Long-Term Transgene Expression in Mice Infected with a Herpes Simplex Virus Type 1 Mutant Severely Impaired for Immediate-Early Gene Expression

doi:10.1128/JVI.74.2.956-964.2000

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Journal of Virology, January 2000, p. 956-964, Vol. 74, No. 2
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Long-Term Transgene Expression in Mice Infected with a Herpes Simplex Virus Type 1 Mutant Severely Impaired for Immediate-Early Gene Expression

Ker R. Marshall,¹ Robin H. Lachmann,² Stacey Efstathiou,² Angela Rinaldi,¹ and Chris M. Preston¹^,^*

Medical Research Council Virology Unit, Glasgow G11 5JR, Scotland,¹ and Division of Virology, Department of Pathology, University of Cambridge, Cambridge CB2 1QP, England²

Received 27 August 1999/Accepted 14 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The role of viral immediate-early (IE) gene expression in herpes simplex virus type 1 (HSV-1) latency was investigated. TheHSV-1 multiple mutant in1312, defective for the expression ofthe virion transactivator VP16 and the IE proteins ICP0 and ICP4,was used as the parent for these studies. The coding sequencesof the Escherichia coli lacZ gene, preceded by the encephalomyocarditisvirus internal ribosome entry site, were inserted into the regionof in1312 that encodes the latency-associated transcripts (LATs)such that transcription of the transgene was controlled by theLAT promoter. This insert has previously been shown to directlong-term latent-phase expression of $beta$ -galactosidase in a wild-typeHSV-1 genome (R. H. Lachmann and S. Efstathiou, J. Virol. 71,3197-3207, 1997). The resulting recombinant, in1388, was apathogenicafter inoculation into mice via the footpad and did not detectablyreplicate in dorsal root ganglia (DRG) or footpads. Mutant in1388established latency in DRG, and $beta$ -galactosidase was expressedin increasing numbers of neurons over the first 25 days of infection.During latency, more than 1% of neurons in ganglia that innervatethe footpad expressed $beta$ -galactosidase, with the number of positivecells remaining constant for at least 5 months. Rescue of theVP16, ICP0, or ICP4 mutations of in1388 did not affect the numberof $beta$ -galactosidase-expressing neurons detected during latency.The results demonstrate that HSV-1 mutants severely impaired forIE gene expression are capable of establishing latency and efficientlyexpressing a foreign gene product under control of the LATpromoter.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Infection with herpes simplex virus type 1 (HSV-1) normally results in productive replication of virus and death of the hostcell. Neurons, however, are able to survive infection and retainthe HSV-1 genome in a latent state for the lifetime of the host.Reactivation of latent virus and, in some instances, reappearanceof disease occur in response to stimuli that cause stress to theneuron or to the host organism (reviewed in references 43, 54,60).

Transcription of the HSV-1 genome is largely controlled by the immediate-early (IE) proteins ICP4 (Vmw175) and ICP0 (Vmw110)and by the virion protein VP16 (Vmw65 or $alpha$ -TIF). ICP4 is a transcriptionactivator that is absolutely required for productive infection.Early and late gene transcription does not occur after infectionwith virus mutants lacking functional ICP4 (10, 38, 62).ICP0 alters the intranuclear environment such that entry of HSV-1into the lytic cycle is facilitated (17, 18). Infection atlow multiplicity of infection (MOI) with viruses possessing mutationsthat inactivate ICP0 results in only a small proportion of infectedcells supporting replication and most viral genomes being retainedin a quiescent state (16, 40, 44, 45, 56, 57). Theabsence of ICP0 can, however, be overcome by carrying out infectionat a high MOI (16, 44, 57). Transcription of the IE genesis stimulated by VP16, a component of the incoming virus particlewhich interacts with the cell factors Oct-1 and HCF to form amultiprotein complex at the TAATGARAT (R is a purine nucleotide)sequences found in all IE promoters (reviewed in reference 36).The virus mutant in1814, which expresses nonfunctional VP16, exhibitsa phenotype similar to that of ICP0 mutants, with most cells infectedat low MOI failing to initiate early or late gene expression andretaining the HSV-1 genome in a quiescent state (1, 23).The absence of functional ICP4, ICP0, or VP16 therefore arreststhe HSV-1 lytic cycle at earlystages.

During latency in humans or animals, gene expression characteristic of productive replication cannot be detected; insteadonly one portion of the genome, located within the long repeat(R_L) region, is transcribed to yield the latency-associated transcripts(LATs) (20, 55). The factors controlling the repression ofviral lytic gene expression and the selective transcription ofthe LATs are unclear. It is thought that the lytic and latentoutcomes of infection are mutually exclusive and that a majorcommitment to one or the other pathway is made early after infection(30, 33, 52). The exact point at which the pathways divergeis not known at present, although studies using virus mutantsin animal models of latency point to a major early decision, atthe level of IE gene expression or IE protein function. ICP4 isnot required for latency or production of LATs, since viral DNAand neurons containing LATs can be detected after infection withviral ICP4 deletion mutants (11, 26, 49). It was found thatmutant in1814, defective for VP16 function, established latencyin mice apparently as efficiently as wild-type HSV-1 when comparisonswere made on the basis of PFU in the inoculum, demonstrating thatfunctional VP16 is not absolutely required for latency (12,53). Similarly, viral mutants lacking functional ICP0 were ableto establish latency and to reactivate, although they were attenuatedfor replication in mice (4, 7, 31). For VP16- and ICP0-deficientmutants, however, the quantitative assessment of latency establishmentis imprecise because the mutants are impaired for replicationat the site of inoculation and in ganglia. In addition, only 0.1to 1.0% of virus particles in a preparation can form plaques,compared with the number obtained when VP16 or ICP0 is providedexogenously to complement the effects of the mutations (1,16, 24, 56). For example, in experiments in which animalswere inoculated with equivalent doses (as PFU) of in1814 or arevertant, two factors would have affected the amount of virusreaching the sensory ganglia. First, the mutant inoculum contained100- to 1,000-fold more viral genomes than the revertant inoculum,and second, the revertant replicated more efficiently than themutant at the site of inoculation, compensating to some extentfor the lower number of genomes added. In addition, replicationin the neuron and spread in the nervous system may have affectedthe ultimate number of cells harboring latent viral genomes (8,13, 27, 58). Therefore, when a VP16 or ICP0 mutant is comparedwith a wild-type or revertant virus, differences in replicationat the periphery or in the ganglion may obscure true effects ofthe genetic defect on the establishment of latency. In view ofthese factors, although it is clear that latency can be establishedin the absence of VP16, ICP0, or ICP4, it has not been possibleto make a quantitative evaluation of the contribution of theseproteins to the establishment of latency in terms of events withintheneuron.

One way of overcoming the complexities introduced by differential replication of mutant and wild-type viruses in experimentalanimals is the use of in vitro model systems to study latency.In one approach, primary cultures of sympathetic or sensory neuronsare infected with HSV-1 in the presence of acyclovir to preventvirus replication. Latency is established, provided nerve growthfactor (NGF) is present in the cell culture medium, and many cellsexpress LATs (50, 63, 64). Upon withdrawal of NGF or uponactivation of signal transduction pathways in the presence ofNGF, reactivation occurs and virus replication rapidly resumes(51, 63, 64, 66). A second approach has been to infecthuman fibroblasts with mutants lacking VP16 and/or ICP0 function(23, 24, 40, 45, 46, 56). In these cases, the majorityof viral genomes do not initiate productive replication and areretained in a quiescent state that resembles latency in many respects.The viral genome is sequestered in a nonlinear configuration,as in vivo, and no gene expression is detected; indeed promotersin the viral genome become repressed within the first 24 h afterinfection (40, 45). Reversal of repression in fibroblastsrequires the presence of ICP0 (18, 40, 45, 56). Thereis a major difference between the interaction of HSV-1 with thehost cell in the two model systems in terms of the effect of ICP0.In cultured neurons, viruses with mutations that inactivate ICP0established latency 1,000-fold less efficiently than wild-typevirus, on a virus particle basis (65), whereas in fibroblaststhe absence of ICP0 aids the retention of quiescent viral genomesdue to reduction of cytotoxicity and increased propensity to enterthe quiescent state (24, 39, 40, 45, 46). The differencein the requirement for ICP0 forms a point of focus which distinguishesthe two model latencysystems.

There is considerable interest in the potential use of HSV-1 as a vector for gene therapy, particularly for the treatmentof neurological diseases (reviewed in references 14, 22, and29). The ability of latent virus to be retained for the lifetimeof an individual, coupled with the use of the LAT promoter toachieve long-term expression of foreign gene products, is centralto this approach. Problems arise in the development of HSV-1-derivedvectors, however, due to the toxicity of HSV-1 for mammalian cellsand the complexity of the LAT transcription unit. Cytotoxicityis due mainly to the expression of viral proteins in the infectedcell, and it has been shown that IE proteins are toxic when introducedby transfection of plasmids or infection with viral mutants whichexpress only the IE genes (25, 39, 67). Toxicity can beovercome by severely reducing IE gene expression, and viruseswith mutations in VP16 and IE genes are promising vehicles forthe development of gene therapy vectors (39, 45). The problemof long-term expression of foreign gene products has recentlybeen addressed by a novel modification of the LAT region (28).Insertion of a reporter gene cassette (lacZ or a fusion of lacZand neomycin phosphotransferase named $beta$ -geo) at a position 1.5kbp downstream of the 5' end of the primary LAT transcript resultedin the maintenance of all cis-acting sequence elements for authenticlatent expression. By linking the transgene to the internal ribosomeentry site (IRES) of encephalomyocarditis virus, it was possibleto achieve efficient translation of the resulting transcript,which contains a long 5' leader sequence. Upon inoculation ofmice with such a recombinant virus, expression of $beta$ -galactosidaseactivity was detected only at low levels in dorsal root ganglion(DRG) neurons during the early stages of infection but increasedduring the establishment of latency, as would be expected fora transgene under authentic latentcontrol.

In the experiments reported here, we have introduced the IRES- $beta$ -geo construct into the LAT region of a multiply defectiveHSV-1 mutant impaired for the production of functional VP16, ICP0,and ICP4 and have analyzed $beta$ -galactosidase expression after inoculationinto mice. The experiments were designed to answer three questions.First, can latency be established efficiently after infectionof mice with a multiply defective virus that is unable to replicateat the site of inoculation or in the sensory ganglia that innervatethat site? Second, do the viral transactivator proteins affectthe establishment of latency and/or the expression of LATs? Inherentin this question is a resolution of whether ICP0 is required forefficient establishment of latency in vivo, as it is in culturedneurons, or if ICP0 is not required, as found in studies withfibroblasts. Third, can long-term gene expression in neurons beachieved by use of the IRES- $beta$ -geo construct inserted into theLAT region of an HSV-1 mutant defective for IE gene expression?The final question is relevant to the potential for using multiplydefective mutants as starting points for the construction of HSV-1vectors for long-term gene expression inneurons.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmids. Plasmid pSLAT1 $beta$ geo contains IRES- $beta$ -geo (with the Moloney murine leukemia virus long terminal repeat terminator) cloned betweenthe HpaI sites in the major LATs (nucleotides 120,300 and 120,466in the inverted long repeat [37]), as described by Lachmannand Efstathiou (28). Plasmid pGX158 is the HSV-1 BamHI f fragment,containing VP16 coding sequences, cloned into pAT153, and pGX58is the HSV-1 XhoI c fragment, which contains the ICP4 coding sequences,cloned into the XhoI site of pMK16. Plasmid pAR28 was preparedby cloning a 4,596-bp HpaI/SstI fragment (nucleotides 120,466to 125,062) from pCP2461 (41) between the SstI and HincII sitesofpUC18.

Cells. Baby hamster kidney (BHK) cells were grown in Eagle medium supplemented with 10% newborn calf serum, 10% tryptose phosphate,and 100 U of penicillin and 100 µg of streptomycin per ml (ETC10).Human osteosarcoma U2OS cells were propagated in Dulbecco mediumsupplemented with 5% fetal calf serum, 5% newborn calf serum,and 100 U of penicillin and 100 µg of streptomycin perml.

Construction of recombinant viruses. The locations of restriction endonuclease cleavage sites and fragments used for virus construction are shown in Fig. 1. HSV-1mutants tsK and in1312 have been described previously (9, 38,41). To construct in1388, pSLAT1 $beta$ geo was cleaved with XhoI andScaI and transfected into BHK cells together with DNA isolatedfrom in1312. To identify recombinants containing the IRES- $beta$ -geoinsert, DNA was prepared from pooled or single plaque isolatesand cleaved with EcoRV and XhoI. DNA samples were analyzed bySouthern hybridization with the 4,166-bp PstI/XhoI fragment (nucleotides118,862 to 123,029) from pJR3 (15) as the probe. After fourrounds of plaque purification and screening by Southern hybridization,an isolate containing 3,425- and 2,250-bp fragments from pSLAT1 $beta$ geo,with no detectable 4,074-bp fragment from the in1312 parent, wasobtained and named in1388. To rescue the ICP0 mutation, in1388DNA was cotransfected with HindIII-cleaved pAR28 and DNA fromplaque isolates was prepared. Samples were cleaved with BstEIIand XhoI and probed with a 1,961-bp fragment (nucleotides 121,068to 123,029) from pAR28, which hybridized to a 1,674-bp fragmentfrom in1388 and the 1,961-bp fragment itself from the rescuant(the difference represents the 317-bp deletion of the RING domain).An isolate with no detectable in1388-derived fragment was namedin1365. Restoration of ICP0 function was confirmed by the demonstrationthat superinfection with in1365 reversed the quiescent state ofanother in1312-based virus (40; C. M. Preston, unpublished observations).The VP16 mutation was rescued by cotransfection of in1388 DNAwith HindIII-cleaved pGX158 and subsequent screening for lossof the BamHI site in the VP16 coding sequences (1). A pureisolate was named in1366. Infection with in1366 activated an HSV-1IE promoter present in the in1312 genome, demonstrating that VP16function was restored (C. M. Preston, unpublished observations).The ICP4 mutation was rescued by cotransfection of in1388 DNAwith XhoI-cleaved pGX58 and plaque purification of viruses capableof replication at 38.5°C. An isolate that formed plaques equallyefficiently at 38.5 and 31°C was named in1368. The propertiesof the mutants used are summarized in Table 1.

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FIG. 1. Structure of in1388 in R_L. (A) Organization of the inverted long repeat from nucleotides 118,000 to 125,000, including the locations of the ICP0 mRNA, the primary LAT (terminating outside the region represented), and the stable 2-kb species. (B) Insertion of IRES- $beta$ -geo and the Moloney murine leukemia virus long terminal repeat terminator (Term), plus the deletion of the ICP0 RING domain. Restriction sites used for cloning and for preparing probes are labelled as follows: E, EcoRV; P, PstI; H, HpaI; B, BstEII; A, Asp 718; X, XhoI; S, SstI. The PstI site at nucleotide 118,659 and the BstEII sites at nucleotides 119,194 and 120,091 are not shown.

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TABLE 1. Characteristics of mutants used

Virus assay. The titer of in1388 was measured by plaque formation on BHK cells at 31°C in the presence of 3 mM hexamethylene bisacetamide(HMBA) (34). Direct comparison of the titers of rescuants withthat of in1388 by this method is not informative, because thepresence of VP16 or ICP0 results in more-efficient plaque formationper virus particle of the inoculum. A method described by Caiand Schaffer, based on estimation of viral DNA in virus preparations,was therefore used for comparison between mutants (3). A sampleof each virus preparation was mixed with a fixed amount of in1332,a mutant containing an insertion of Escherichia coli lacZ in thethymidine kinase (TK) coding sequences (39). DNA was preparedfrom the mixtures, cleaved with EcoRI, and analyzed by Southernhybridization, with the HSV-1 EcoRI n fragment as a probe. DNAfrom in1388 and rescuants gave a single 2.4-kbp band (EcoRI nitself), whereas in1382 DNA gave 1.85- and 1.0-kbp bands due tothe lacZ insertion. Quantification was achieved by phosphorimageanalysis of autoradiographs and comparison of the signals fromthe in1388-derived mutants with the signal from the in1382 internalcontrol. In a further test, mutants were titrated on U2OS cells,on which ICP0-deficient and VP16-deficient mutants form plaqueswith normal efficiency (C. M. Preston, unpublished observations;68), at 31°C in the presence of 3 mM HMBA. The relative titersfrom this approach agreed well with the values obtained by hybridization.In the experiments presented here, the titer of in1388 is presentedas the value on BHK cells with 3 mM HMBA present, and equivalentamounts of the other mutants were injected, with the DNA contentsof inocula as the basis fornormalization.

Animal experiments. Five-week-old female BALB/c mice were infected unilaterally via the right rear footpad with 25 µl of cell-released virus suspension,diluted in ETC10. At various times postinfection the ipsilateralDRG from lumbar levels L1 to L6 were partially dissected withina hemiblock of vertebral column from which the spinal cord andspinal nerve trunks had been removed, uncovering the underlyingDRG within the intervertebral foramina. Subsequent fixing (4%paraformaldehyde in phosphate-buffered saline [PBS] for 1 h onice), washing (twice for 15 min in ice-cold PBS), and a whole-mount $beta$ -galactosidase assay (overnight incubation at 37°C in a stainingsolution consisting of 1 mg of 5-bromo-4-chloro-3-indolyl- $beta$ -D-galactoside/mlin PBS containing 5 mM potassium ferrocyanide, 5 mM potassiumferricyanide, 2 mM MgCl₂, 0.1% [vol/vol] NP-40, 0.1% [wt/vol]sodium deoxycholate) was performed with the DRG in situ. DRG wereremoved from the intervertebral foramina for counting blue ( $beta$ -galactosidase-expressing)neurons, after clarification by immersion overnight in PBS containing20% (vol/vol) glycerol. Individual DRG were placed between twomicroscope slides for photography at ×45 magnification withoutcounterstaining. Feet were dissected from mice proximal to theankle joint and frozen at $-$ 70°C prior to processing. Individualfeet were minced with fine scissors, disrupted in glass homogenizers,and homogenized again in 1 ml of ETC10. The homogenate was transferredto screw-cap vials and subjected to two cycles of freezing andthawing at $-$ 70 and 37°C. Samples were sonicated and titrated onU2OS cells at 31°C with 3 mM HMBA present. DRG from each mousefrom levels L3 to L5 were dissected, pooled into 400 µl of ETC10in glass screw-cap vials, and stored at $-$ 70°C. Samples were thawedand homogenized on ice with an Omni µH hand-held homogenizer (CamlabLtd.). Homogenates were sonicated briefly and transferred to 1.5-mlmicrocentrifuge tubes, and cell debris was pelleted. Supernatantswere titrated on U2OS cells at 31°C, with 3 mM HMBApresent.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of HSV-1 mutant in1388. The starting point for the studies presented here was mutant in1312, which contains three mutations: an inactivating insertionin the coding sequences for VP16, a deletion of the RING domainof ICP0, and the ICP4 temperature-sensitive (ts) mutation derivedfrom tsK (41). The last is a tight mutation which reduces virusreplication by approximately 10⁵-fold at 38°C, the core temperature of the mouse (35, 61;C. M. Preston, unpublished observations). In preliminary experiments,mice were inoculated via the footpad with 10⁶ PFU of tsK and DRG were screened for the presence of virus, bysonication and titration at 31°C, 1 and 4 days later. No viruswas detected at either time, demonstrating that the ts mutationeffectively inactivated the function of ICP4 in ganglia. PlasmidpSLAT1 $beta$ geo, containing the IRES- $beta$ -geo cassette in the LAT region,was recombined with in1312 DNA, and progeny plaques were screenedby Southern hybridization through four rounds of purificationuntil no parental sequences were detectable on long autoradiographicexposures, indicating that the insertion was present in both copiesof R_L. The resulting virus was named in1388.

Latent expression of $beta$ -galactosidase by in1388. Mice were inoculated with 8 × 10⁵ PFU of in1388, and ganglia were examined by histochemical staining for $beta$ -galactosidase atvarious times (Fig. 2 and 3). This assay quantifies the establishmentof latency by monitoring the activity of the LAT promoter to directthe synthesis of transcripts containing the $beta$ -geo sequences. Expressionof $beta$ -galactosidase was readily detected in L3, L4, and L5 DRG,and the number of positive cells increased through 3, 5, and 25days, remaining at undiminished levels until at least 6 monthspostinoculation. Only ganglia containing neurons which innervatethe footpad were positive, and staining was observed exclusivelyin cells which morphologically resembled neurons. No $beta$ -galactosidasewas detected in ganglia innervating the uninoculated foot. Therelationship between input virus dose and number of positive neuronswas investigated (Table 2). A 10-fold reduction of in1388 dose,to 8 × 10⁴ PFU per mouse, gave an approximately 2-fold decrease in the numberof expressing neurons, and a further 10-fold reduction to 8 ×10³ PFU per mouse gave numbers additionally 6-fold lower, close tothe limit of reliable quantification.

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FIG. 2. Expression of $beta$ -galactosidase in DRG neurons. Mice were infected with 8 × 10⁵ PFU of in1388, and L3, L4, and L5 DRG were histochemically stained for the presence of $beta$ -galactosidase at 3 (A), 5 (B), 25 (C), and 182 (D) days after inoculation.

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FIG. 3. Time course of $beta$ -galactosidase expression. Mice were infected with 8 × 10⁵ PFU of in1388, and the positive neurons in DRG were counted at various times. The values for L3, L4, and L5 DRG combined per mouse are presented, with standard deviations (sd) shown.

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TABLE 2. Effect of input dose on expression of $beta$ -galactosidase

Effects of rescuing mutations of in1388. To assess whether VP16, ICP0, or ICP4 functions affected the establishment of latency, the mutations in the genes encodingthese proteins were rescued, giving viruses in1365 (ICP0 rescued),in1366 (VP16 rescued), and in1368 (ICP4 rescued). Mice were inoculatedwith 8 × 10⁴ or 8 × 10³ PFU of in1388 or equivalent amounts of the rescuants, and $beta$ -galactosidase-positiveneurons were counted at 42 days postinfection (Fig. 4 and Table3). The doses were chosen because, as shown in Table 2, theyrepresent points at which the dose-response curve was almost linear.In all cases, the numbers of positive neurons in animals inoculatedwith the rescuants were indistinguishable from those of animalsinoculated with in1388, and no differences in intensity of stainingwere observed.

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FIG. 4. Expression of $beta$ -galactosidase by rescuants of in1388. Mice were infected with 8 × 10⁴ PFU of in1388 (A) and an equivalent amount of in1365 (B), in1366 (C), or in1368 (D). DRG were stained for the presence of $beta$ -galactosidase at 42 days after inoculation. The L4 and L5 DRG are shown.

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TABLE 3. Expression of $beta$ -galactosidase after inoculation with rescuants of in1388

Absence of detectable in1388 replication in DRG or footpads. The retention and possible replication of in1388 in the footpad and ganglion were examined and compared with those of in1368,in which ICP4 is fully functional (Fig. 5). The titer of in1388,measured by titration on U2OS cells in the presence of 3 mM HMBA,declined rapidly from 6 h postinfection (a time before virus replicationwould be expected), with no virus detectable by 4 days postinoculation.The titer of in1368 also declined, but less rapidly than thatof in1388 such that low levels of virus were present at 4 days,but not at 7 days, postinoculation. Infectious virus could notbe detected in DRG at any time after infection with in1388. Forin1368-inoculated mice, all ganglion samples were negative withthe exception of pooled DRG from one animal of four at 3 dayspostinfection (1 PFU in L3, L4, and L5 combined) and two animalsof four at 4 days postinfection (1 PFU in each animal). Therefore,no in1388 and only very low levels of in1368 were detected inDRG, indicating that extensive replication of mutants, even whenICP4 was functional, did not occur. In the footpad, the declinein the titer of in1388 was consistent with clearance of the initialinoculum without significant increase in virus load due to replication,suggesting that the inoculum provided the source of virus to nervetermini. The lower rate of decline of in1368 suggested that, asexpected, limited replication of this mutant occurred but, again,that the amount of virus in the footpad was primarily determinedby the input inoculum.

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FIG. 5. Virus titers in footpads. Mice (four per point) were inoculated with 8 × 10⁴ PFU of in1388 or an equivalent amount of in1368. At various times after inoculation (the first point, defined as 100%, was at 6 h), feet were homogenized and virus titers on U2OS cells in the presence of 3 mM HMBA were determined. The ranges of values are shown.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We describe HSV-1 mutant in1388, which is severely impaired for the production of IE gene products and additionally containsan insertion of IRES- $beta$ -geo in the LAT region, thereby allowinglatently infected neurons to be detected by the histochemicalstaining of ganglia. After inoculation of in1388 into the mousefootpad, the numbers of neurons expressing $beta$ -galactosidase increasedup to 25 days postinfection and remained constant over a further5 months. Therefore, as found with a wild-type virus containingthe IRES- $beta$ -geo construct (L $beta$ B), transgene expression was controlledby a latency-active promoter (28). The numbers of $beta$ -galactosidase-expressingneurons after inoculation with the two higher doses of in1388used were comparable to those observed in corresponding experimentsusing L $beta$ B and ear inoculation (28), although in1388 gave muchgreater consistency between mice, probably due to the absenceof virus replication at the periphery or in theganglion.

To a first approximation, in1388 established latency in the DRG with an efficiency comparable to that of a VP16 mutant (in1851),which is unable to replicate in neurons due to an insertion thatdisrupts the TK coding sequences (12), since the number of $beta$ -galactosidase-positiveneurons after inoculation with in1388 is similar to the numberof LAT-containing cells in in1851-infected mice when the sameroutes of inoculation and approximately equal titers of virusare used. Between 1 and 2% of DRG neurons (based on a value of10,000 neurons in L3, L4, and L5 DRG [12]) expressed $beta$ -galactosidaseby 25 days postinoculation, although this value underestimatesthe proportion of positive neurons in the infected population.Many DRG neurons project to parts of the limb other than the foot,and even within the foot not all nerve endings would be exposedto the inoculum. The large amount of virus that can be injectedwith apathogenic mutants can compensate to a considerable extentfor the absence of input virus amplification by replication, althoughin other studies the numbers of LAT-positive neurons were greaterthan 1 to 2% after inoculation of replication-competent HSV-1(12, 33). The absence of detectable virus in the DRG showsthat the combination of VP16, ICP0, and ICP4 mutations preventsprogression to the lytic route of infection; indeed, the VP16and ICP0 mutations together, as in in1368, are sufficient to blockreplication in the footpad and ganglion almost completely. Itappears, therefore, that in1388 genomes reaching the sensory neuronsare exclusively directed to latency and that the lytic route ofinfection is not operative. It would not be expected that thedisruption of the LAT region is an important factor affectingthe establishment of latency by in1388, since recent studies suggestthat any early functions of LATs in establishment of latency areconcerned with prevention of lytic replication, possibly by interferencewith IE gene expression and function, thereby preventing deathof neurons due to virus replication (5, 21, 32, 47, 59).In the absence of ICP0 and ICP4, infection would not proceed asfar as the expression of IE gene products and thus this propertyof LATs would not berelevant.

The results formally demonstrate that, as in cultured neurons (65), a functional ICP0 is not essential for the activityof the LAT promoter in mice, a point that has not been made previouslysince all ICP0 mutants used to date for animal latency studiesalso have all or part of LATsdeleted.

It is important to note that our studies use the activity of the LAT transcription unit as a measure of latency establishment.Reactivation has not been investigated, although this parameterof latency would be difficult to address quantitatively becausethe debilitating nature of the mutations present in the in1388genome would severely reduce virus replication once reactivationhadoccurred.

The data presented here strongly suggest that no peripheral replication is required for efficient latency establishment. Althoughwe cannot exclude the possibility that very limited replicationof in1388 occurred in the foot, the effect of progeny from suchreplication would be negligible compared with the large amountof virus delivered in the inoculum. Even with ICP4 function fullyrestored, as in in1368, viral titers in the foot declined over4 days after inoculation. If the differences in titers betweenthe two curves of Fig. 5 are considered to be a measure of theamount of new virus produced by replication of in1368, it canbe calculated that replication increased the virus load providedby the input inoculum by no more than 50%.

The establishment of latency was not detectably affected by restoration of VP16, ICP0, or ICP4 coding sequences. This observationis compatible with the view that the natural block to lytic geneexpression is at the IE level, since if later functions were required,enhancement of IE gene expression would be expected to increasethe establishment of latency. The lack of effect of VP16 was notsurprising, since previous studies have suggested that this proteindoes not function in neurons (48). Functional ICP4 repressesLAT expression during lytic infection of neurons (19), but nodifferences in the expression of $beta$ -geo by in1388 and in1368 wereobserved, again emphasizing that initiation of the lytic pathwayof infection is not operational with the mutants described here.Repair of the ICP0 deletion did not affect the establishment oflatency in our assay, showing that ICP0 is not required for theestablishment of stable, LAT-positive latency. It is importantto note, however, that our results show only the absence of majoreffects on the establishment of latency and that the variationbetween animals precludes detection of small differences betweenthe behavior ofmutants.

The finding that multiply impaired mutants establish latency efficiently and that ICP0 did not affect this process supportsthe view that latency arises when IE gene expression (or function)is insufficient to trigger the lytic cycle, as found after infectionof fibroblasts with mutants impaired for VP16, ICP0, and ICP4function (40, 45). These observations are not apparently compatiblewith the strong reduction in HSV-1 genome retention in culturedneurons when ICP0 is absent (65). It should be noted, however,that neurons in culture may produce more ICP0 than the cells invivo, because VP16 is added with the inoculum to cultures whereastransactivation is thought not to occur in the animal (48).On the other hand, the quiescent state reached by VP16, ICP0,and ICP4 triple mutants in fibroblasts appears to be analogousto latency by in1388 in vivo, differing only in expression fromthe LAT promoter, which is controlled by neuron-specific elements(2, 6, 69). The relevance of cell culture models to latencyin vivo is discussed in a recent review (42).

The experiments described here show that the advantage of long-term expression, achieved by use of the IRES- $beta$ -geo insertionin the LAT locus, can be harnessed in a multiple mutant in whichcytotoxicity and other adverse effects of IE proteins are largelyeliminated. This result provides "proof of principle" that HSV-1mutants severely impaired for the three major transactivatorscan direct long-term expression of a foreign protein under latentcontrol, provided that the appropriate construction is made inthe LAT region. Previous studies showed that the LAT promoter,when present in a wild-type HSV-1 genome, is active in centralnervous system neurons which connect to the relevant ganglionicsites after peripheral inoculation (28). The highly attenuatednature of in1388 suggests that injection of this virus into specificareas of the brain may result in long-term expression of $beta$ -galactosidase,which would represent an important advance in the developmentof therapeutically useful HSV-1vectors.

	ACKNOWLEDGMENTS

We acknowledge support from the Medical Research Council to R.H.L. and S.E.

K. R. Marshall, A. Rinaldi, and C. M. Preston are members of the Medical Research Council VirologyUnit.

	FOOTNOTES

^* Corresponding author. Mailing address: Medical Research Council Virology Unit, Church St., Glasgow G11 5JR, Scotland. Phone:44 141 330 3921. Fax: 44 141 337 2236. E-mail: c.preston{at}vir.gla.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ace, C. I., T. A. McKee, J. M. Ryan, J. M. Cameron, and C. M. Preston. 1989. Construction and characterization of a herpes simplex virus type 1 mutant unable to transinduce immediate-early gene expression. J. Virol. 63:2260-2269[Abstract/Free Full Text].

2. Batchelor, A. H., and P. O'Hare. 1992. Localization of cis-acting sequence requirements in the promoter of the latency-associated transcript of herpes simplex virus type 1 required for cell type-specific activity. J. Virol. 66:3573-3582[Abstract/Free Full Text].

3. Cai, W., and P. A. Schaffer. 1991. A cellular function can enhance gene expression and plating efficiency of a mutant defective in the gene for ICP0, a transactivating protein of herpes simplex virus type 1. J. Virol. 65:4078-4090[Abstract/Free Full Text].

4. Cai, W., T. L. Astor, L. M. Liptak, C. Cho, D. M. Coen, and P. A. Schaffer. 1993. The herpes simplex virus type 1 regulatory protein ICP0 enhances viral replication during acute infection and reactivation from latency. J. Virol. 67:7501-7512[Abstract/Free Full Text].

5. Chen, S.-H., M. F. Kramer, P. A. Schaffer, and D. M. Coen. 1997. A viral function represses accumulation of transcripts from productive-cycle genes in mouse ganglia latently infected with herpes simplex virus. J. Virol. 71:5878-5884[Abstract].

6. Chen, X., M. C. Schmidt, W. F. Goins, and J. C. Glorioso. 1995. Two herpes simplex virus type 1 latency-active promoters differ in their contributions to latency-associated transcript expression during lytic and latent infections. J. Virol. 69:7899-7908[Abstract].

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1.	Ace, C. I., T. A. McKee, J. M. Ryan, J. M. Cameron, and C. M. Preston. 1989. Construction and characterization of a herpes simplex virus type 1 mutant unable to transinduce immediate-early gene expression. J. Virol. 63:2260-2269[Abstract/Free Full Text].
2.	Batchelor, A. H., and P. O'Hare. 1992. Localization of cis-acting sequence requirements in the promoter of the latency-associated transcript of herpes simplex virus type 1 required for cell type-specific activity. J. Virol. 66:3573-3582[Abstract/Free Full Text].
3.	Cai, W., and P. A. Schaffer. 1991. A cellular function can enhance gene expression and plating efficiency of a mutant defective in the gene for ICP0, a transactivating protein of herpes simplex virus type 1. J. Virol. 65:4078-4090[Abstract/Free Full Text].
4.	Cai, W., T. L. Astor, L. M. Liptak, C. Cho, D. M. Coen, and P. A. Schaffer. 1993. The herpes simplex virus type 1 regulatory protein ICP0 enhances viral replication during acute infection and reactivation from latency. J. Virol. 67:7501-7512[Abstract/Free Full Text].
5.	Chen, S.-H., M. F. Kramer, P. A. Schaffer, and D. M. Coen. 1997. A viral function represses accumulation of transcripts from productive-cycle genes in mouse ganglia latently infected with herpes simplex virus. J. Virol. 71:5878-5884[Abstract].
6.	Chen, X., M. C. Schmidt, W. F. Goins, and J. C. Glorioso. 1995. Two herpes simplex virus type 1 latency-active promoters differ in their contributions to latency-associated transcript expression during lytic and latent infections. J. Virol. 69:7899-7908[Abstract].
7.	Clements, G. B., and N. D. Stow. 1989. A herpes simplex virus type 1 mutant containing a deletion within immediate early gene 1 is latency-competent in mice. J. Gen. Virol. 70:2501-2506[Abstract/Free Full Text].
8.	Coen, D. M., M. Kosz-Vnenchak, J. G. Jacobson, D. A. Leib, C. L. Bogard, P. A. Schaffer, K. L. Tyler, and D. M. Knipe. 1989. Thymidine kinase-negative herpes simplex virus mutants establish latency in mouse trigeminal ganglia but do not reactivate. Proc. Natl. Acad. Sci. USA 86:4736-4740[Abstract/Free Full Text].
9.	Davison, M.-J., V. G. Preston, and D. J. McGeoch. 1984. Determination of the sequence alteration in the DNA of the herpes simplex virus type 1 temperature-sensitive mutant ts K. J. Gen. Virol. 65:859-863[Abstract/Free Full Text].
10.	DeLuca, N. A., and P. A. Schaffer. 1985. Activation of immediate-early, early, and late promoters by temperature-sensitive and wild-type forms of herpes simplex virus type 1 protein ICP4. Mol. Cell. Biol. 5:558-570.
11.	Dobson, A. T., T. P. Margolis, F. Sederati, J. G. Stevens, and L. T. Feldman. 1990. A latent, nonpathogenic HSV-1-derived vector stably expresses $beta$ -galactosidase in mouse neurons. Neuron 5:353-360[CrossRef][Medline].
12.	Ecob-Prince, M. S., C. M. Preston, F. J. Rixon, K. Hassan, and P. G. E. Kennedy. 1993. Neurons containing latency-associated transcripts are numerous and widespread in dorsal root ganglia following footpad inoculation of mice with herpes simplex virus type 1 mutant In 1814. J. Gen. Virol. 74:985-994.
13.	Efstathiou, S., S. Kemp, G. K. Darby, and A. C. Minson. 1989. The role of herpes simplex virus type 1 thymidine kinase in pathogenesis. J. Gen. Virol. 70:869-879[Abstract/Free Full Text].
14.	Efstathiou, S., and A. C. Minson. 1995. Herpes virus-based vectors. Br. Med. Bull. 51:45-55[Abstract/Free Full Text].
15.	Everett, R. D. 1984. Transactivation of transcription by herpes virus products: requirement for two HSV-1 immediate-early polypeptides for maximum activity. EMBO J. 3:3135-3141[Medline].
16.	Everett, R. D. 1989. Construction and characterisation of herpes simplex virus type 1 mutants with defined lesions in immediate early gene 1. J. Gen. Virol. 70:1185-1202[Abstract/Free Full Text].
17.	Everett, R. D., P. Freemont, H. Saitoh, A. Orr, M. Kathoria, and J. Parkinson. 1998. The disruption of ND10 during herpes simplex virus infection correlates with the Vmw110- and proteasome-dependent loss of several PML isoforms. J. Virol. 72:6581-6591[Abstract/Free Full Text].
18.	Everett, R. D., A. Orr, and C. M. Preston. 1998. A viral activator of gene expression functions via the ubiquitin-proteasome pathway. EMBO J. 17:7161-7169[CrossRef][Medline].
19.	Farrell, M. J., T. P. Margolis, W. A. Gomes, and L. T. Feldman. 1994. Effect of the transcription start region of the herpes simplex virus type 1 latency-associated transcript promoter on expression of productively infected neurons in vivo. J. Virol. 68:5337-5343[Abstract/Free Full Text].
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