Three Herpes Simplex Virus Type 1 Latency-Associated Transcript Mutants with Distinct and Asymmetric Effects on Virulence in Mice Compared with Rabbits

doi:10.1128/JVI.75.19.9018-9028.2001

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Journal of Virology, October 2001, p. 9018-9028, Vol. 75, No. 19
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.19.9018-9028.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Three Herpes Simplex Virus Type 1 Latency-Associated Transcript Mutants with Distinct and Asymmetric Effects on Virulence in Mice Compared with Rabbits

Guey-Chuen Perng,¹ Daniel Esmaili,¹ Susan M. Slanina,¹ Ada Yukht,¹ Homayon Ghiasi,¹^,² Nelson Osorio,¹ Kevin R. Mott,¹ Barak Maguen,¹ Ling Jin,¹ Anthony B. Nesburn,¹^,² and Steven L. Wechsler¹^,²^,^*

Ophthalmology Research Laboratories, Cedars-Sinai Medical Center Burns & Allen Research Institute, Los Angeles, California 90048,¹ and Department of Ophthalmology, UCLA School of Medicine, Los Angeles, California 90024²

Received 9 April 2001/Accepted 14 June 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Herpes simplex virus type 1 latency-associated transcript (LAT)-null mutants have decreased reactivation but normal virulencein rabbits and mice. We report here on dLAT1.5, a mutant withLAT nucleotides 76 to 1667 deleted. Following ocular infectionof rabbits, dLAT1.5 reactivated at a lower rate than its wild-typeparent McKrae (6.1 versus 11.8%; P = 0.0025 [chi-square test]).Reactivation was restored in the marker-rescued virus dLAT1.5R(12.6%; P = 0.53 versus wild type), confirming the importanceof the deleted region in spontaneous reactivation. Compared withwild-type or marker-rescued virus, dLAT1.5 had similar or slightlyreduced virulence in rabbits (based on survival following ocularinfection). In contrast, in mice, dLAT1.5 had increased virulence(P < 0.0001). Thus, deletion of LAT nucleotides 76 to 1667 increasedviral virulence in mice but not in rabbits. In contrast, we alsoreport here that LAT2.9A, a LAT mutant that we previously reportedto have increased virulence in rabbits (G. C. Perng, S. M. Slanina,A. Yuhkt, B. S. Drolet, W. J. Keleher, H. Ghiasi, A. B. Nesburn,and S. L. Wechsler, J. Virol. 73:920-929, 1999), had decreasedvirulence in mice (P = 0.03). In addition, we also found thatdLAT371, a LAT mutant that we previously reported to have wild-typevirulence in rabbits (G. C. Perng, S. M. Slanina, H. Ghiasi, A.B. Nesburn, and S. L. Wechsler, J. Virol. 70:2014-2018, 1996),had decreased virulence in mice (P < 0.05). Thus, these threemutants, each of which encodes a different LAT RNA, have differentvirulence phenotypes. dLAT1.5 had wild-type virulence in rabbitsbut increased virulence in mice. In contrast, LAT2.9A had increasedvirulence in rabbits but decreased virulence in mice, and dLAT371had wild-type virulence in rabbits but decreased virulence inmice. Taken together, these results suggest that (i) the 5' endof LAT and/or a gene that overlaps part of this region is involvedin viral virulence, (ii) this virulence appears to have species-specificeffects, and (iii) regulation of this virulence may becomplex.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Herpes simplex virus type 1 (HSV-1) is a double-stranded neurotropic DNA virus. It is ubiquitous in the general populationand establishes lifelong latent infections in host sensory neurons.Following ocular infection, the virus travels up nerves and establisheslatent infection in neurons of the trigeminal ganglia (TG). Viaa mechanism that remains to be fully elucidated, the latent viruscan reactivate at various times throughout the life of the individualand produce recurrent disease. Recurrent HSV-1 infection in theeye can result in corneal scarring, leading to loss of vision.As a result, HSV-1 is one of the most common infectious causesof corneal blindness in the developedworld.

During neuronal latency, the latency-associated transcript (LAT) is the only viral gene that is abundantly transcribed (4,11, 27, 30, 32, 33). The primary LAT transcript is 8.3kb long (35, 40) and overlaps two viral genes, ICP0 and ICP34.5,in an antisense direction (27, 33). A very stable intron,the 2-kb LAT, is spliced from the primary transcript (9) andis the major LAT RNA detected during latency (6, 30, 31,36, 37, 39).

LAT is essential for wild-type levels of spontaneous and induced reactivation in the rabbit ocular model (12, 20). Thisfunction maps to within the first 1.5 kb of the primary LAT (22).This 1.5-kb region does not overlap ICP0 or ICP34.5, encompassesonly the first 837 nucleotides of the stable 2-kb LAT, and doesnot retain the 2-kb LAT stability (22). Thus, LAT appears toenhance spontaneous reactivation in the rabbit by a mechanismthat does not involve antisense regulation of ICP0, does not requireproduction of the 2-kb LAT, and does not require the presenceof a highly stable LAT RNA. We have recently shown that LAT canpromote cell survival in vitro and block apoptosis in rabbit TGduring acute infection (13, 19). This may increase the numberof neurons that become latently infected (25, 28, 34), therebyincreasing spontaneous reactivation by increasing the pool oflatently infected neurons available for subsequent reactivation.In some situations, it might also affect viralvirulence.

LAT-null mutants in which the LAT promoter has been deleted and no LAT RNA is detected appear to have wild-type virulencein animal models (1, 2, 12, 20, 29). This suggeststhat LAT does not play a role in viral virulence. However, werecently showed that deletion of LAT nucleotides 76 to 447 froma virus that could transcribe only the first 1.5 kb of LAT (producinga mutant designated LAT2.9A), significantly increases the deathrate in the rabbit ocular model (24). This suggests that thefirst 1.5 kb of LAT is involved in virulence as well as latency.However, the potential role of the remainder of the primary 8.3-kbLAT transcript (the region of LAT from 1.5 to 8.3 kb) has notbeenaddressed.

We describe here a LAT mutant designated dLAT1.5. This mutant has LAT nucleotides 76 to 1667 deleted but contains the entireLAT promoter and expresses the primary 8.3-kb LAT with the exceptionof the deleted region (i.e., it expresses the region of LAT from1.67 to 8.3 kb). dLAT1.5 was wild type for ocular replicationand eye disease. As expected, dLAT1.5 had reduced spontaneousreactivation compared with the parental McKrae wild-type virusor marker-rescued virus (dLAT1.5R). In rabbits dLAT1.5 had wild-typeor slightly reduced virulence (as measured by survival). In contrast,in mice, dLAT1.5 was significantly more virulent than dLAT1.5Ror wild-typevirus.

We previously reported that LAT2.9A has increased virulence in the rabbit (24). In contrast, we found here that LAT2.9Ahad reduced virulence in mice. We also previously reported thata third LAT mutant, dLAT371, has wild-type virulence in rabbits.dLAT371 contains the same 371-nucleotide deletion in the 5' endof LAT as does LAT2.9A. However, in contrast to LAT2.9A, dLAT371expresses the remainder of both copies of LAT. Thus, dLAT371 isstructurally similar to dLAT1.5 in that both mutants express bothcopies of LAT with the exception of a deletion in the 5' end.Furthermore, both deletions begin at the same StyI restrictionenzyme site. In contrast to the case for dLAT1.5, we found thatdLAT371 has decreased (rather than increased) virulence in mice.Thus, compared with wild-type virus and their corresponding marker-rescuedviruses, each of these three LAT mutants affected virulence differentlyin rabbits compared with mice. There were also differences amongthe mutants regarding in which animal model they were more virulent.These results suggest that LAT and/or a gene overlapping partof the 5' end of LAT can affect virulence and that this effectcan differ in rabbits compared with mice depending on the exactportion of LAT that isdeleted.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells and virus. Rabbit skin (RS) cells were grown in Eagle's minimal essential medium (MEM) supplemented with 5% fetal calf serum (FCS). CV-1cells were grown in MEM supplemented with 10% FCS. CV-1 cellswere used for growth kinetic studies. RS cells were used for allother tissue culture procedures, including preparation of virusstocks. All mutants were derived from HSV-1 strain McKrae. Theparental McKrae virus and all mutants were triple plaque purifiedand passaged only one or two times prior to use. The constructionand properties of dLAT2903, dLAT371, LAT3.3A, and LAT2.9A havebeen previously described (20, 22, 24). LAT3.3A was originallydesignated LAT1.5a (22), but its designation was changed (7,8, 24) to maintain nomenclature consistency with our othermutants (the number prior to the A indicates the size of the LATregion added between UL37 andUL38).

Construction of the mutant dLAT1.5. The previously cloned BamHI B fragment from HSV-1 strain McKrae (21) was digested with MluI, the overhang was filled inusing the Klenow fragment and digested with SwaI, and PacI linkerwas added. The fragment was then digested with PacI, and the productswere separated by agarose gel electrophoresis. A resulting 3.6-kbband (SwaI to MluI; LAT nucleotides $-$ 798 to +2850) which includesthe LAT promoter and the entire 2-kb LAT was isolated by electroelutionand cloned into the PacI site of plasmid pNEB193 to produce theplasmid SMpNEB193. SMpNEB193 was digested with StyI and HpaI,the StyI overhang was filled in using the Klenow fragment, andthe blunt ends were self-ligated to produce the plasmid pLAT1.5dl,which contains a deletion from LAT nucleotide 76 to 1667. pLAT1.5dlwas amplified by transformation into Escherichia coli strain RR1 $lambda$ CI857according to standard protocols (21).

dLAT1.5 was generated by homologous recombination of pLAT1.5dl with dLAT2903 as we previously described (20, 22, 23,26). dLAT2903 is a mutant of HSV-1 strain McKrae containinga 1.8-kb (EcoRV-HpaI) deletion in both copies of LAT that removed0.2 kb of the LAT promoter and 1.6 kb of the 5' end of the primary8.3-kb LAT transcript (20). Briefly, pLAT1.5dl was cotransfectedwith infectious dLAT2903 DNA by the calcium phosphate method.Viruses from the cotransfection were plated, and isolated plaqueswere picked and screened by Southern analysis. Selected plaqueswere triple plaque purified and reanalyzed by restriction digestionand Southern analysis to ensure that the LAT promoter had beenrestored and that the region from LAT nucleotide 76 to 1667 wasdeleted from both copies of LAT (one in each long repeat). A finalplaque was purified and designated dLAT1.5. The marker-rescuedvirus, dLAT1.5R, was generated as described above by homologousrecombination of dLAT1.5 DNA with the plasmid SMpNEB193. Thisrestored the deletion in dLAT1.5 back to wildtype.

Replication of virus in tissue culture. CV-1 cell monolayers at approximately 70 to 80% confluency were infected with virus at 0.01 PFU/cell, and all monolayers wererefed with exactly the same amount of MEM containing 10% FCS.Virus was harvested for titration at various times by two cyclesof freeze-thawing of the monolayers plus medium ( $-$ 80°C to roomtemperature). PFU per milliliter were determined by standard plaqueassays on RScells.

Animals. Rabbits were 8- to 10-week-old female New Zealand White from Irish Farms. Mice were 6-week-old female Swiss Webster from Harlan.Rabbits and mice were treated in accordance with Association forResearch in Vision and Ophthalmology, American Association forLaboratory Animal Care, and National Institutes of Healthguidelines.

Rabbit model of ocular HSV-1 infection, latency, and spontaneous reactivation. The McKrae strain of HSV-1 does not require corneal scarification in rabbits or mice for efficient ocular infection (20).Rabbits were bilaterally infected without scarification or anesthesiaby placing 2 × 10⁵ PFU of HSV-1 per eye into the conjunctival cul-de-sac, closingthe eye, and rubbing the lid gently against the eye for 30 s (20).At this dose of HSV-1 McKrae, virtually all of the surviving rabbitsharbor a bilateral latent HSV infection in both TG, resultingin a high group rate of spontaneous reactivation with the McKraestrain of HSV-1. In each animal group, tear films were collectedfrom five eyes, each from a different rabbit, on days 3, 5, 7,and 10 postinfection (p.i.) for acute ocular replication. Virulence(animal death) was monitored daily for up to 21 days p.i. Beginningon day 31 p.i., tear film specimens were collected daily fromeach eye for 26 days as previously described (20, 23, 26),using a nylon-tipped swab. The swab was then placed in 0.5 mlof tissue culture medium and squeezed, and the inoculated mediumwas used to infect RS cell monolayers. These cell monolayers wereobserved in a masked fashion by phase light microscopy for upto 5 days for HSV-1 cytopathic effects (CPE). All positive monolayerswere blind passaged onto fresh cells to confirm the presence ofvirus. DNA was purified from positive cultures and analyzed byrestriction enzyme digestion and Southern blotting to confirmthat the CPE was due to reactivated HSV-1 and that the reactivatedvirus was identical to the inputvirus.

Ocular infection of mice. Swiss Webster mice were bilaterally infected without scarification or anesthesia by placing 10⁶ PFU of HSV-1 per eye into the conjunctival cul-de-sac as describedfor rabbits. Tear films were collected on various days p.i. fromone eye per animal. The amount of virus in each tear film wasdetermined by standard plaque assays on RS cells. Virulence wasdetermined by survival at 21 days after ocularinfection.

Virus replication in mouse TG and brains. Mice were infected as described above and euthanized at various times p.i. The brain and TG were removed and individuallyhomogenized, debris was pelleted by low-speed centrifugation,and the amount of infectious virus in the supernatant was determinedby standard plaque assays on RScells.

Statistical analyses. Statistical analyses were performed using GraphPad Prism version 3.00 for Windows (GraphPad Software, San Diego, Calif.).Results were considered statistically significant when the P valuewas <0.05.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Genomic structures of viruses. dLAT1.5 was constructed as described in Materials and Methods. This mutant contains a deletion from LAT nucleotide 76 (a StyIrestriction enzyme site) to 1667 (a HpaI restriction enzyme site)in both copies of the LAT gene (one in each long repeat) (Fig.1D). This deletion does not alter the primary LAT promoter. Thus,dLAT1.5 transcribes the primary LAT with the exception of thedeleted region. The marker-rescued virus, dLAT1.5R, is identicalto the parental wild-type strain McKrae (Fig. 1A). Also employedin this study were the following previously described mutants.(i) dLAT2903 (20) (Fig. 1B) has LAT nucleotides $-$ 161 to 1667deleted (a region including the primary LAT promoter and a putativesecond LAT promoter sometimes called LAP2). (ii) dLAT371 (17,23) (Fig. 1C) contains a StyI-StyI restriction site fragmentdeletion in both copies of LAT (LAT nucleotides 76 to 447). TheStyI-StyI deletion in dLAT371 and the StyI-HpaI deletion in dLAT1.5begin at the same StyI site. Thus, the genomic structure of dLAT371is identical to that of dLAT1.5 except for the size of the deletionin both copies of LAT. (iii) LAT2.9A (24) (Fig. 1F) containsthe same LAT deletion as dLAT2903 (Fig. 1B) and therefore makesno LAT from the normal LAT genomic location. LAT2.9A containsan ectopic insert between UL37 and UL38 consisting of the entireLAT promoter and the first 1.5 kb of the primary LAT transcriptfrom which the same StyI-StyI region deleted in dLAT371 (Fig.1C) has been deleted. This virus therefore expresses only LATnucleotides 1 to 76 plus 447 to 1499. (iv) LAT3.3A (22) (Fig.1E), from which LAT2.9A was derived, is included here for clarity.This mutant, originally designated LAT1.5a, was renamed to maintainconsistency with some of our other mutants. The 3.3 in the designationrefers to the approximate size, in kilobases, of the ectopic insert.

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FIG. 1. Genomic structures of the viruses used in this study. (A) Prototypic genomic structure of parental wild-type McKrae and marker-rescued viruses dLAT1.5R, dLAT2903R, and dLAT371R. TRL and IRL, terminal and internal long repeats, respectively; TRS and IRS, terminal and internal short repeats, respectively; UL and US, long and short unique regions, respectively. The LAT gene is located in the viral long repeats and is thus present in two copies. The primary 8.3-kb LAT transcript is shown expanded below the genome. The stable 2-kb LAT is indicated by a black rectangle. The relative locations of the ICP0 and ICP34.5 transcripts are shown for reference. (B) dLAT2903 (20) has an EcoRV-to-HpaI restriction fragment deletion from LAT nucleotide $-$ 161 to +1667 relative to the start of LAT transcription at +1 (XXXX). This deletion removes the core LAT promoter, including the TATA box, and a second proposed promoter near the 5' end of the 2-kb LAT. No LAT is transcribed, as indicated by the dashed lines. (C) dLAT371 has a 371-nucleotide StyI-StyI restriction fragment deletion from LAT nucleotide 76 to 447 (X) in both copies of LAT (23). The primary LAT promoter is intact, and the remaining portion of the primary 8.3-kb LAT is transcribed. (D)dLAT1.5 has a StyI-to-HpaI restriction fragment deletion from LAT nucleotide 76 to 1667 (XXX). The primary LAT promoter is intact, and the remaining portion of the primary 8.3-kb LAT is transcribed. (E) LAT3.3A (22) contains the LAT promoter driving the first 1,499 nucleotides of LAT inserted into an ectopic location between the UL37 and UL38 viral genes of dLAT2903. This virus transcribes only the first 1.5 kb of LAT yet has wild-type spontaneous reactivation. LAT2.9AR (24) was marker rescued from LAT2.9A and has the same genomic structure as LAT3.3A. (F) LAT2.9A (24) has the same genomic structure as LAT3.3A except for a StyI-StyI restriction fragment deletion from LAT nucleotide 76 to 447 in the ectopic LAT insert.

Spontaneous reactivation. Rabbit eyes were infected with 2 × 10⁵ PFU of dLAT1.5, dLAT1.5R, or wild-type McKrae per eye as described in Materials andMethods. Starting at 31 days p.i., at which time latency had alreadybeen established, tear films were collected daily from all eyesand individually plated on indicator cells (RS cells) to detectspontaneously reactivated virus. Southern analysis of spontaneouslyreactivated viruses grown from tear films (not shown) confirmedthat all cultures which scored positive based on the presenceof viral CPE contained reactivated virus and that the spontaneouslyreactivated dLAT1.5 virus retained the deletion in both copiesof LAT. The cumulative number of virus-positive tear film culturesper eye during 26 days for each virus are shown in Fig. 2A. Wild-typeMcKrae and dLAT1.5R appeared to have similar average cumulativespontaneous reactivation rates of approximately three positivecultures per eye on day 26 of collection. In contrast, dLAT1.5appeared to have a lower average spontaneous reactivation rateof approximately 1.6 positive cultures per eye.

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FIG. 2. Spontaneous reactivation of dLAT1.5. Rabbits were ocularly infected with dLAT1.5 (dL1.5), marker-rescued dLAT1.5R (dL1.5R), or parental wild-type (wt) McKrae. Beginning on day 31 p.i., at which time latency had been established, tear films were collected daily for 26 days, plated on RS cells, and observed for the presence of CPE. Randomly selected positive cultures were confirmed by passage and Southern analysis. (A) The y axis represents the cumulative number of HSV-1-positive cultures for each virus group divided by the number of eyes in the group. (B) The percentage of tear films containing spontaneously reactivated virus was calculated for each individual eye. The results are shown as a scattergram. In the dLAT1.5 column, some of the zero points are plotted at 0.7 so that all of the zero points can be visualized. Similarly, in the dLAT1.5R column, two points with an actual value of 7.7 are plotted at 8.4. The P values shown were determined by one-way ANOVA and Dunnet's posttest. Results for the wild type and dLAT1.5R were similar (P > 0.05).

A statistical analysis of positive (spontaneously reactivated) tear film cultures versus total cultures is shown in Table1. Approximately 6.1% of the tear films from rabbits latentlyinfected with dLAT1.5 contained spontaneously reactivated virus.This was significantly less than the results for wild-type McKrae(11.8%) and dLAT1.5R (12.6%). Because the above analyses do nottake into account the number of eyes in each group, we calculatedthe percentage of time that each eye in each group was positivefor spontaneous reactivation (i.e., the percentage of virus- positivecultures) and plotted the results as scattergrams (Fig. 2B). Thisanalysis is considered more stringent because it takes into accountboth the number of eyes and the period of time in a single calculation(22-24). By this analysis spontaneous reactivation of dLAT1.5 wasalso significantly reduced compared with those of the wild-typeand marker-rescued viruses (P < 0.01). The above analyses indicatedthat spontaneous reactivation of dLAT1.5 was reduced comparedwith those of its marker-rescued virus and wild-type virus.

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TABLE 1. Spontaneous reactivation of dLAT1.5^a

Survival following ocular dLAT1.5 infection. Survival in the rabbits used for the above-described spontaneous reactivation study was quantitated at 21 days p.i. (Fig.3A). Although not statistically significant, there was a suggestionin this experiment of increased survival in the rabbits infectedwith dLAT1.5 (60%) compared with marker-rescued dLAT1.5R (45%)and wild-type McKrae (41%). Thus, it was of interest to determineif significant differences might be seen with larger numbers ofanimals. Due to difficulties with using large numbers of rabbits,we decided to examine survival in mice. Groups of 104 mice wereinfected with 10⁶ PFU of dLAT1.5 or dLAT1.5R per eye. Surprisingly, instead ofthe expected decrease in virulence, in mice dLAT1.5 was significantlymore virulent than dLAT1.5R (Fig. 3B) (43% survival compared with71% survival; P < 0.0001 [chi-square test]). In a separate experiment(see Fig. 9 below) the virulence of dLAT1.5R in mice was similarto that of the original wild-type parental virus (P = 0.39). Thus,as judged by survival of mice following ocular HSV-1 challenge,dLAT1.5 was more virulent than either wild-type virus or its marker-rescuedvirus.

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FIG. 3. Survival of rabbits (A) and mice (B) infected with dLAT1.5. (A) Survival of the rabbits used in the experiments shown in Fig. 2 was determined on day 21 p.i. The numbers above each bar indicate the number of surviving rabbits/total number of rabbits infected. P was determined by the chi-square test for all pairs of rabbits. dL1.5, dLAT1.5; dL1.5R, dLAT1.5R; wt, parental wild-type McKrae. (B) Mice were bilaterally ocularly infected with 10⁶ PFU/eye without scarification, and survival was determined at 21 days p.i.

Replication of dLAT1.5 in tissue culture, eyes, TG, and brains. CV-1 cell monolayers were infected at a multiplicity of infection of 0.01 PFU/cell, and the kinetics of replication were determinedas described in Materials and Methods. Replication of dLAT1.5was indistinguishable from that of dLAT1.5R, wild-type virus,or the LAT-null mutant dLAT2903 (Fig. 4A). Rabbits were infectedwith 2 × 10⁵ PFU/eye. Tear films were collected from five rabbit eyes on days3, 5, 7, and 10 p.i. Figure 4B shows the average amount of virusdetected in the eye swabs at each time point. Although replicationof dLAT1.5 appeared to be slightly less than that of dLAT1.5Ror the wild type in rabbit eyes on day 5 p.i., the differenceswere not significant (P > 0.05 at all time points by analysisof variance [ANOVA]). In addition, the peak virus titers (day5 p.i. for the wild type and dLAT1.5R; day 7 for dLAT1.5) appearedto be very similar for all three viruses (P = 0.8).

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FIG. 4. Replication of dLAT1.5 in tissue culture, eyes, TG, and brains. (A) Semiconfluent monolayers of CV-1 cells were infected with 0.01 PFU of dLAT1.5, dLAT1.5R, the LAT-null mutant dLAT2903, or wild-type (wt) McKrae. At the indicated times, the infected-cell monolayers were harvested by freeze-thawing, and the amount of virus was determined by plaque assay on RS cells. The result for each time point is the average of two determinations. (B) Rabbits were ocularly infected with 2 × 10⁵ PFU of the indicated virus per eye as described in Materials and Methods. In each group tear films were collected from five individual eyes (each from a different rabbit) on days 3, 5, 7, and 10, and virus titers were determined by standard plaque assays. There was no statistical difference between the groups on any day (by ANOVA, P = 0.69 for day 3, P = 0.055 for day 5, P = 0.76 for day 7, and P = 0.84 for day 10). (C) Mice were ocularly infected as described above, and virus replication in the eye was determined as for rabbits in panel B. Results from two independent experiments are shown. Experiment 1 (six eyes per group) compared dLAT1.5 to dLAT1.5R. Experiment 2 (five eyes per group) compared the wild type to dLAT1.5R. There was no statistical difference between the viruses in each experiment on any day (P > 0.2 for experiment 1; P > 0.5 for experiment 2 [Mann-Whitney test]). (D) Mice were infected as described above. Both TG were removed from five mice per group at necropsy on days 2, 3, 5, 7, and 10 p.i., and the amount of infectious virus in each individual TG was determine by plaque assay as described in Materials and Methods. There was no statistical difference on any day (P > 0.1 on each day [ANOVA]). (E) Mice were infected as described above, and brains (five per group per time point) were harvested and virus titers were determined on the days indicated. The asterisk indicates the only day for which statistical significance was obtained (day 5, P = 0.013 [ANOVA]; dLAT1.5 versus dLAT1.5R, P = 0.02 [Mann-Whitney test]; dLAT1.5 versus wild type, P = 0.008 [Mann-Whitney test]). (F) The experiment in panel E was repeated for dLAT1.5 and dLAT1.5R using 10 mice per group on day 5 p.i. Each data point represents the virus titer from an individual brain on this day. The horizontal lines indicate the medians. The P value was determined by the Mann-Whitney rank sum test. (G) The experiment in panel E was repeated for dLAT1.5 (9 mice) and dLAT1.5R (10 mice) on day 7 p.i., and the results are plotted as in panel F. Error bars indicate standard deviations.

Mice were infected with 10⁶ PFU/eye, and replication in eyes was examined. Figure 4C shows the results of two independent experiments.In experiment 1, ocular replication of dLAT1.5 and dLAT1.5R weresimilar (P > 0.23 at each time point). In experiment 2, the wildtype and dLAT1.5R were similar (P > 0.53 at each time point).Thus, replication of dLAT1.5 in mouse eyes was similar to thatof its marker-rescued virus, which in turn was similar to thatof the original parental wild-type virus. Thus, alterations indLAT1.5 virulence (death rate) did not appear to be due to alteredocularreplication.

For analysis of replication in mouse TG, five mice per group were ocularly infected for each time point shown (Fig. 4D), andthe amount of infectious virus was determined individually foreach TG at each time point. There was no significant differenceamong the dLAT1.5, dLAT1.5R, and wild-type viruses at any timepoint (P > 0.1 [ANOVA]). The amounts of virus in the brains ofthe same mice were similarly determined. On day 5 p.i. (Fig. 4E),the average amount of virus in the brains of mice infected withdLAT1.5 was significantly higher than that of either dLAT1.5Ror the wild type (P = 0.005 [ANOVA]). On day 7 p.i., the day ofpeak virus titer in the brain, the amount of dLAT1.5 detectedwas 3.5- to 10-fold higher than that of dLAT1.5R or the wild type.However, this difference did not reach statistical significance(P = 0.1 [ANOVA]), perhaps because only five mice were used pertime point. To increase the statistical power, additional experimentswere performed using 9 or 10 mice per group. (Fig. 4F and G).On both days 5 and 7 p.i. significantly more virus was detectedin the brains of dLAT1.5-infected mice than in those of dLAT1.5R-infectedmice (P = 0.009 and P = 0.04, respectively [Mann-Whitney ranksum test]). Thus, it appears that dLAT1.5 grew more efficientlyin mouse brains than its marker-rescued virus or wild-type virus.This was consistent with the increased virulence of dLAT1.5 inmice and suggests that the increased virulence in mice may havebeen due to increased virus load in the brain. Replication ofdLAT1.5 in rabbit TG or brain was not examined both because thisvirus did not have significantly altered virulence in rabbitsand because these analyses are highly variable in therabbit.

Virulence of LAT2.9A in mice. LAT3.3A (Fig. 1E) was constructed by inserting the LAT promoter and the first 1.5 kb of LAT into an ectopic location in theLAT-null mutant dLAT2903. This virus, which expresses just thefirst 1.5 kb of LAT, has wild-type virulence in rabbits (22)and mice (unpublished results). The LAT2.9A genome is structurallyidentical to that of LAT3.3A, with the exception of a 371-nucleotidedeletion between LAT nucleotides 76 and 447 in the ectopic insert.We previously showed that LAT2.9A has increased virulence in rabbits(24). Because of the difference in virulence found above fordLAT1.5 in mice compared with rabbits, it was of interest to examinethe virulence of LAT2.9A in mice, since to our knowledge, thisis the only other LAT mutant reported to have altered virulence.Groups of 104 mice were therefore bilaterally ocularly infectedwith 10⁶ PFU/eye, and survival was determined on day 21 p.i. (Fig 5).LAT2.9A had significantly reduced virulence in mice compared withwild-type virus (P = 0.03). As shown below (see Fig. 9), the marker-rescuedvirus LAT2.9AR (24) and wild-type virus had similar virulencein mice (P = 0.19). Taken together, these two results indicatethat LAT2.9A had reduced virulence in mice compared with bothwild-type virus and its marker-rescued virus. Thus, as judgedby the ability to kill animals following ocular infection, LAT2.9Ahad decreased virulence in mice and increased virulence in rabbits,while dLAT1.5 had increased virulence in mice but wild-type orslightly decreased virulence in rabbits.

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FIG. 5. Virulence of LAT2.9A in mice. Mice were ocularly infected as described for Fig. 4, and survival was determined at 21 days p.i. Numbers above each bar indicate the number of surviving mice/total number of mice. P was determined by the chi-square test. wt, wild type.

Replication of LAT2.9A. We previously showed that replication of LAT2.9A in tissue culture and in rabbit eyes was similar to that of wild-type virus,suggesting that the increased virulence of LAT2.9A in rabbitsis not due to enhanced replication (24). Replication in rabbitTG and brain was not examined because of problems with high variability,as mentioned above. To determine if the decreased virulence ofLAT2.9A in mice might be related to decreased replication of thevirus in mice, we examined replication in mouse eyes, TG, andbrain. Mice were infected and replication was determined as describedabove for dLAT1.5, using either five eyes, five TG, or five brainsper time point per group. The replication kinetics of LAT2.9Awere indistinguishable from those of wild-type virus in the eyes,TG, and brains of mice (Fig. 6A, B, and C) (P > 0.05 at each timepoint). For further confirmation, 10 eyes, 10 TG, or 10 brainswere similarly analyzed on the day of peak virus titer as determinedfrom these results (Fig. 6D, E, and F). Again, no differenceswere detected (P > 0.05). Thus, the decreased virulence of LAT2.9Ain mice did not appear to be a result of decreased virus load.Since replication of LAT2.9A was indistinguishable from that ofwild-type virus, there was no need to compare replication of LAT2.9Awith that of its marker-rescued virus.

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FIG. 6. Replication of LAT2.9A in mouse eyes, TG, and brains. (A, B, and C) Experimental procedures and analyses were as described for Fig. 4C, D, and E, respectively, except that 10 samples were used per group at each time point. The P value was >0.05 at all time points. (D, E, and F) Scatterplots showing the virus titers for individual eyes, TG, and brains on the day of peak virus titer for the samples shown in panels A, B, and C, respectively. The horizontal lines indicate the median (as opposed to the means shown in panels A, B, and C). Error bars indicate standard deviations.

Virulence of dLAT371 in mice. dLAT371 contains the same StyI-StyI restriction fragment deletion (LAT nucleotides 76 to 447) as LAT2.9A. Like dLAT1.5, dLAT371contains a deletion starting at LAT nucleotide 76 in both copiesof the otherwise unaltered LAT gene. The only difference betweenthe structures of dLAT1.5 and dLAT371 is the size of the deletion(1,591 nucleotides for dLAT1.5 versus 371 nucleotides for dLAT371).Although LAT2.9A contains the same deletion as dLAT371, LAT2.9Acontains only one copy of LAT, the LAT is in an ectopic location,and LAT2.9A transcribes LAT only up to LAT nucleotide 1499. Thus,although we have previously shown that dLAT371 has wild-type virulencein rabbits, it was of interest to examine the virulence of dLAT371inmice.

As done above with dLAT1.5 and LAT2.9A, 104 mice per group were infected with 10⁶ PFU of dLAT371, dLAT2903, or dLAT2903R per eye. dLAT2903 is aLAT-null mutant, and dLAT2903R is its marker-rescued virus (Fig.1A and B) (20). This particular combination of mutants was usedbecause this experiment was originally aimed at comparing dLAT371with the LAT-null mutant. dLAT371 had reduced virulence comparedwith either dLAT2903 or dLAT2903R (20) (Fig. 7) (P = 0.0004and P = 0.008, respectively [chi-square] test). As shown below(see Fig. 9), in mice the virulences of dLAT2903R and dLAT371R(marker-rescued dLAT371) were both similar to that of the wildtype (P = 0.19 and P = 0.68, respectively). Thus, consistent withLAT2.9A, but in contrast to dLAT1.5, in mice, dLAT371 was lessvirulent than wild-type virus or its marker-rescued virus.

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FIG. 7. Virulence of dLAT371 in mice. Mice were ocularly infected and survival was determined as described for Fig. 4. P was determined by the chi-square test. dL371, dLAT371; dLAT, dLAT2903; dLATR, dLAT2903R.

Replication of dLAT371. We previously reported that replication of dLAT371 was indistinguishable from that of wild-type virus in tissue culture andin rabbit eyes. The kinetics of replication of dLAT371 in mouseeyes, TG, and brain were examined, using 10 samples per time pointper group (Fig. 8A, B, and C). Scattergrams are also shown forthe day of peak replication at each site (Fig. 8D, E, and F).Although dLAT371 appeared to grow slightly less well than wild-typevirus in mouse eyes (P = 0.043 on day 3 p.i. [Mann-Whitney ranksum test]), replication of dLAT371 in mouse TG and brains wasindistinguishable from that of wild-type virus (P > 0.05 for alltimes and P = 0.74 and P = 0.68, respectively, for peak titers).Thus, it appears unlikely that decreased replication of dLAT371in mouse brains could account for the decreased virulence of thismutant in mice. Since replication of dLAT371 in TG and brainswas wild type, comparisons with dLAT371R were not made.

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FIG. 8. Replication of dLAT371 (d371) in mouse eyes, TG, and brains. Experimental procedures and analyses were done as described in the legend to Fig. 6. The P value was >0.05 by the Mann-Whitney rank sum test at all time points except for mouse eyes on day 3. By the Student t test, the P value was 0.13 for this time point. wt, wild type. Error bars indicate standard deviations.

Virulence of marker-rescued viruses. Groups of mice were ocularly infected as described above, and virulence was determined based on survival on day 21 p.i. Thevirulences of dLAT1.5R, LAT2.9AR, dLAT371R, and dLAT2903R wereall indistinguishable from that of wild-type McKrae (Fig. 9) (P> 0.05).

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FIG. 9. Virulence of marker-rescued viruses in mice. Mice were ocularly infected as described for Fig. 4, and survival was determined at 21 days p.i. The numbers above each bar represent the number of surviving mice/total number of mice. The P value in the box was determined by the chi-square test using a 5-by-2 contingency table. The P values above individual bars were determined by the chi-square test compared with the wild type. wt, wild-type McKrae; dL15R, marker-rescued dLAT1.5; dLATR, marker-rescued dLAT2903; dL371R, marker-rescued dLAT371; LAT2.9R, marker-rescued LAT2.9A.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The virulence results presented here can perhaps be most simply summarized by separating the mouse and rabbit data. Thus,in mice, compared with wild-type virus and marker-rescued viruses(all of which had wild-type virulence), dLAT1.5 had increasedvirulence, while LAT2.9A and dLAT371 had decreased virulence.In rabbits, compared with wild-type and marker-rescued viruses,LAT2.9A had increased virulence, dLAT371 had wild-type virulence,and dLAT1.5 had wild-type or slightly reducedvirulence.

LAT is essential for wild-type levels of spontaneous reactivation in the rabbit ocular model. We previously showed that expressionof just the first 1.5 kb of the 8.3-kb LAT, as found in LAT3.3A,is sufficient for wild-type levels of spontaneous reactivation(22). Thus, a major function involved in spontaneous reactivationin the rabbit maps to within the first 1.5 kb of LAT, a regionrepresenting less than 20% of the primary LAT transcript. dLAT1.5was constructed and studied in this work because it representsa mutant complementary to LAT3.3A. Thus, while LAT3.3A expressesonly the first 1.5 kb of LAT, dLAT1.5 expresses all of LAT exceptfor a similar region (LAT nucleotides 76 to 1667). As expected,like the LAT-null mutant dLAT2903, dLAT1.5 had reduced spontaneousreactivation. This demonstrated that in the rabbit ocular model,not only is the first 1.5 kb of LAT sufficient for wild-type spontaneousreactivation, but part or all of the first 1.5 kb is also requiredfor wild-type levels of spontaneous reactivation. In addition,these results suggest that LAT does not contain a region outsideof the first 1.67 kb of LAT that is independently able to supportwild-type levels of spontaneous reactivation

We previously showed that compared with wild-type virus, LAT2.9A (Fig. 1E) has increased virulence in rabbits (i.e., increaseddeath rate following ocular infection) compared with marker-rescuedor wild-type virus (24). In contrast, as reported here, in miceLAT2.9A was significantly less virulent than marker-rescued orwild-type virus. Thus, the virulence phenotype for LAT2.9A notonly appeared to be very different in mice compared with rabbits,it appeared to be asymmetric in rabbits compared with mice (i.e.,more virulent than the wild type in one species and less virulentthan the wild type in anotherspecies).

Note that in this report we use the term virulence to mean death following ocular infection. We are not distinguishing betweenneuroinvasiveness (the ability of the virus to get to the brainfollowing infection at a peripheral site) and neurovirulence (theability of the virus to kill the animal once it reaches thebrain).

We also showed in this report that following ocular infection of rabbits, dLAT1.5 had virulence similar to or slightly lessthan that of wild-type virus or marker-rescued dLAT1.5R. In contrast,in mice, dLAT1.5 was significantly more virulent than the wildtype or dLAT1.5R. Thus, the virulence phenotype for dLAT1.5 alsoappeared to differ in mice compared with rabbits. The asymmetricvirulence results in mice versus rabbits with LAT2.9A and dLAT1.5were unexpected. Although mutations that alter the virulence ofHSV-1 in mice but not rabbits have been reported (38), we arenot aware of any previous report of a mutant that is more virulentthan its marker-rescued and parental wild-type viruses in oneanimal species and less virulent than its marker-rescued and parentalwild-type viruses in a secondspecies.

Also surprising was that dLAT1.5 and LAT2.9A had opposite phenotypes. That is, compared with wild-type virus and the mutant-specificmarker-rescued virus, one mutant had decreased virulence in micewhile the other mutant had increased virulence in mice, and viceversa in rabbits. This is of particular interest, because bothof these viruses contain deletions of part of the LAT gene. Themost direct conclusion to draw from these results is that differentLAT deletion mutants can affect virulence differently and thatthe direction of virulence (i.e., increased or decreased comparedwith the wild type) can differ in mice versus rabbits. This inturn strongly suggests that in addition to being involved in theHSV-1 latency cycle of establishment of and reactivation fromlatency, LAT is also involved in viralvirulence.

Because dLAT1.5 and LAT2.9A have significant genomic structural differences in addition to the size of the LAT deletion beginningat LAT nucleotide 76, it was of interest to also examine the virulenceof a third LAT mutant, dLAT371 (23). All three of these mutants(dLAT1.5, LAT2.9A, and dLAT371) contain a deletion starting atLAT nucleotide 76 (Fig. 1). dLAT371 and dLAT1.5 have identicalgenomic structures except for the size of the deletion (371 versus1,591 nucleotides). In contrast, LAT2.9A and dLAT371 have significantlydifferent genomic structures (Fig. 1C and F) but contain identical371-nucleotide deletions in LAT. Consistent with LAT2.9A, butin contrast to dLAT1.5, dLAT371 had reduced virulence in mice.Thus, in mice, the larger 1,591-nucleotide deletion in dLAT1.5resulted in increased virulence, while the smaller 371-nucleotidedeletion in dLAT371 and LAT2.9A resulted in decreasedvirulence.

We previously reported that dLAT371 has wild-type virulence and wild-type spontaneous reactivation in rabbits (23). Thisis in contrast to LAT2.9A, which has increased virulence and decreasedspontaneous reactivation in rabbits. Since these mutants haveidentical deletions in the 5' end of LAT, the phenotypic differencesin rabbits appear to be due to either (i) the lack of LAT nucleotides1500 to 8324 in LAT2.9A, (ii) undetected differences in LAT expressionor stability in LAT2.9A compared with dLAT371, (iii) the singlecopy of LAT in LAT2.9A, or (iv) the ectopic location of LAT inLAT2.9A. However, we think that the ectopic location and the singleLAT copy are unlikely possibilities, since LAT3.3A and LAT2.9AR,which contain the same single-copy ectopic insert but withoutthe 371-nucleotide deletion, both have wild-type virulence andwild-type spontaneousreactivation.

HSV-1 kills rabbits and mice by causing encephalitis. In this study, virulence refers to this encephalitic death followingocular infection. In a simple model, the relative level of HSV-1virulence would be expected to be directly related to the virusload in the brain. That is, if there was more virus in the brain,there would be more encephalitic death. For dLAT1.5 in mice, thissituation appeared to hold. dLAT1.5 was more virulent in micethan its marker-rescued virus, and the amount of dLAT1.5 in mousebrains was significantly increased compared with that of its marker-rescuedvirus. In contrast, this model did not appear to hold for LAT2.9Aor dLAT371 in mice. These mutants had reduced virulence in mice,yet the viral load in the brain was the same as that of wild-typevirus. This strongly suggests, and supports a previous report(15), that the virus load in the brain is not always a goodpredictor of neurovirulence for HSV-1.

LAT may partially inhibit productive gene expression (3, 10, 18). In addition, it has been proposed that a 0.7-kb transcriptbeginning and terminating just upstream of the LAT promoter affectsviral virulence (38). Both of these findings suggest that deletionof the LAT promoter in LAT-null mutants might alter virulence.However, we are not aware of any reports of a LAT-null mutantwith altered virulence (1, 5, 14, 16, 20). We have,however, previously reported that LAT2.9A has increased virulencein rabbits (24). Thus, although complete lack of LAT expression(see Fig. 1B) does not appear to alter virulence, expression ofjust specific portions of LAT, as in LAT2.9A (Fig. 1F), dLAT371(Fig. 1C), and dLAT1.5 (Fig. 1D), can alter virulence. Thus, wehave a situation in which a large deletion (i.e., LAT-null mutants,which have no LAT promoter and which are therefore equivalentto deletion of the entire gene) has no impact on virulence, whilesmaller deletions which are encompassed by the larger deletion(those in LAT2.9A, dLAT371, and dLAT1.5) do alter virulence. Aswe previously speculated in regard to LAT2.9A (24), this situationis similar to that seen in promoter-mapping studies. Because promotersusually have multiple functional elements that may work eitherin concert or antagonistically, deletion of increasingly largerportions of the 5' end of a promoter often produces multiple increasesand decreases in promoter activity. The situation with LAT2.9A,dLAT371, and dLAT1.5 is analogous. These different deletions produceddifferent increases and decreases in virulence, suggesting thatLAT may have multiple functional elements. Since LAT may not encodea protein (8), it is possible that the LAT RNA may directlyor indirectly regulate the expression or function of viral and/orcellular genes that in turn influence virulence. In this case,the different deletions may alter the LAT RNA structure or stability,which in turn affects the LAT RNAfunction.

Finally, the results presented here strongly suggest that LAT has multiple functions, since it affects both virulence andspontaneousreactivation.

	ACKNOWLEDGMENTS

This work was supported by Public Health Service grants EY07566, EY11629, and EY12823; the Discovery Fund for Eye Research;and the Skirball Program in MolecularOphthalmology.

We thank Anita Avery for her expert technical support and Steven J. Robbins for productivediscussions.

	FOOTNOTES

^* Corresponding author. Mailing address: Ophthalmology Research Laboratories, Cedars-Sinai Medical Center Burns & Allen ResearchInstitute, Davis Bldg., Room 5072, 8700 Beverly Blvd., Los Angeles,CA 90048. Phone: (310) 423-6457. Fax: (310) 423-0225. E-mail:Wechsler{at}csmc.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Mott, K. R., Osorio, N., Jin, L., Brick, D. J., Naito, J., Cooper, J., Henderson, G., Inman, M., Jones, C., Wechsler, S. L., Perng, G.-C. (2003). The bovine herpesvirus-1 LR ORF2 is critical for this gene's ability to restore the high wild-type reactivation phenotype to a herpes simplex virus-1 LAT null mutant. J. Gen. Virol. 84: 2975-2985 [Abstract] [Full Text]
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Perng, G.-C., Maguen, B., Jin, L., Mott, K. R., Kurylo, J., BenMohamed, L., Yukht, A., Osorio, N., Nesburn, A. B., Henderson, G., Inman, M., Jones, C., Wechsler, S. L. (2002). A Novel Herpes Simplex Virus Type 1 Transcript (AL-RNA) Antisense to the 5' End of the Latency-Associated Transcript Produces a Protein in Infected Rabbits. J. Virol. 76: 8003-8010 [Abstract] [Full Text]
Perng, G.-C., Maguen, B., Jin, L., Mott, K. R., Osorio, N., Slanina, S. M., Yukht, A., Ghiasi, H., Nesburn, A. B., Inman, M., Henderson, G., Jones, C., Wechsler, S. L. (2002). A Gene Capable of Blocking Apoptosis Can Substitute for the Herpes Simplex Virus Type 1 Latency-Associated Transcript Gene and Restore Wild-Type Reactivation Levels. J. Virol. 76: 1224-1235 [Abstract] [Full Text]

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