Herpes Simplex Virus ICP0 Mutants Are Hypersensitive to Interferon

doi:10.1128/JVI.74.4.2052-2056.2000

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Journal of Virology, February 2000, p. 2052-2056, Vol. 74, No. 4
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Herpes Simplex Virus ICP0 Mutants Are Hypersensitive to Interferon

Karen L. Mossman, Holly A. Saffran, and James R. Smiley^*

Department of Medical Microbiology & Immunology, University of Alberta, Edmonton, Alberta, Canada T6G 2H7

Received 5 October 1999/Accepted 18 November 1999

	ABSTRACT

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Interferon (IFN) is an important immune system molecule capable of inducing an antiviral state within cells. Herpes simplexvirus type 1 (HSV-1) replication is somewhat reduced in tissueculture in the presence of IFN, presumably due to decreased viraltranscription. Here, we show mutations that inactivate immediate-early(IE) gene product ICP0 render HSV-1 exquisitely sensitive to IFNinhibition, resulting in greatly decreased levels of viral mRNAtranscripts and the resulting polypeptides and a severe reductionin plaque formation ability. Mutations in other HSV-1 genes, includingthe genes coding for virion transactivator VP16 and the virionhost shutoff protein vhs, IE gene ICP22, and the protein kinaseUL13 gene, do not increase the IFN sensitivity of HSV-1. Interestingly,ICP0 mutants demonstrate the same level of sensitivity to IFNas wild-type virus on U2OS cells, an osteosarcoma cell line thatis known to complement mutations in ICP0 and VP16. Thus, in somecell types, functional ICP0 is required for HSV-1 to efficientlybypass the inhibitory effects of IFN in order to ensure its replication.The significance of this link between ICP0 and IFN resistanceisdiscussed.

	TEXT

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Interferon (IFN) was initially characterized as a soluble factor mediating viral interference (21). Although it is now clearthat both alpha/beta IFN (IFN- $alpha$ / $beta$ ) and gamma IFN (IFN- $gamma$ ) IFNsare potent and pleiotropic immune modulators, antiviral defenseis likely the major function of the alpha/beta IFNs (17). TheIFN-induced cellular antiviral response is the primary defensemechanism against viral infection, and many viruses have thereforeevolved strategies to bypass the inhibitory effects of IFN (reviewedin references 22 and 24). Members of the poxvirus family interceptIFN ligand molecules prior to cell-surface receptor engagementby producing IFN receptor decoys, thus preventing IFN signal transduction(3, 38). Human cytomegalovirus also perturbs IFN signal transduction,by decreasing the levels of two key components, JAK1 and p48 (35).Several IFN-induced pathways contribute to the intracellular antiviralresponse; however, the double-stranded RNA-dependent protein kinasePKR appears to be among the most effective (8). Accordingly,each step in the PKR pathway has been shown to be subject to negativeregulation by a variety of RNA and DNA viruses (16).

While IFN severely inhibits the replication of several viruses, such as vesicular stomatitis virus (VSV) (31), replicationof herpes simplex virus type 1 (HSV-1) is only marginally reducedin cultured cells (28, 29, 41). However, in vivo studieswith IFN receptor-null mice and a variety of HSV-1 mutants illustratedthe importance of IFN- $alpha$ / $beta$ s in controlling early acute infectionin intact animals and demonstrated a role for host factors indefining the phenotype of several HSV-1 mutants (27). HSV-1is a large enveloped DNA virus that replicates in the nuclei ofmammalian cells. HSV genes are transcribed by host RNA polymeraseII in a regulatory cascade in which three distinct classes ofgenes (immediate-early [IE], early, and late) are sequentiallyactivated in a defined temporal sequence (20, 47). Five IEgenes are transcribed first, and four of these encode regulatoryproteins (ICP0, -4, -22, and -27) that drive progression to theearly and late phases of infection. Transcription of the IE genesis activated by the virion protein VP16, a 65-kDa phosphoproteinfound within the HSV-1 tegument that contains a potent C-terminalacidic transcriptional activation domain (44).

Preliminary studies suggested that IFN or its inducers can specifically target HSV-1 translation (2, 29), while subsequentinvestigations showed that IFN treatment decreases IE gene transcription(36, 42, 43). IE transactivation is a major function ofVP16; thus, it was initially believed that IFN blocks IE geneexpression by interfering with the function of VP16 (10, 25).However, experiments with a VP16 activation mutant, in1814, demonstratedthat inhibition of IE gene expression by IFN- $alpha$ is VP16 independent(41). Relatively little is known concerning the mechanisms involved,although a recent study shows that the effects vary with bothIFN and cell type (51).

To date, no studies have explored the basis for the relatively IFN-resistant phenotype established by HSV-1 in cell culture.While the late gene products $gamma$ ₁34.5 and US11 have been implicatedin the inhibition of PKR activity (6, 18, 19, 37, 45),no direct link between these proteins and resistance to IFN hasbeen established. To determine whether the relative resistanceof HSV-1 to IFN depends on a specific regulatory protein, we examinedthe effects of mutations that alter known regulatory proteinson the sensitivity to IFN- $alpha$ in a plaque reduction assay. For technicalreasons, our initial screen was limited to viral regulatory geneproducts that are dispensable for virus replication in tissueculture.

Control and IFN- $alpha$ -pretreated monolayers of Vero cells were infected with serial dilutions of wild-type HSV-1 strains KOS and17syn+, and mutants of these strains bearing lesions in the genesencoding IE proteins ICP0 and IC22, the virion transactivatorVP16, the predicted protein kinase encoded by the UL13 gene, andthe virion host shutoff protein (vhs) encoded by the UL41 gene.Viral titers were then determined by counting plaques, and theresults were expressed as the ratio of the titers observed inthe absence and presence of IFN (Table 1). Consistent with previousdata (23), plaque formation by wild-type strains KOS and 17syn+was only marginally reduced by IFN- $alpha$ (two- to fivefold reduction).In striking contrast, ICP0 mutants of both strains exhibited greatlyincreased sensitivity to IFN. Isolates 7134 (5), dl1403 (50),and n212 (5) were inhibited more than 200-fold, while dlX3.1(48) displayed a greater than 1,000-fold reduction in titer.Isolates 7134, dl1403, and dlX3.1 bear large deletions of ICP0coding sequences, while n212 is truncated by an amber codon followingresidue 212. The deletion in dlX3.1 also removes the majorityof the transcriptional regulatory signals upstream of the ICP0gene. ICP0 mutants display impaired expression of IE, early, andlate genes during infection of cultured cells (15), and so itwas possible that the hypersensitivity exhibited by these mutantswas an indirect consequence of reduced expression of one or moreviral proteins that are downstream in the lytic cascade. However,this seems unlikely, since the VP16 in1814 (1) and V422 (49)mutations, which eliminate VP16 transactivation, cause defectsin viral gene expression similar to those exhibited by ICP0-nullmutants (1, 39, 49), but are much less sensitive to IFN- $alpha$ (Table 1). In agreement with previous results (23), in1814was inhibited to a slightly greater extent than parental wild-typestrain 17syn+, while V422 was approximately 5- to 10-fold moresensitive than parental wild-type strain KOS. This latter resultis consistent with our previous data indicating that V422 displaysa somewhat more severe phenotype than in1814 (39). Mutants defectivein the protein kinase encoded by the UL13 gene (d13lacZ) (30),IE protein ICP22 (d22lacZ) (30), and the virion host shutoffprotein vhs ( $Delta$ Sma) (46) were as resistant to IFN- $alpha$ as parentalwild-type HSV-1 strain KOS (Table 1). Taken in combination, thesedata demonstrate that expression of functional ICP0 is requiredfor the relatively IFN-resistant phenotype of wild-type HSV-1.

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TABLE 1. Effects of IFN- $alpha$ and cell type on plaque formation efficiency of different viruses^a

Previous studies have shown that the growth defects of ICP0 and VP16 mutants are "complemented" in U2OS osteosarcoma cells(39, 49, 52). Interestingly, all of the mutants analyzedabove demonstrated approximately the same sensitivity to IFN- $alpha$ on U2OS cells as wild-type HSV-1 on Vero cells (Table 1). Thus,in Vero cells, HSV-1 mutants lacking functional ICP0 are exquisitelysensitive to IFN- $alpha$ , while in U2OS cells, IFN- $alpha$ inhibition is notaffected by the functional status of ICP0. These data raise thepossibility that the ability of U2OS cells to "complement" ICP0mutants (52) may stem from a defect in one or more componentsof the IFN-inducible antiviral defense system. Consistent withthis possibility, VSV is also highly resistant to IFN- $alpha$ in U2OScells (Table 1). Further experiments are required to test thishypothesis.

Given the published data indicating that IFN- $alpha$ inhibits IE transcription during infection with wild-type HSV, it seemed possiblethat the hypersensitivity of ICP0 mutants revealed above stemsat least in part from a failure to accumulate adequate quantitiesof IE mRNAs. We therefore examined the accumulation of viral transcriptsin IFN-treated and control Vero cells at various times postinfectionwith 5 PFU of wild-type HSV-1, in1814, n212, and dlX3.1 per cell(Fig. 1). Viral titers were determined on U2OS cells in the presenceof 3 mM hexamethylene-bis-acetamide (34, 39, 49) to controlfor the known increase in the particle/PFU ratio of VP16 and ICP0mutants (1, 15). Untreated cells accumulated easily detectableamounts of the IE mRNAs encoding ICP4 and ICP27 by 8 h postinfection,regardless of the infecting virus, although in1814, n212, anddlX3.1 were significantly delayed relative to KOS. In contrast,only KOS displayed readily detectable IE RNA in IFN- $alpha$ -treatedcells at the 8-h time point. By 24 h postinfection, however, aclear distinction was observed between IFN- $alpha$ -treated cells infectedwith in1814 and those infected with n212 or dlX3.1. High levelsof IE RNA were observed in cells infected with in1814, while muchless RNA was detected in cells infected with either ICP0 mutant.Identical results were obtained when the blots were stripped andreprobed for ICP0 mRNA, except that, as expected, dlX3.1 failedto accumulate the ICP0 transcript (data not shown). A similartrend was observed for the early transcript encoding ICP8, exceptfor slightly delayed kinetics, as expected. These data indicatethat ICP0 mutants display a severe defect in accumulation of IERNAs in IFN- $alpha$ -treated Vero cells. In marked contrast, all of themutant viruses rapidly accumulated high levels of viral IE transcriptsin both control and IFN- $alpha$ -treated U2OS cells (data not shown).Concurrent Western blot analyses yielded a good correlation betweenmRNA levels and the levels of ICP4, ICP27, and ICP8 protein duringinfection of Vero cells (Fig. 2).

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FIG. 1. Effect of IFN pretreatment on accumulation of viral mRNAs. Vero cells were mock treated ( $-$ ) or pretreated (+) with 1,000 U of IFN- $alpha$ per ml for 16 h prior to infection with 5 PFU of the indicated virus per cell. Total RNA was harvested either 4, 8, or 24 h postinfection by using Trizol (Gibco BRL). Aliquots (5 µg) were then analyzed for ICP4, ICP27, or ICP8 transcript levels by Northern blot analysis with ³²P random-primer-labeled probe by using ExpressHyb (Clontech).

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FIG. 2. Effect of IFN pretreatment on accumulation of ICP4, ICP27, and ICP8. Vero cells were mock treated ( $-$ ) or pretreated (+) with 1,000 U of IFN- $alpha$ per ml for 16 h prior to infection with 5 PFU of the indicated virus per cell. Infected cells were harvested directly into sodium dodecyl sulfate-polyacrylamide gel electrophoresis sample buffer at 4, 8, and 24 h postinfection. Lysates were run on 9% polyacrylamide gels, transferred to nitrocellulose membranes, and blotted for ICP4, ICP27, or ICP8 protein by using a 1:2,000 dilution of GICR 1114, 1113, or 1115, respectively (Goodwin Institute for Cancer Research).

Taken together, these experiments demonstrate that ICP0 is required to overcome the antiviral effects of IFN- $alpha$ . In the absenceof VP16 activation function, accumulation of viral RNA and proteinis significantly delayed, but eventually proceeds, giving riseto high levels of viral gene products. In contrast, ICP0 mutantsare severely crippled in their ability to bypass the IFN-inducedblockade. It is tempting to speculate that the slightly increasedIFN sensitivity of VP16 mutants revealed in the plaque reductionassay stems from reduced and/or delayed production ofICP0.

The link between ICP0 and the resistance of HSV-1 to IFN revealed by our data is both intriguing and significant, given theresults of recent studies of the role of ICP0 during HSV-1 infection.ICP0 has been shown to interact strongly and specifically witha ubiquitin-specific protease, HAUSP (13), as well as localizeto and subsequently disrupt discrete nuclear domains called ND10(33). ND10 are considered sites of DNA virus transcription andregulation, because many DNA viral genomes are deposited at theperiphery of ND10 early in infection (32). ND10 are sites ofaccumulation of various proteins, most notably PML and Sp100,both of which are highly inducible by IFN, suggesting that ND10may be involved in a nuclear defense mechanism (32). ICP0 appearsto abrogate the SUMO-1 (ubiquitin-like) modification of ND10-specificproteins, thus causing the proteasome-dependent degradation ofkey cellular factors, whose normal protection by HAUSP is eliminatedthrough its interaction with ICP0 (7, 11, 40). It has alsobeen suggested that intact ND10 may inhibit viral DNA replicationby masking important nuclear attachment sites, sites that areexposed upon disruption of ND10 by ICP0 (4).

Recent experiments have shown that the interaction with HAUSP contributes to the functional activities of ICP0 (12) andthat inhibition of the ubiquitin-proteasome pathway inhibits theability of ICP0 to stimulate lytic infection as well as reactivationof latent genomes (11). One interpretation of these data isthat host repression proteins target incoming viral genomes, andICP0 is required to induce the degradation of these inhibitoryproteins (13, 14). Interpreted within the framework of thismodel, our data strongly suggest that some or many of the keyinhibitory proteins targeted by ICP0 are IFN inducible. Identificationof possible IFN-induced repressor proteins would solidify thishypothesis and warrants further investigation. If this model iscorrect, then it is possible that U2OS cells are defective inthe repression mechanism, instead of expressing an ICP0-like activatoras originally suggested (52). In this context, we are intriguedby the observation that VSV is highly resistant to IFN- $alpha$ in thesecells (Table 1). This result implies that U2OS cells are defectivein one or more IFN-induced antiviral mechanisms. Although it isnot yet clear if this defect accounts for the efficient replicationof ICP0 mutants in this cell line in the absence of IFN (52),it is tempting to speculate that basal expression of one or moreIFN-inducible inhibitors accounts for the requirement for ICP0in other cell types. Consistent with this hypothesis, ICP0 mutantsreplicate poorly in wild-type mice, but replication is almostfully restored in IFN receptor-null mice, attesting to the importanceof both ICP0 for HSV-1 and IFN for the host (9, 26, 27).

While the antiviral mechanisms of IFN are exerted through both nuclear and cytoplasmic events, the majority of the viral proteinsthat counteract IFN act either outside the cell or within thecytoplasm. While our data do not identify the key targets of ICP0,it is possible that one or more targets are nuclear. Due to thedesign of our experiments, in which an IFN-induced antiviral statehas been established prior to infection, it is fairly clear thatICP0 is not involved in disrupting the IFN- $alpha$ signal transductioncascade, as is the case for human cytomegalovirus, but insteadtargets events which occur following production of IFN-stimulatedantiviral proteins. Further studies are ongoing to elucidate moreprecisely where and how ICP0 functions relative to IFN, in orderto further understand the mechanisms of action of both IFN andICP0 in Vero and U2OScells.

	ACKNOWLEDGMENTS

We thank Rob Maranchuk for technical assistance and P. Schaffer and R. Everett for generously providing mutant virusrecombinants.

This work was supported by a grant from the Medical Research Council of Canada. K.L.M. is funded by fellowships from the MRCand the Alberta Heritage Foundation for Medical Research. J.R.S.was a Terry Fox Senior Scientist of the National Cancer InstituteofCanada.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Medical Microbiology & Immunology, 1-41, Medical Sciences Bldg., Universityof Alberta, Edmonton, Alberta, Canada T6G 2H7. Phone: (780) 492-2308.Fax: (780) 492-7521. E-mail: jim.smiley{at}ualberta.ca.

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Mossman, K. L., Smiley, J. R. (2002). Herpes Simplex Virus ICP0 and ICP34.5 Counteract Distinct Interferon-Induced Barriers to Virus Replication. J. Virol. 76: 1995-1998 [Abstract] [Full Text]
Preston, C. M., Harman, A. N., Nicholl, M. J. (2001). Activation of Interferon Response Factor-3 in Human Cells Infected with Herpes Simplex Virus Type 1 or Human Cytomegalovirus. J. Virol. 75: 8909-8916 [Abstract] [Full Text]
Halford, W. P., Kemp, C. D., Isler, J. A., Davido, D. J., Schaffer, P. A. (2001). ICP0, ICP4, or VP16 Expressed from Adenovirus Vectors Induces Reactivation of Latent Herpes Simplex Virus Type 1 in Primary Cultures of Latently Infected Trigeminal Ganglion Cells. J. Virol. 75: 6143-6153 [Abstract] [Full Text]
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Halford, W. P., Schaffer, P. A. (2001). ICP0 Is Required for Efficient Reactivation of Herpes Simplex Virus Type 1 from Neuronal Latency. J. Virol. 75: 3240-3249 [Abstract] [Full Text]
Burkham, J., Coen, D. M., Hwang, C. B. C., Weller, S. K. (2001). Interactions of Herpes Simplex Virus Type 1 with ND10 and Recruitment of PML to Replication Compartments. J. Virol. 75: 2353-2367 [Abstract] [Full Text]
Mossman, K. L., Macgregor, P. F., Rozmus, J. J., Goryachev, A. B., Edwards, A. M., Smiley, J. R. (2001). Herpes Simplex Virus Triggers and Then Disarms a Host Antiviral Response. J. Virol. 75: 750-758 [Abstract] [Full Text]
Halford, W. P., Schaffer, P. A. (2000). Optimized Viral Dose and Transient Immunosuppression Enable Herpes Simplex Virus ICP0-Null Mutants To Establish Wild-Type Levels of Latency In Vivo. J. Virol. 74: 5957-5967 [Abstract] [Full Text]

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