mutantbackground (48, 88) and the deletion of subsets of IE genes(99, 117) reduce toxicity. Both ICP0 and ICP22 contribute totoxicity, as demonstrated by the improved survival of infectedcells when these activities were individually abrogated in thebackground of viruses already deleted for ICP4 and ICP27 (99,117). However, both of these triple mutants remained toxic athigh multiplicities of infection (MOI). For one of these studies,we hypothesized that the elimination of ICP22 activity from theICP4 ICP27 ICP0 background would further reduce toxicity.

Another point of consideration with viral vectors is the degree of transgene expression. The IE proteins of HSV have multipleand varied effects on the expression of viral genes, mostly, butnot entirely, acting to increase gene expression. Similar effectsare to be expected for transgenes inserted into the viral genome.Therefore, the elimination of viral IE genes may be expected todecrease toxicity but also might significantly reduce transgeneexpression. In support of this hypothesis, elimination of VP16,ICP4, and ICP0 activity reduced cytotoxicity but also reducedgene expression (88, 89). The same observation was made instudies of an ICP4 ICP27 ICP0 mutant (99). In the latter study it was concluded that ICP0could significantly increase the transcription rates of genesin the absence of ICP4 and ICP27. The genes of HSV are standardpol II transcription units (15). Therefore, heterologous polII promoters used to express transgenes may be affected by HSVIE genes in the same way as HSV promoters are affected.

In the current study, we set out to further assess the toxicity of different IE mutant backgrounds and examine the level ofgene expression as a consequence of reduced toxicity and eliminationof viral trans-acting factors. In all the mutants that are deletedfor ICP4 and ICP27, an expression cassette containing the greenfluorescent protein (GFP) reporter gene under the control of thehuman cytomegalovirus (HCMV) IE promoter-enhancer was insertedinto the ICP27 deletion locus as a model transgene. The followingpoints were addressed, with the stated general outcomes.

(i) Vector toxicity. Both ICP0 and ICP22 contribute to the toxicity of a virus deleted for ICP4 and ICP27. Elimination of these functions in additionto ICP47 resulted in a virus that was by several criteria nontoxicto Vero and human embryonic lung (HEL) cells at high MOI.

(ii) Genome persistence. The genome of the virus (d109) that did not express any IE proteins was capable of long-term persistence in both HEL and Verocells.

(iii) Gene expression. The abundant expression of the HCMVIEp-GFP transgene was dependent on the ICP0 protein. In the absence of ICP0, the levelof transgene expression was very low in most cells but abundantin a subpopulation of cells. Expression of the transgene couldalso be induced weeks after infection in cells containing persistentd109 genomes.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Cells and viruses. Vero cells and the complementing cell lines E5 (ICP4⁺) (20), E26 (ICP4⁺ ICP27⁺) (98), L7 (ICP0⁺) (99), and FO6 (ICP4⁺ ICP27⁺ ICP0⁺) (99) were maintained by standard cell culture procedures aspreviously described (17, 24). Tissue culture medium for maintainingL7 cells was supplemented with 400 µg of G418 (GIBCO-BRL)/ml.For maintaining FO6 cells, the medium was supplemented with 400µg of G418 and 300 µg of hygromycin B (Boehringer Mannheim)/ml.Viruses carrying single or multiple IE mutations were propagatedand subjected to titer determination on the appropriate cell lines.The viruses d92 (ICP4 ICP27), d96 (ICP4 ICP22), and d95 (ICP4 ICP27 ICP22) were described previously (98, 117). The viruses with mutationsin capsid genes, including K23Z (22), K5 $Delta$ Z (22), KUL26 $Delta$ Z (23),and K $Delta$ 19C (85), were generously provided by Stanley Person (JohnsHopkins University, Baltimore, Md.). In experiments that compared107, d106, d104, and d109, the infectivities of the virus stockswere normalized on the basis of the number of genomes in infectednuclei at 6 h postinfection (p.i.) as determined by PCR amplification.

Plasmid constructions. The plasmid pEB $Delta$ AE contains the EcoRI-B genomic fragment with deleted copies of ICP4 (d120) (18) and ICP0 (0 $Delta$ ) and a wild-type(wt) copy of ICP27. The boundaries of the deletion in the ICP0gene are defined by the BsmI site at nucleotide (nt) 120142 andthe AseI site at nt 124775. pEB $Delta$ AE was constructed by insertingthe 2.7-kb XbaI fragment isolated from pAE into the unique XbaIsite of pEB. Both pEB and pAE derived their cloned HSV sequencesfrom pdlEB, which contains the EcoRI-B genomic fragment isolatedfrom the virus mutant d120 ligated into the unique EcoRI siteof pBR325 (21). To construct pEB, pdlEB was cleaved with BsmIand the ends of the resulting fragments were modified by ligationof adapter oligonucleotides (5'-CGTCTAGACGCG-3') to convert theBsmI sites to XbaI sites. This pool of fragments was digestedsimultaneously with EcoRI and XbaI and then fractionated in a0.8% agarose gel to isolate the 10-kb EcoRI-XbaI fragment. Afterbeing isolated by electroelution, this 10-kb fragment was clonedinto the corresponding sites of puc19 to generate pEB. To constructpAE, pdlEB was cleaved simultaneously with AseI and EcoRI. Afterthe ends of the resulting fragments were filled in with DNA polymeraseI Klenow fragment, they were modified with XbaI linkers. Fromthis pool of fragments, a 2.7-kb XbaI fragment was isolated byelectroelution and ligated into the XbaI site of puc19 to producepAE.

In plasmid pGFP27, the GFP gene, under the control of the HCMV IE promoter (HCMVIEp), is substituted between the BamHI andSalI sites in the ICP27 locus. pGFP27 was constructed by insertionof the 1.6-kb HCMVIEp-GFP cassette into the unique PacI site ofpAT2. The insert corresponded to an AseI-MluI fragment derivedfrom pGFPX whose ends were modified with PacI linkers. pGFPX wasderived from pEGFP-C1 (Clontech) by deletion of the multiple cloningsites between the BamHI and BglII restriction enzyme sites. pAT2resulted from the conversion of the unique XbaI site in pAT1 intoa PacI site. Both pAT2 and pAT1 contain the EcoRI-to-SalI (nt110095 to 120902) HSV sequence with the 1.2-kb deletion betweenthe BamHI and SalI sites in the ICP27 locus. At the site of theICP27 deletion is a unique XbaI site in pAT1. Construction ofpAT1 was done by cloning the 3.2-kb EcoRI-BamHI fragment isolatedfrom pKEB-S1 (4) into the corresponding site in pucSF. Theplasmid pucSF contains the 6.4-kb SalI fragment derived from pKSF(4) inserted into the corresponding site in puc19.

The plasmid pTGT $Delta$ contains the joint fragment of the HSV genome (P isotype) extending from the AseI site (nt 124775) 5' ofICP0 to the proximal BamHI site (nt 136289) 3' of ICP22, withthe d120 mutation and the 270-bp TGT $Delta$ deletion in the ICP22 promoterlocated in the c' repeat sequence. The TGT $Delta$ mutation removes theTAATGARAT elements in the ICP22 promoter and is defined by theEcoRI and BssHII restriction enzyme sites. pTGT $Delta$ was generatedby insertion of the 2.7-kb XbaI fragment isolated from pAE intothe unique XbaI site of pucBN $Delta$ XB. To construct pucBN $Delta$ XB, pucBN(99) was digested with XbaI and BssHII. The large vector fragmentisolated from this digest was then ligated in the presence ofthe oligonucleotide adapters 5'-CGCGCTTAATTAAT-3' and 5'-CTAGATTAATTAAG-3'to allow joining of the XbaI- and BssHII-restricted ends. Bothof these restriction enzyme recognition sites remained intactin the resulting plasmid, pucBN $Delta$ XB, and the oligonucleotide adaptersalso introduced a PacI site.

The pucGFP plasmid used as the source for the GFP fragment probe carries the 1.6-kb PacI fragment derived from pGFP27 andinserted into the unique PacI site of pNEB193 (New England Biolabs).The orientation of the insert is such that a HindIII-NheI doubledigestion results in a 1-kb fragment containing the GFP codingsequence.

Virus constructions. The DNA-calcium phosphate precipitates used for transfections were prepared essentially as described by Graham and van derEb (36). A typical mixture used to transfect approximately 10⁶ cells plated in two 60-mm-diameter dishes contained 3 µg of viralDNA, 1 to 3 µg of the linearized plasmid carrying the mutant IEalleles, 1 µg of the plasmid pW3 $Delta$ HS8 (20), and 1 µg of pGreenLantern-1 (GIBCO-BRL). pW3 $Delta$ HS8 provides ICP0, which improves thetransfection efficiency of recombinant virus mutants deficientin this gene product. The plasmid pGreen Lantern-1 was added toallow convenient monitoring of transfection efficiency. It wasnot added for the construction of d104. Generation of mutantsby crossing two viruses was done by coinfecting cells with approximately5 PFU of each parent virus per cell.

Southern blot analysis. DNA, isolated from the IE mutant viruses as previously described (98), was cleaved with HpaI to detect the GFP substitutionin ICP27, with PstI and SacI to detect the 0 $Delta$ deletion in ICP0,with BamHI and SacI to detect the d120 mutation in ICP4 (18),and with NcoI to detect the TGT $Delta$ mutation in the ICP22 and ICP47promoters. Digested viral DNA was fractionated by agarose gelelectrophoresis, transferred to nitrocellulose, and hybridizedto nick-translated probes as previously described (100, 107).Gel-purified DNA fragments that were nick translated and usedas probes included the 2.4-kb BamHI-SacI fragment derived frompKHX-BH (4) for detecting ICP27, the 1.3-kb PstI fragment frompEB for detecting ICP0, the 1.8-kb BamHI-Y fragment from pKBY(98) for detecting ICP4, and the 1.6-kb PvuII fragment frompucBN $Delta$ XB for detecting the TGT $Delta$ mutation.

Isolation of infected-cell RNA and Northern blot analysis. Total infected-cell RNA was prepared as previously described (98). For infections performed in the presence of cycloheximide(CHX), the medium was supplemented with the inhibitor (100 µg/ml)1 h prior to and during infection. Fractionation of the RNA samplesin 1.3% agarose-formaldehyde gels and the conditions for blotting,hybridization, and washing have also been previously described(45). Gel-purified DNA fragments that were nick translated andused as probes included the 2-kb HindIII fragment from pucBN (99)for detecting the ICP22 mRNA, the 2.4-kb BamHI-SacI fragment frompKHX-BH (4) for detecting ICP27, and the 1-kb NheI-HindIIIfragment from pucGFP for detecting GFP.

Analysis of viral proteins. Viral polypeptides were radiolabeled by incubating approximately 6 × 10⁵ cells infected at the indicated MOI with 100 µCi of [³⁵S]methionine per ml of medium at 6 to 9 h p.i. The CHX-treatedcells were incubated in the presence of the inhibitor (100 µg/ml)for 1 h prior to infection until 6 h p.i. The treated monolayerswere then washed twice with Tris-buffered saline and further incubatedfor 3 h in the presence of actinomycin D (10 µg/ml) and [³⁵S]methionine (100 µCi per plate). The labeled viral proteins weresolubilized in sodium dodecyl sulfate (SDS) sample solution andseparated by SDS-polyacrylamide gel electrophoresis (SDS-PAGE)as previously described (60, 66). For Western blot analysisof GFP, proteins separated by SDS-PAGE were electroblotted tonitrocellulose and analyzed using an anti-GFP ( $alpha$ -GFP) monoclonalantibody (Clontech) diluted 1:500 and a chemiluminiscence Westernblotting kit (Boehringer Mannheim).

Colony formation inhibition assays. Inhibition of colony formation by the different viral mutants was assayed as previously described (117). Briefly, Vero cellsinfected at different MOI and control uninfected monolayers weretrypsinized at 6 h p.i. to prepare single-cell suspensions thatwere then serially diluted and plated in medium supplemented with20% fetal bovine serum. Ten to 14 days after plating, the colonieswere stained with crystal violet and counted.

PCR analysis. For normalizing virus stocks, 2 × 10⁶ cells plated in 60-mm-diameter dishes were infected at an MOI of 10 based on titers determinedby plaque assay. At 6 h p.i., the cultured cells were washed withcold Tris-buffered saline and scraped from the plates. The cellswere pelleted by low-speed centrifugation and resuspended in 0.5ml of RSB buffer (10 mM NaCl, 10 mM Tris-HCl [pH 7.4], 3 mM MgCl₂).Nonidet P-40 (1%, 0.5 ml in RSB) was then added, and the mixturewas vigorously vortexed. The infected nuclei were pelleted, resuspendedin lysis buffer (1.2% Nonidet P-40 and 0.4 mg of proteinase Kper ml, prepared in Tris-EDTA buffer) and incubated overnightat 45°C. The mixtures were then heated at 95°C to inactivate theproteinase. Aliquots (2.5 µl) of these nuclear lysates were usedin PCRs. For determining the number of genomes in persistentlyinfected cells, total cell DNA was prepared from the infectedcells as previously described (98) and equivalent aliquots fromall the samples were used in PCRs.

The PCR conditions, with minor modifications, and the primers used to amplify glycoprotein C (gC) sequences were describedpreviously (55). A typical PCR mixture made up to 100 µl contained10 mM Tris-HCl (pH 8.3), 50 mM KCl, 10% glycerol, 3 mM MgCl₂,0.2 mM each deoxynucleoside triphosphate, 50 pmol of each upstreamand downstream primer (gC-1, 5'-GGGTCCGTCCCCCCCAAT-3'; gC-2, 5'-CGTTAGGTTGGGGGCGCT-3')(55), 2.5 U of Taq DNA polymerase (Boehringer Mannheim), andthe sample or standard DNA. Amplifications were done with a Perkin-ElmerGeneAmp PCR System 2400 with an initial denaturation step (94°C,5 min) followed by 25 cycles of denaturation (94°C, 30 s), annealing(60°C, 30 s), and extension (72°C, 30 s) and a final extensionstep (72°C, 7 min). For detection of the 109-bp gC PCR product,equal aliquots of each reaction mixture were run on a 1% agarose-1%NuSieve GTG (FMC BioProducts) gel. The gel was treated with 0.4N NaOH for 30 min and blotted on a GeneScreen Plus membrane (NENLife Science Products) in 0.4 N NaOH. After being subjected toUV cross-linking for 30 s (UV Stratalinker 2400; Stratagene),the membrane was prehybridized (6× SSC [1× SSC is 0.15 M NaClplus 0.015 M sodium citrate], 1% SDS, 5× Denhardt's solution,8 µg of salmon sperm DNA per ml) at 50°C for 1 h and hybridized(6× SSC, 1% SDS, 10⁵ to 10⁶ cpm/ml probe) at 50°C for 1 h. The end-labeled oligonucleotideprobe (gC-3, 5'-TAGAGGAGGTCCTGACGAACA-3') (55) was used at aconcentration of approximately 10 ng/ml of hybridization solution.After hybridization, the blots were washed (6× SSC, 0.001% SDS)with several changes of buffer, rinsed with 2× SSC, allowed todry, and exposed to film for autoradiography. The radioactivesignals were quantitated with an AMBIS 4000 radioanalytic imagingsystem (AMBIS, Inc., San Diego, Calif.).

Immunofluorescence. Infected and uninfected cells were prepared on circular coverslips. For detection of promyelocytic leukemia antigen (PML),cells were fixed with methanol as previously described (117).For simultaneous detection of ICP0 or ICP4 with GFP, the infectedcells were fixed with paraformaldehyde as previously described(40). Briefly, the cells were washed with phosphate-bufferedsaline (PBS), incubated in 4% paraformaldehyde solution for 10min, and then rinsed with PBS. Following paraformaldehyde fixation,the cells were permeabilized with 0.2% Triton X-100 for 2 minand then rinsed twice with PBS. Staining of the cells for PML,ICP0, or ICP4 was done as previously described (117). The monoclonalantibodies against PML (Santa Cruz Biotechnology, Santa Cruz,Calif.), ICP0, and ICP4 (no. 1112 and no. 1011, respectively;Goodwin Institute for Cancer Research, Inc., Plantation, Fla.)were used at dilutions of 1:30, 1:1,000, and 1:1,000, respectively.The stained antigens were visualized at a magnification of ×100(PML) or ×60 (ICP0 and ICP4) with the appropriate cubes for fluorescentimaging in conjunction with a Nikon FXA photomicroscope.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

We have previously described mutants inactivated for ICP22 or ICP0 in an ICP4 ICP27 background (99, 117). Cells infected with d95 (ICP4 ICP27 ICP22) exhibited prolonged cell survival and high-level expressionof ICP0 as well as some early genes (117). Although d95-infectedcell monolayers maintained their normal morphology for an extendedperiod of time, the cells stopped dividing and eventually died.Gene expression from the genome was severely restricted upon inactivationof ICP0 in the same ICP4 ICP27 background. In this virus, d97 (ICP4 ICP27 ICP0), the level of expression of an inserted lacZ transgene underthe control of the ICP0 promoter was initially high but declinedsoon thereafter to low levels that could still be detected upto 2 weeks p.i. The survival of d97-infected cells was improvedrelative to that of d92- or d95-infected cells, although the viruswas still toxic to cells at high MOI. The characteristics of bothd95 and d97 demonstrate the contributions of ICP0 and ICP22 tovirus toxicity. The studies detailed herein examine genome persistence,vector toxicity, and transgene expression in the absence of IEprotein functions.

Generation of mutants inactivated for multiple IE genes. Construction of the virus d109 (ICP4 ICP27 ICP0 ICP22 ICP47) proceeded in a series of steps that generated and utilized aset of mutants defective in sets of IE genes. All mutants deficientin ICP4 carried the d120 allele of the gene. ICP0 was inactivatedby a substantial deletion (0 $Delta$ ) that removed the entire codingregion along with the promoter (Fig. 1C). The sequences deletedin ICP27 are the same as those deleted in the 5dl1.2 allele (71)of the gene. In place of the deletion in ICP27, an HCMVIEp-GFPtransgene cassette containing the GFP gene under the control ofthe HCMV IE promoter was inserted (Fig. 1B).

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FIG. 1. Structures of isogenic mutants defective in combinations of IE genes. (A) The viral genome is represented with the unique long (U_L) and short (U_S) regions bounded by terminal and internal repeats (white boxes). The genomic locations and directions of transcription of the IE genes are indicated (arrowheads). (B) The TAATGARAT deletion, TGT $Delta$ (bracketed), introduced into the promoter regions of ICP22/47. The positions of the TAATGARAT elements (open arrows), binding sites for the transcription factor SP1 (arrowheads), TATA boxes (open squares), and oriS (open circle) are shown relative to the transcription start sites of ICP4 and ICP22/47. (C) Expanded map of the right end of the d109 genome, showing the coding sequences of the IE genes (solid arrows) and the deletion mutations (white bars) in ICP4 (d120), ICP0 (0 $Delta$ ), and the ICP22/47 promoter (TGT $Delta$ ). The transgene cassette containing the GFP reporter gene under the control of the HCMV IE promoter substituted into the deletion in ICP27 is represented by a shaded bar, with the arrow inside indicating the direction of transcription. The relevant restriction sites are indicated and are a bbreviated as follows: H, HpaI; P, PstI; S, SacI; B, BamHI; and N, NcoI. The line of asterisks represent the nick-translated DNA fragments used as probes for Southern blot analysis. (D) Structures of the isogenic mutants. The deletion mutations in ICP4, ICP0, and the ICP22/47 promoter present in the different virus mutant strains are indicated by the shaded bars inside the white boxes representing the repeat sequences. The GFP substitution in ICP27 is also shown (inverted triangles). The mutant designations are indicated on the right along with a list of the IE proteins not synthesized by the viruses in the absence of complementation. Viral DNA isolated from cells infected with the indicated viruses were digested with HpaI (E), PstI-SacI (F), BamHI-SacI (G), or NcoI (H) and analyzed by Southern hybridization. The probes used are shown in panel C and described in Materials and Methods.

To inactivate ICP22, a 270-bp sequence containing the TAATGARAT elements was deleted from its promoter (Fig. 1C). Since thispromoter is the same as that upstream of the ICP47 gene, the mutation(TGT $Delta$ ) affects expression of both ICP22 and ICP47. The mutatedpromoter, which retains the TATA box and several Sp1 sites, closelyresembles some of the early and late promoters activated by ICP4.It was assumed that removal of the TAATGARAT elements would eliminatethe responsiveness of the promoter to induction by VP16 but perhapsnot to activation by ICP4. The TGT $Delta$ mutation was intended to abrogateICP22 and ICP47 expression under the noncomplementing conditionsin which these experiments are conducted but also to allow expressionof functional ICP22 under the complementing conditions used toisolate and grow the mutants. The latter takes into account theapparent growth advantage that ICP22 provides to multiple IE mutants.

The virus d100 (Fig. 1D) was generated by cotransfecting E26 cells with d92 viral DNA and pEB $Delta$ AE linearized by HindIII. Thed92 virus carries the d120 (ICP4) and 5dl1.2 (ICP27) mutant alleles.The plasmid pEB $Delta$ AE contains a genomic fragment that carries thed120 (ICP4) and 0 $Delta$ (ICP0) mutations as well as a wt copy of ICP27.Progeny from the cotransfection were plated on FO6 cells, andindividual plaques were initially screened by Southern blot analysisfor incorporation of the $Delta$ 0 allele. Plaque isolates whose ICP0loci were both converted to the 0 $Delta$ allele were further analyzedto determine the state of the ICP27 gene. None of the isolatesretained the deletion in ICP27. One isolate carrying the intendeddeletions in both loci of ICP4 and ICP0 was further purified anddesignated d100. The virus d99 (Fig. 1D) was derived by rescuingthe d120 mutation of d100 to produce a virus that carried onlythe 0 $Delta$ mutation.

To construct d104 (Fig. 1D), FO6 cells were cotransfected with pGFP27 cleaved with HindIII and d100 viral DNA. The plasmidpGFP27 contains the HCMVIEp-GFP transgene inserted in the ICP27locus. Viruses derived from the cotransfection were plated onFO6 cells, and well-isolated green fluorescent plaques were furtherpurified and analyzed by Southern blotting to confirm incorporationof the GFP insert into the ICP27 locus. The virus resulting fromthis construction, d104, has the d120 (ICP4) and 0 $Delta$ (ICP0) mutationsas well as the GFP substitution in ICP27.

To generate virus d103 (Fig. 1D), E5 cells were cotransfected with d96 viral DNA and EcoRI-cleaved pTGT $Delta$ . The d96 virus carriesthe d120 (ICP4) and n199 (ICP22) mutant alleles. The pTGT $Delta$ plasmidcontains a wt ICP22 gene, the d120 mutation, and the TGT $Delta$ deletionthat removes the TAATGARAT elements from the ICP22 promoter (Fig.1C). Progeny from the cotransfection were plated on E5 cells,and individual plaques were screened by Southern hybridizationfor both the incorporation of the TGT $Delta$ deletion and repair ofthe n199 nonsense mutation in ICP22. One isolate carrying thed120 mutation in ICP4, the TGT $Delta$ mutation in the ICP22 and ICP47promoters, and a wt copy of the ICP22 gene was propagated anddesignated d103.

Viruses d106 and d107 (Fig. 1D) were derived from a cross between d103 and d104. The virus d109 (Fig. 1D) was generated bycrossing d106 and d104. Isolated green fluorescent plaques resultingfrom these coinfections were analyzed by Southern blotting todetermine their genotypes. The mutant d107 carried the d120 deletionin ICP4 and the GFP substitution in ICP27. d106 carried both ofthese mutations in addition to the TGT $Delta$ deletion in the ICP22and ICP47 promoters. The isolate designated d109 carried the d120(ICP4), 0 $Delta$ (ICP0), and TGT $Delta$ (ICP22 and ICP47 promoters) deletionsas well as the GFP substitution in ICP27.

Figure 1E to H shows Southern blot analyses in which restriction digests of KOS, d107, d106, d104, and d109 were probed todemonstrate the structures of the IE genes in d109. Figure 1Bshows an expanded map of the right end of the genome, highlightingthe sequences used to probe the Southern blots (asterisks), thelocations of the coding sequences for the IE genes, relevant restrictionsites, and the mutant alleles. To visualize the ICP27 sequencesin the viruses, electrophoretically separated HpaI fragments ofthe viral DNA were probed with the indicated fragment. The substitutedHCMVIEp-GFP transgene provides an additional HpaI site (Fig. 1B),and as a consequence of this substitution in the ICP27 locus,all the mutant viruses contained the shortened HpaI fragment (Fig.1E). To visualize the ICP0 sequences in the viruses, separatedPstI-SacI fragments of viral DNA were probed with the indicatedfragments. The 4.6-kb deletion (0 $Delta$ ) in ICP0 present in d104 andd109 resulted in the shorter PstI-SacI fragment relative to thewt allele of the gene (Fig. 1F). To visualize the ICP4 sequencesin the viruses, fractionated BamHI-SacI fragments of viral DNAwere probed with the indicated fragments. All the mutant virusescarried the d120 allele, as indicated by the fusion of BamHI-Ysequences (corresponding to the probe fragment) to the BamHI-SacIfragment spanning the joint, by virtue of the deletion in ICP4(Fig. 1B). This 2.2-kb BamHI-SacI fragment spanning the jointis detected running slightly behind the 1.8-kb BamHI fragmentcharacteristic of the wt ICP4 allele (Fig. 1G). Variation in thenumber of copies of the a' repeat sequence in a given populationproduces the multiple bands observed above the 2.2-kb fragment.The smaller, 1.3-kb fragment detected by the probe correspondsto the S-terminal BamHI of d120. To demonstrate the presence ofthe TGT $Delta$ mutation in the ICP22 and ICP47 promoters of the differentviruses, electrophoretically separated NcoI fragments of viralDNA were probed with the indicated fragment. Incorporation ofthe TGT $Delta$ mutation in d106 and d109 is indicated by the loss ofan NcoI site located within the 270-bp deleted sequence (Fig.1B). As a consequence of this deletion in d106 and d109, two adjacentNcoI fragments are fused, resulting in larger NcoI fragments of4.6 and 2.8 kb encompassing ICP22 and ICP47, respectively (Fig.1H). The wt NcoI fragments containing ICP22 and ICP47 are 4.1and 2.3 kb in size, respectively, and these were not detectedin d106 and d109, demonstrating the presence of the TGT $Delta$ mutationin both copies of the c' repeat. Therefore, d109 contains thed120 (ICP4), 0 $Delta$ (ICP0), and TGT $Delta$ (ICP22 and ICP47 promoters) deletionsas well as the GFP substitution in ICP27.

The TGT $Delta$ mutation introduced into the ICP22 and ICP47 promoters was intended to restrict expression of these genes under noncomplementingconditions but also to allow for expression of functional ICP22under the complementing conditions used to isolate and grow themutants. Figure 2 shows the effect of the TGT $Delta$ deletion presentin d103 on the expression of ICP22. As a consequence of the TGT $Delta$ mutation, accumulation of the ICP22 mRNA in d103-infected Verocells was significantly reduced compared to that in d120- or d96-infectedcells (top left). The levels of the ICP27 mRNA in cells infectedin the presence of CHX indicate that the virus input used forthe d103 infections was in fact larger (bottom left), therebysuggesting that the actual level of ICP22 mRNA made in d103-infectedcells is lower than that observed. Moreover, the d103 mutant stillexpresses the other IE activator, ICP0. In the absence of ICP0,such as in the mutant d109, expression of ICP22 is expected tobe even further reduced. This prediction was borne out at thelevel of protein synthesis, as shown below. In the presence ofICP4 provided by the complementing cell line E5, ICP22 mRNA expressedby d103 accumulated to levels comparable to those in d120-infectedcells (Fig. 2, top right). These results indicate that the TGT $Delta$ mutation can effectively reduce expression of ICP22. In the absenceof the TAATGARAT elements, induction by VP16 does not occur andICP22 is no longer expressed as an IE gene. However, the mutatedICP22 promoter remains responsive to activation by ICP4, so thatunder complementing conditions in which ICP4 is present, the geneis expressed, perhaps with the same kinetics as an early gene.Consistent with this interpretation, the relative abundance ofthe ICP22 mRNA in d103-infected Vero and E5 cells is reminiscentof that of thymidine kinase in the two cell types (45). As predicted,expression of functional ICP22 under these conditions gives thevirus a growth advantage since d103 can be propagated to highertiters than can d96 (data not shown).

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FIG. 2. Effect of the TGT $Delta$ mutation on expression of ICP22. Total cell RNA, isolated at 6 h p.i. from Vero or E5 cells (ICP4⁺) infected (MOI = 10) with the indicated viruses, was processed for Northern blot analysis. For infections of Vero cells done in the presence of CHX, the medium was supplemented with the inhibitor 1 h prior to and during infection. The blots were hybridized to probes specific for ICP22 and ICP27 mRNAs as indicated (22 and 27, respectively). KOS is the wt virus control, and d96 (ICP4 ICP22) (117) carries the d120 $Delta$ deletion in ICP4 and the n199 nonsense mutation in ICP22 (93).

The viruses d106, d107, d104, and d109 carry mutations that should abrogate the expression of specific sets of IE proteins.To demonstrate that this is the case, a CHX reversal experiment(42) was performed on cells infected with the multiple IE mutants.This type of experiment predominantly limits viral gene expressionto that of the IE genes. The results of this experiment are shownin Fig. 3. In addition to the SDS-9% polyacrylamide gel routinelyused for these experiments (Fig. 3A), the same samples were alsorun on an 18% gel (Fig. 3B) to allow the detection of the smaller27-kDa GFP and 11-kDa ICP47 proteins. The mobility of GFP coincideswith that of a cellular protein. To verify the identity of theband corresponding to GFP, a Western blot analysis was also performed(Fig. 3C). As expected from the genotypes of these viruses, noneof the mutants expressed ICP4 or ICP27. ICP0 was not synthesizedin d104- or d109-infected cells. ICP22 and ICP47 were not synthesizedin d106- or d109-infected cells. Also, under conditions of CHXreversal, all four mutants synthesized GFP to similar levels.These results show that in infected Vero cells, d109 does notexpress ICP4, ICP27, ICP0, ICP22, or ICP47, and it synthesizesGFP in the absence of prior viral protein synthesis.

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FIG. 3. Synthesis of viral proteins in cells infected with d109. Vero cells were infected (MOI = 20) with the indicated viruses in the presence or absence of CHX, pulsed with [³⁵S]methionine at 6 to 9 h p.i., and processed for SDS-PAGE. The CHX-treated cultures were incubated in the presence of actinomycin D during labeling. The samples were run on 9% (A) and 18% (B) SDS-polyacrylamide gels (the latter to better visualize the smaller viral proteins). The positions of the IE proteins and GFP, as well as some early and late proteins, are indicated. (C) The same samples were also transferred to a membrane for Western blot analysis with an $alpha$ -GFP monoclonal antibody. Mock, uninfected cells.

Expression of the viral genome in the absence of IE proteins. In the absence of regulatory functions encoded by the IE proteins, viral gene expression from d109 was expected to be severelyrestricted and solely a function of cellular factors. The contributionof the virion component, VP16, in this case is irrelevant sincenone of the endogenous IE promoters remain intact. Figure 3 showsthe results of a parallel experiment conducted in the absenceof inhibitors (untreated). Under these conditions, the effectsof expressed IE proteins on subsequent gene expression can beobserved. A typical permissive pattern of viral protein synthesisfrom 6 to 9 h p.i. is seen in cells infected with the wt virusKOS. Except for d106, which synthesized abundant amounts of ICP0and ICP6, none of the mutants expressed the viral gene productsto a significant degree. The polypeptide profile of d109 was indistinguishablefrom that of uninfected cells, thus showing that little or noHSV protein is made in this background.

The GFP transgene was synthesized to abundant levels in d106- or d107-infected cells, in which ICP0 was present (Fig. 3C).In cells infected with a mutant that does not express ICP0 (d104or d109), the abundance of GFP was greatly reduced. These resultsclearly indicate that in the absence of ICP4, ICP0 can be a majordeterminant of gene expression driven from the HCMV IE promoter.Another notable observation is that the amount of GFP made inuntreated cells infected with d104 or d109 was very low comparedto that expressed in similarly infected CHX-treated cells. Prestonand Nicholl previously observed that the heterologous HCMV promoteris active in CHX-treated cells infected with the mutant in1332,which is defective for the viral activators VP16, ICP0, and ICP4(89). In the absence of the inhibitor, the activity of the HCMVpromoter in this background was reduced. These observations suggestthat an active mechanism represses the HCMV promoter in the absenceof viral activators. This inhibition may involve a cellular factorthat is transiently expressed and therefore not made in the presenceof CHX.

The greater reduction in the levels of cell and viral proteins seen in d104- or d107-infected cells suggests an increase inshutoff of protein synthesis and correlates with the presenceof ICP22 in these viruses. The vhs gene product (UL41) of HSVfunctions in attenuating host protein synthesis by destabilizingpreexisting host mRNAs (31, 91, 111) and ensures the rapidturnover of viral mRNAs after the onset of viral transcription(58, 83). Similar activities have not been described for ICP22,although it is possible that the effect of ICP22 in this caseis exerted indirectly. Previous studies with d92 and d97, viruseswith IE mutations analogous to those of d107 and d104, respectively,did not show this same effect on cellular protein synthesis (99).However, these previous experiments were conducted at a lowerMOI that may be below the threshold level at which the effectsof ICP22 are observed. Additional studies are required to determinethe contribution of ICP22 to this effect and the status of vhsor its ability to function in these mutant backgrounds.

The accumulation of stable GFP mRNA at 6 h p.i. (Fig. 4A) was consistent with the levels of GFP synthesized by the differentmutants early in infection (Fig. 3C). GFP mRNA was abundantlyexpressed in d106- or d107-infected cells, accumulating to a lesserdegree in the latter. This minor difference may be due to thehigher level of ICP0 synthesized in d106-infected cells (Fig.3A). In d104- or d109-infected cells, GFP mRNA was barely detectableat 6 h p.i. However, at 24 h p.i., the relative level of GFP mRNAseen in d104-infected cells increased, while in d109-infectedcells it remained very low (Fig. 4A). This difference suggestsa possible contribution of ICP22 to the transcription of GFP latein infection. The abundance of the GFP mRNA in d106-infected cellsrelative to that in d107-infected cells at 24 h p.i. is difficultto assess because of the heterogeneity in the size of the mRNAin the latter. This effect was also observed with d104, and itcorrelates with the presence of ICP22 in these two mutants. TheGFP mRNA is not spliced, so this heterogeneity may reflect differentialprocessing of the mRNA at the 3' end. Rice et al. have previouslynoted that ICP22 phosphorylates the carboxy-terminal domain (CTD)of pol II, resulting in a novel modified form of the enzyme (93).A possible explanation for the above-described results is suggestedby recent findings of McCracken et al. showing a functional linkagebetween the CTD and 3' RNA processing (72). They further demonstrateda specific interaction of the CTD with the cleavage-polyadenylationfactors CPSF and CstF. An alteration in the polyadenylation processmay thus be a consequence of the CTD modification mediated byICP22. Further studies are necessary to determine the connectionbetween the activity of ICP22 and the coupled processes of transcriptionand mRNA processing.

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FIG. 4. Accumulation of GFP mRNA and protein. (A) Total cell RNA, isolated at 6 and 24 h p.i. from Vero cells infected (MOI = 10) with the indicated viruses, was processed for Northern blot analysis with a GFP-specific probe. (B) Proteins extracted at 24 h p.i. from infected cells (MOI = 10) were separated on an SDS-18% polyacrylamide gel and transferred to a membrane for Western blot analysis with an $alpha$ -GFP monoclonal antibody. Mock, uninfected cells.

The relative levels of GFP synthesized by the different mutants at 24 h p.i. (Fig. 4B) correlated with the amounts of GFPmRNA they express late in infection (Fig. 4A). GFP was abundantin cells infected with d107 or d106 (Fig. 4B). The increased amountof GFP mRNA expressed by d104 late in infection was also reflectedproportionally at the protein level. With d109, the amount ofGFP expressed was very small. The amount of GFP expressed by thedifferent mutants late in infection was consistent with the levelof green fluorescence exhibited by the infected monolayers whenviewed under a UV microscope (data not shown). At 24 h p.i., allcells in d106- or d107-infected monolayers fluoresce, with thosein the latter exhibiting significant cytopathic effects, consistentwith previous observations on analogous mutants d95 and d92, respectively(117). A smaller proportion of fluorescing cells was observedin d104-infected monolayers, and with d109 there were even fewerof these GFP-expressing cells.

Results of the above-described studies show that in the absence of the IE proteins, the level of gene expression from thed109 genome is very low, even from the HCMV promoter, which isgenerally associated with high levels of transcriptional activity.Possible explanations for this apparent repression of the genomein the absence of viral activators are discussed below.

Toxicity and persistence of d109. Previous observations suggested that both ICP0 and ICP22 contribute to virus toxicity and that simultaneous elimination ofthese gene products in an ICP4 ICP27 background would improve the survival of infected cells. To evaluatethe toxicity of the different multiple IE mutants, Vero cell monolayerswere infected at different MOI. At 6 h p.i., the monolayers weretrypsinized to generate single-cell suspensions, and dilutionsof these suspensions were plated to enumerate CFU. The abilitiesof d107 and d106 to inhibit colony formation by infected cellswere quite similar (Fig. 5). In comparison, d104-infected cellsshowed enhanced survival, although virus toxicity was still observedat the higher MOI. These results are consistent with previousobservations on the analogous mutants d92, d95, and d97 (99).The survival of d109-infected cells was indistinguishable fromthat of uninfected cells, even at the highest MOI of 30 PFU/cell.Therefore, from the standpoint of colony-forming ability of theinfected cells, d109 is nontoxic.

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FIG. 5. Survival of cells infected with IE mutants. Vero cell monolayers were infected with the IE mutant viruses at the indicated MOI. The monolayers were harvested at 6 h p.i. and plated for determination of CFU. Colonies were counted 10 days after cell plating. Points plotted represent the surviving fractions of the infected cells relative to uninfected cells.

As another potential measure of perturbation of normal host cell function, the different IE mutants were assessed for theirability to disrupt the punctate nuclear bodies known as ND10.Early in infection, ICP0 localizes to these discrete nuclear structures(ND10), which are thought to be involved in the proliferativeor differentiation state of the cell (26, 53, 116). As infectionprogresses, ICP0 perturbs the structure and the composition ofthese nuclear bodies, which are known to contain a number of cellularproteins, including PML (29, 67, 68). Similar activitieshave also been described for the IE proteins E4-ORF3 of adenovirusand IE1 of HCMV (25, 54). The association of viral genomesand replication proteins with ND10 early in infection led to thesuggestion that these nuclear structures serve as sites whereinitial stages of HSV replication occur (46, 69). Consistentwith previous observations, the discrete PML-containing ND10 structureswere not observed in cells infected with mutants that expressICP0 (d107 and d106) (Fig. 6). In contrast, the characteristicpunctate staining, similar to that seen in mock-infected cells,was readily observed in d104- or d109-infected cells. There wasa small perturbation in the quality and quantity of staining ind104-infected cells late after infection, suggesting that ICP22may directly or indirectly affect ND10 structure and composition.

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FIG. 6. Nuclear distribution of PML in cells infected with IE mutants. Human fetal lung cells infected (MOI = 10) with the indicated viruses were processed at 6 and 24 h p.i. for immunofluorescence with an $alpha$ -PML antibody. Shown are stained infected nuclei (magnification, ×100).

Considering that d109 was nontoxic to cells, we thought it likely that the virus could establish a long-term or persistentinfection. To address this possibility, uninfected and d109-infectedVero cells were maintained and monitored for a period of 28 days.Even when infected at an MOI of 20, only a subpopulation of d109-infectedmonolayers expressed GFP (Fig. 7), and the number of these fluorescingcells decreased with time. Given the abundant expression of GFPin the presence of ICP0, it was reasonable to expect that providingICP0 to the d109-infected monolayers would induce GFP and thuscause cells harboring d109 to fluoresce. Therefore, a parallelset of d109-infected cultures was superinfected with d95 1 dayprior to each time point. The only IE regulatory protein thatd95 expresses is ICP0, and this virus does not encode GFP. Withthe induction of GFP upon superinfection with d95, d109-infectedcells were more readily identified, and these could be observedfor the duration of the experiment (Fig. 7). Considering thatthe cells doubled in number about three times during this period,as deduced from the amount of total DNA isolated (Fig. 8), a significantnumber of d109-infected cells were maintained for up to 28 daysp.i. This observation was also seen in HEL cells infected withd109 for up to 6 weeks (data not shown). PCR quantitation of thenumber of d109 genomes in the nuclei of infected Vero cells showeda gradual decline over time, although the number of viral genomespresent at 28 days p.i. still constituted about one-third of thegenomes present at 1 day p.i. (Fig. 8).

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FIG. 7. Persistence and induction of d109. Mock-infected (Mock) and d109-infected (MOI = 20) Vero cells were maintained for a period of 28 days in 2% serum at 34°C to limit cell division. At different time points (in days) after infection (indicated on the left), the monolayers were photographed under phase-contrast and fluorescence microscopes. A separate set of d109-infected cultures was superinfected with d95 (MOI = 20) 1 day prior to the time points indicated on the left.

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FIG. 8. Persistence of d109 genomes in infected cells. A separate set of d109-infected monolayers was maintained in parallel to those described in the legend to Fig. 7. At the same time points indicated, total infected cell DNA was isolated. Equivalent aliquots of the DNA samples, along with standards, were used in PCRs to amplify sequences from the gC gene (top). The amounts of total infected cell DNA (in micrograms) isolated at different time points (in days) after infection with d109 are plotted along with the number of viral genomes derived from quantitation of the gC PCR products.

The number of d109 genomes present in the nuclei at 1 day p.i. exceeded the expected value by about 10-fold. Jamieson et al.found that the number of viral genomes in the nuclei 1 day afterinfection with in1833 exceeded the number present at 1 day p.i.because capsid uncoating proceeded relatively slowly (47a). Itmay be that since our input inoculum was normalized to the numberof genomes present in the nuclei at 6 h p.i., the larger numberdetected at 1 day p.i. reflected additional genomes that had notbeen uncoated by 6 h p.i. It is also noteworthy that at 28 daysp.i. the number of genomes present in the cells exceeded the numberof cells in the culture. There were approximately 7 × 10⁷ genomes of d109 (Fig. 8) and 1.5 × 10⁷ cells, assuming that the cell number doubled three times overthe 28-day period. However, only about one-third of the cellsappeared to express detectable GFP upon infection with d95 at28 days (Fig. 7). The reason for this is unclear. The cells wereinfected at an MOI of 20; however, at present we do not know howthese genomes partition from the initially infected cell intodaughter cells following cell division. It may be that some daughtercells do not contain genomes while others retain multiple genomes.Alternatively, the infection of overly confluent monolayers withd95 may not result in efficient infection, or some of the quiescentgenomes may not respond to ICP0. With respect to these last twopoints, when monolayers of d109-infected (28 days p.i.) HEL cellswere infected with d95, nearly all of the cells fluoresced (datanot shown). HEL cells are more prone to contact inhibition thanare Vero cells and therefore did not divide to the same extentas Vero cells over the 28-day period.

Taken together, the results presented thus far demonstrate that d109 is a noncytotoxic virus that can efficiently establisha persistent infection. Furthermore, the results show that geneexpression from the persisting quiescent viral genomes remainsinducible after long-term maintenance of the infected cultures.In the absence of induction, the number of green-fluorescing cellsin d109-infected monolayers varies, but it is generally low. Thereason for the high level of activity of the HCMV promoter regulatingGFP expression in this subpopulation of cells is not known atthe present time. To rule out the possibility that this smallfraction of d109-infected cells expressing GFP was due to a low-levelcontamination with viruses that synthesize ICP0 or ICP4, Verocells were infected with d109 and at 24 h p.i. were processedfor immunofluorescence staining with $alpha$ -ICP0 and $alpha$ -ICP4 monoclonalantibodies. The results show that the d109-infected cells, whichexpressed GFP, did not express ICP4 or ICP0 (Fig. 9). Therefore,the expression of GFP from the HCMV IE promoter was not due tocontamination of the infected cultures by viruses expressing ICP4or ICP0.

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FIG. 9. Absence of ICP0 and ICP4 in GFP-expressing d109-infected cells. Vero cells were infected with d109 (MOI = 10) and, at 24 h p.i., processed for immunofluorescence with $alpha$ -ICP0 and $alpha$ -ICP4 monoclonal antibodies. Also included were d106- and d99-infected cells as positive controls for ICP0 and ICP4 staining, respectively. The secondary antibody used was conjugated to rhodamine. Photomicrographs in each column represent the same field viewed by phase-contrast microscopy (top) or fluorescence microscopy with the appropriate filter blocks for observing green (middle) or red (bottom) fluorescence.

The properties of d109 suggest that it is capable of transducing functional genes into cells with minimal effects on cellsurvival. As an immediate test of this capability, we exploredthe possibility that d109-infected monolayers could serve as complementingcells for plaque formation by HSV mutants defective in essentialgenes. This prediction would hold true assuming that the regionof the d109 genome required for complementation is maintainedin the infected cells. To address this possibility, Vero monolayerswere infected with d109 and, at 24 h p.i., the infected monolayerswere used to determine the titers of virus mutants with lesionsin capsid genes.

The titers of the capsid mutants obtained on d109-infected Vero cells were not significantly different from their known titersdetermined on dedicated cell lines that contain and express complementinglevels of the genes mutated in the virus (Fig. 10). Induction ofGFP from the resident d109 genomes was evident in all of the cellsof the plaques (data not shown). It is important to note thatthe formation of the plaques on the monolayer was possible becaused109 is sufficiently nontoxic that the nonsuperinfected areasof the monolayer maintained their integrity. These results furtherunderscore the persistence and subsequent functionality of thed109 genomes resident in noncomplementing cells.

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FIG. 10. Efficiency of plating of capsid gene mutants on d109-infected cells. Vero cell monolayers were infected with d109 (MOI = 10), and at 24 h p.i. the infected monolayers were used to determine the titers of virus mutants with lesions in capsid genes. The structure of the d109 genome is shown, along with the genomic locations of the capsid genes mutated in the viruses whose titers were measured. Virus stock titers of the mutants, determined with the appropriate complementing cell lines, were provided by S. Person. See the legend to Fig. 1 for definitions of symbols and abbreviations.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

This study was undertaken to determine the effects of the HSV IE proteins expressed from virus mutants defective in ICP4 oncell survival and gene expression. The information gained fromthese studies is relevant to the activities of the IE genes andthe utility of replication-defective viruses as gene transfervehicles. The results of this study clearly demonstrate that bothICP0 and ICP22 are toxic to cells. We found it necessary to abrogateall IE gene expression to completely eliminate the toxicity associatedwith HSV infection. Furthermore, both ICP0 and ICP22 affectedtransgene expression, with ICP0 having the greater effect. Onevirus, d109, which did not express any IE proteins in noncomplementingcells, was capable of establishing a long-term relationship withthe cell, in which the genome persisted in the nucleus in a relativelyinactive but potentially functional state.

Toxicity of viral mutants. The toxicity associated with ICP4 mutants has long been documented. Chromosomal damage occurs (49), and the infected cellsdie, probably due to both necrotic and apoptotic modes of celldeath (49, 63). In the absence of ICP4, the remaining IE proteinsare overexpressed. Considering the large number of cellular proteinsand metabolic systems that the IE proteins have been found tointeract with or modify, it is probable that the observed toxicityis a complex superposition of many deleterious effects.

A UV-irradiated virus is not toxic to cells (78), suggesting, but not proving, that the virus particle itself is not toxic.Elimination of toxicity with the d109 mutant clearly demonstratesthat the virion is not toxic to cells. Considering that the virusparticle contains enzymatic functions, including a protein involvedin the attenuation of host protein synthesis, UL41 or vhs (59,79, 91), it is surprising that cells infected with d109 ata high multiplicity (30 PFU/cell) are indistinguishable from uninfectedcells with respect to morphology, protein synthesis, and the abilityto divide. Perhaps d109 virions contain smaller numbers of particularproteins, such as vhs, relative to wt virions. This could occuras a consequence of suboptimal complementation during propagationon FO6 cells. Alternatively, as suggested from the studies withUV-irradiated virus, the effects of the virion proteins in theabsence of IE proteins or metabolic inhibitors are not sufficientto adversely affect cell function.

This study complements and extends previous studies from our lab demonstrating that elimination of either ICP22 (117) orICP0 (99) from an ICP4 ICP27 virus (98) reduced toxicity. While these reports do not elucidatethe mechanism by which ICP0 and ICP22 cause cell death, all threestudies clearly demonstrate that mutants expressing ICP0 inhibitcolony formation, probably by affecting cell cycle progression.The phenotypes of d95 (ICP4 ICP27 ICP22)- and d106 (ICP4 ICP27 ICP22 ICP47)-infected cells are similar in that the cells do not divide.They grow in size and continue to be otherwise metabolically activeuntil they die. Further experiments are necessary to determineif and how the ability of ICP0 to affect transcription (50,99), translation (51), and the activity of DNA-dependent proteinkinase (61) and to interact with ubiquitin proteases (30),translation factors (51), cyclins (52), and PML oncogenicdomains (PODs) (29, 67, 68) contributes to this phenotype.Considering this, and the observed phenotype of viruses expressingICP0, such vectors may be of limited utility. Finally, it shouldbe noted that these studies do not directly address the potentialcontribution of ICP47 to toxicity, since the abrogation of itsexpression was obligatory to the abrogation of ICP22 expressionby construction. However, the results of previous transfectionexperiments imply that ICP47 does not significantly contributeto toxicity (48).

Gene expression. ICP0 is a promiscuous transactivator of gene expression (27, 33, 81, 90). Viral gene expression is also generallyreduced in ICP0 mutants (5, 6). In accord with these observations,we found that GFP expression from the HCMV IE promoter was highlydependent on ICP0. In the absence of all of the HSV IE proteins,the level of expression was extremely low. Like HSV IE promoters,the HCMV IE promoter can be activated by an IE protein (12,108) and a virion component (65, 109). Both the HSV and HCMVgenomes localize to ND10 structures early in infection, in theabsence of viral protein synthesis (47, 69). Both establishlatent infections in which the viral genomes, including the IEpromoters, are relatively silent (77, 94). HSV and HCMV alsoexpress IE proteins, ICP0 by HSV and IE1 by HCMV, which are transactivatorsthat localize to ND10 and dissociate PML from the POD structures.In the case of HSV, ICP0 has been shown to be involved in reactivationevents in vivo and in tissue culture model systems (5, 14,35, 41, 95, 119). Our studies showed that a virus expressingICP0 will activate a previously silent HCMV promoter on persistingd109 genomes weeks after infection. HCMV infection will also activateGFP expression in d109-infected HEL cells (data not shown). Perhapsthe observed low level of HCMV promoter activity in d109-infectedcells represents the true "ground state" of genomes localizedat ND10 in the absence of viral activator proteins, and it mayreflect some of the events that occur in latency. The observationsof Preston and Nicholl are consistent with ours, and they haveproposed that HSV and HCMV IE promoters are repressed in the absenceof VP16, ICP4, and ICP0 (89).

GFP expression in d109-infected cells was not uniform, being abundant in a subpopulation of cells and undetectable in mostcells. It may be that the HCMV promoter is active in the absenceof ICP0 only in cells which are in a particular stage of the cellcycle or state of activation by signaling pathways. Cai and Schafferhave shown that at a particular point in the cell cycle, the intracellularenvironment reduces the requirement for ICP0 (6). It is possiblethat the occurrence of GFP-expressing d109-infected cells is areflection of cells in this state. Alternatively, the fluorescentcells may represent those in which the appropriate signaling pathwaysfor specific targets in the HCMV promoter are activated. The HCMVpromoter contains sites for NF- $kappa$ B, CREB, retinoic acid receptor,and AP-1 (1, 34, 44, 101), all of which are componentsof regulated pathways. It remains to be tested whether the HCMVpromoter on the d109 genome can be activated by one of these pathways.

d109 as a gene transfer vector. From the standpoints of toxicity, genome persistence, and efficiency of gene delivery, d109 is clearly an optimal replication-defectiveherpesvirus vector. However, the very manipulations that conferredthese attributes resulted in low-level and perhaps repressed geneexpression. It may be that this level of gene expression is sufficientfor some applications. Most cellular genes are not expressed atthe level of an ICP0-induced viral gene. However, it is likelythat systems for cell- or tissue-specific expression of transgeneswill have to be incorporated into d109.

It is interesting that the development of adenovirus vectors has proceeded along parallel lines, with analogous results. E1-deletedadenovirus exhibits high-level expression of transgenes from theHCMV promoter; however, other viral proteins are also expressed,and the virus is somewhat toxic to cells (16). The additionaldeletion of the E4 region resulted in a virus that was less toxicand persisted in cells for long periods of time (2, 32).However, expression from the HCMV promoter was greatly reduced.E4 contains seven open reading frames (64). One of them, Orf3,like ICP0, perturbs ND10 structures (11, 25). The adenovirusgenome also localizes to ND10 structures in the absence of viralprotein synthesis (96). Considering these parallels as wellas the similar phenotypes of E1-E4-deleted adenovirus and d109,it is likely that approaches for promoting or regulating geneexpression from the vectors will have similar outcomes in bothviruses.

The development of HSV strains has systematically progressed (18, 98, 99, 117) to the point where we now have a virusthat has no detectable harmful effects on cells, does not expressits own genes, and efficiently delivers the genome to the nucleus,where it persists for a prolonged period of time in a functionalform. The lack of toxicity does not appear to be constrained bythe input MOI. The results of this study allow future effortsto be aimed at understanding the association between persistingHSV genomes and the cell nucleus and determining how this associationaffects transcription. These considerations have obvious relevanceto expression of transgenes from HSV vectors and may reflect eventsoccurring during latency, when the genome is relatively silentbut persists in a potentially functional state.

	ACKNOWLEDGMENTS

This work was supported by NIH grants DK44935 and AI30612.

We are grateful to Stanley Person for providing the capsid gene mutants and to Colton A. Smith and Michael J. Carrozza forreviewing the manuscript. We also thank Patricia Bates for supplyingthe specific PCR conditions and Arthur Webb for the constructionof pAT1 and pAT2.

	FOOTNOTES

^* Corresponding author. Mailing address: E1257 Biomedical Science Tower, Department of Molecular Genetics and Biochemistry,University of Pittsburgh School of Medicine, Pittsburgh, PA 15261.Phone: (412) 648-9947. Fax: (412) 624-1401. E-mail: neal{at}hoffman.mgen.pitt.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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