The V Protein of Simian Virus 5 Inhibits Interferon Signalling by Targeting STAT1 for Proteasome-Mediated Degradation

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Journal of Virology, December 1999, p. 9928-9933, Vol. 73, No. 12
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

The V Protein of Simian Virus 5 Inhibits Interferon Signalling by Targeting STAT1 for Proteasome-Mediated Degradation

L. Didcock,¹ D. F. Young,¹ S. Goodbourn,² and R. E. Randall¹^,^*

School of Biology, University of St. Andrews, Fife, Scotland KY16 9TS,¹ and Department of Biochemistry, St. George's Hospital Medical School, University of London, London SW17 ORE,² United Kingdom

Received 10 June 1999/Accepted 9 August 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

To replicate in vivo, viruses must circumvent cellular antiviral defense mechanisms, including those induced by the interferons(IFNs). Here we demonstrate that simian virus 5 (SV5) blocks IFNsignalling in human cells by inhibiting the formation of the IFN-stimulatedgene factor 3 and gamma-activated factor transcription complexesthat are involved in activating IFN- $alpha$ / $beta$ - and IFN- $gamma$ -responsivegenes, respectively. SV5 inhibits the formation of these complexesby specifically targeting STAT1, a component common to both transcriptioncomplexes, for proteasome-mediated degradation. Expression ofthe SV5 structural protein V, in the absence of other virus proteins,also inhibited IFN signalling and induced the degradation of STAT1.Following infection with SV5, STAT1 was degraded in the absenceof virus protein synthesis and remained undetectable for up to4 days postinfection. Furthermore, STAT1 was also degraded inIFN-pretreated cells, even though the cells were in an antiviralstate. Since pretreatment of cells with IFN delayed but did notprevent virus replication and protein synthesis, these observationssuggest that following infection of IFN-pretreated cells, SV5remains viable within the cells until they eventually go out ofthe antiviralstate.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Virus infection of susceptible host cells activates the transcription of many cellular genes, including the interferons (IFNs),that are involved in antiviral defense, cell growth regulation,and immune activation. IFNs represent a group of cytokines withthe unique ability to establish an antiviral state in cells throughthe expression of many IFN-stimulated genes (ISGs). A number ofthese ISGs encode intracellular enzymes, the best known of whichis a protein kinase (PKR). Although induced by IFN, PKR remainsinactive unless cells also produce excess double-stranded RNA(e.g., as a result of viral infection). Activated PKR modifiesand inactivates eukaryotic initiation factor 2 $alpha$ , a key componentof the eukaryotic translational apparatus, leading to the shutoffof viral protein synthesis (9). IFNs also induce 2'5' oligoadenylatesynthetase (30), which, together with RNase L, results in acceleratedRNA degradation and thus also an inhibition of protein synthesis.In addition, IFNs down-regulate the cell cycle (45) and inducea proapoptotic state in cells (3) as well as up-regulate thesurface expression of class I major histocompatibility complex(MHC) molecule, thereby enhancing peptide presentation to T cells(27).

The biological activities of IFNs are initiated by the binding of IFN- $alpha$ / $beta$ and IFN- $gamma$ to their cognate receptors, which resultsin the activation of distinct but related signalling pathways.IFN- $alpha$ / $beta$ signal via receptor-associated tyrosine kinases, Jak1and Tyk2, that phosphorylate and activate the signal transducersand activators of transcription, STAT1 and STAT2. Upon phosphorylation,STAT1 and STAT2 form heterodimers which translocate to the nucleus,where they associate with the DNA-binding protein p48 to forminterferon-stimulated gene factor 3 (ISGF3). ISGF3 binds IFN-stimulatedresponse elements (ISREs) to drive the expression of IFN- $alpha$ / $beta$ regulatedgenes. Similarly, IFN- $gamma$ signals via receptor-associated tyrosinekinases, Jak1 and Jak2, mediating phosphorylation and activationof STAT1 but not STAT2. STAT1 homodimers form the active transcriptioncomplex, gamma-activated factor (GAF) which bind to gamma-activatedsequence (GAS) elements in regulatory regions of IFN- $gamma$ -induciblegenes. Since STAT1 is also activated by IFN- $alpha$ / $beta$ , the GAS complexcan be formed in response to IFN- $alpha$ / $beta$ . Thus, Jak1 and STAT1 arethe common components of IFN- $alpha$ / $beta$ and IFN- $gamma$ signal transductionpathways (for a review, see reference 43). The STAT1 gene containsmultiple exons which encode two forms of STAT1 (37). STAT1 $alpha$ (91 kDa) is 750 amino acids in length; STAT1 $beta$ (84 kDa) is theproduct of a differentially spliced mRNA which encodes a proteinof 712 amino acids (37, 50). Both forms are known to be phosphorylatedon a single residue, Tyr-701, allowing their dimerization andtranslocation to the nucleus to bind DNA (40, 41). However,STAT1 $alpha$ is the only transcriptionally active form of STAT1 sinceSTAT1 $beta$ lacks the 38 C-terminal amino acids containing the knowntranscriptional activation domain (24, 37). For maximal transcriptionalactivity, STAT1 $alpha$ must also be phosphorylated on Ser-727 (49),a residue that is missing in STAT1 $beta$ .

For most known IFN-induced antiviral activities, there are examples of virally encoded gene products that antagonize theireffects. Viral products that specifically inhibit PKR, block ordown-regulate MHC class I expression, stimulate cell division,inhibit apoptosis, or act as decoy MHC-like molecules to preventNK cell activation have been described (31, 39, 42). Todate, there are few examples of viruses inhibiting transcriptionalresponses to IFNs; certain poxviruses secrete soluble IFN receptorproteins which block the IFN- $gamma$ responses (47); similarly, vacciniavirus encodes a soluble IFN- $alpha$ / $beta$ receptor (44). Other viruseshave been shown to block transcriptional responses by alteringthe levels or function of critical components of the signallingpathways. For example, the E1A product of adenovirus has beendescribed as having the ability to block IFN responses by interferingwith transcription (19), and Look et al. (20) have shown thatthe adenovirus E1A protein can directly suppress STAT1 function.It has also been demonstrated that the K9 open reading frame ofhuman herpesvirus 8 can block transcriptional responses to IFN- $alpha$ / $beta$ and IFN- $gamma$ (52), and there is evidence that human cytomegalovirusalters Jak1 levels, thereby disrupting the IFN- $alpha$ / $beta$ and IFN- $gamma$ signallingpathways (23). It has also been noted that there are decreasedlevels of STAT1 $alpha$ in cells persistently infected with mumps virus(51).

We have previously demonstrated that the paramyxovirus simian virus 5 (SV5) blocks IFN- $alpha$ / $beta$ signalling in human but not murinecells (6), thereby defining a host cell constraint which mayprevent SV5 from crossing species barriers and causing diseasein mice. Here we extend these findings by showing that SV5 canalso block IFN- $gamma$ signalling in human cells and identify both thecellular target and the viral protein responsible for thisinhibition.

SV5 is an enveloped virus with a nonsegmented, negative-sense RNA genome. The single-stranded genome encodes eight proteins:the nucleocapsid protein (NP), V protein (V), phosphoprotein (P),matrix protein (M), fusion protein (F), small hydrophobic protein,hemagglutinin-neuraminidase protein, and large polymerase protein(for a review of paramyxoviruses and their replication, see reference17). P and V are both structural proteins and are encoded bya single gene. They share the same 164 N-terminal amino acidsbut have unique C termini. The C terminus of V is cysteine rich,binds two atoms of zinc per molecule (28), and is highly conservedamong paramyxoviruses. V mRNA is a faithful transcript of theP/V gene, but P mRNA contains two additional nontemplated G residues(46), specifically inserted by the viral RNA polymerase stutteringduring transcription of the gene (48), which alters the readingframe of the mRNA. Although it is known that P is part of thevirus-encoded polymerase complex, the roles of V in virus replicationand pathogenesis are unclear. It appears to be dispensable forvirus replication in tissue culture cells, but it is essentialfor virus pathogenesis in Sendai virus (SeV) (5, 13). TheV protein of SV5 has also been shown to bind soluble but not polymericforms of NP (33), and also to bind to the cellular UV DNA damagebinding protein (21). Here we demonstrate that the V, but notthe P, protein of SV5 also blocks IFN signalling by targetingSTAT1 for proteasome-mediateddegradation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture and virus infections. Human diploid fibroblast 2fTGH cells (29) were maintained in Dulbecco's modified Eagle's medium (DMEM) supplemented with10% fetal bovine serum (growth medium). SV5 (strain W3 [4])and recombinant Semliki Forest virus (SFV) infections were performedat a multiplicity of infection (MOI) of 10 in DMEM containing2% fetal bovine serum (maintenance medium) and in reduced-serummedium (Opti-MEM; Gibco-BRL), respectively. After an adsorptionperiod of 1 to 2 h, the inoculum was removed and replaced withmaintenance medium. Cells were treated with either recombinanthuman IFN- $alpha$ A/D (rHuIFN- $alpha$ A/D [34]) or human IFN- $gamma$ (catalog no.80-3348-01; Genzyme Diagnostic) added to maintenance medium at1,000 IU/ml. For proteasome inhibitor experiments, 2fTGH cellsin 6- or 24-well plates were mock infected or infected with SV5or recSFV in medium containing 0.2% dimethyl sulfoxide (DMSO)that had or had not been supplemented with either 10 µM MG132or 10 µM lactacystin (catalog no. PI-104; BIOMOL Research LaboratoriesInc.). After a 1- to 2-h adsorption period, the medium was removedand replaced with maintenance medium supplemented with 0.2% DMSOor 0.2% DMSO containing 10 µM MG132 or lactacystin, and cellswere incubated for a further 6 h. In experiments monitoring I $kappa$ B $alpha$ degradation, cells then were or were not treated with tumor necrosisfactor alpha (TFN- $alpha$ ) at 10 ng/ml. At 8 h postinfection, (p.i.),the cell monolayers were washed twice in phosphate-buffered saline(PBS) and lysed directly in sodium dodecyl sulfate (SDS)-gel loadingbuffer (0.05 M Tris-HCl [pH 7.0], 0.2% SDS, 5% 2-mercaptoethanol,5%glycerol).

Immunoblotting. At the time of harvest, cells were washed twice in PBS, scraped in SDS-gel loading buffer, and boiled for 5 min. Proteinswere separated by electrophoresis through SDS-7.5% polyacrylamidegels, transferred to nitrocellulose membranes, and detected withspecific antisera, including a polyclonal anti-STAT1 antibodyraised against the N-terminal 194 amino acids, a monoclonal antibody(MAb) reactive to the C terminus of STAT1, and a MAb to the N-terminalregion of STAT2 (catalogue no. G16930, S21120, and S21220, respectively;Transduction Laboratories) and polyclonal antibodies to eitherphosphotyrosine (701) STAT1 or phosphoserine (727) STAT1 (catalogueno. 06-657 or 06-802, respectively; Upstate Biotechnology). Unlessotherwise stated, STAT1 was detected with an antibody to the Nterminus of STAT1. It should also be noted that antibodies raisedagainst both the N and C termini of STAT1 (G16930 and S21120,respectively) react with STAT1 $alpha$ and STAT1 $beta$ . I $kappa$ B $alpha$ was detectedwith the MAb 10B (12). All protein-antibody interactions weredetected by enhanced chemiluminescence using horseradish peroxidase-conjugatedsheep anti-mouse or donkey anti-rabbit immunoglobulin G (AmershamInternational Ltd., Little Chalfont, UnitedKingdom).

Plasmid DNAs. The IFN- $alpha$ / $beta$ -responsive plasmid, p(9-27)4tk $Delta$ ( $-$ 39)lucter, contained four tandem repeat sequences of the ISRE from the IFN-induciblegene 9-27 fused to the firefly luciferase gene (16); the IFN- $gamma$ -responsiveplasmid, p(GAS)2tk $Delta$ ( $-$ 39)lucter, contained a minimal thymidinekinase (TK) promoter and two tandem repeat sequences of the IRF-1GAS site fused to the luciferase gene (16). pJATlacZ, a plasmidused as a transfection standard, contains a $beta$ -galactosidase geneunder the control of the rat $beta$ -actin promoter (22).

To construct pEF.SV5-P and pEF.SV5-V vectors, SV5 P and V cDNA sequences were obtained from pGEM3 expression plasmids intowhich the P and V genes had been originally cloned (32). ThecDNAs were inserted between the NcoI and XhoI sites of the EF1apromoter vector, pEFlink2 (a kind gift from R. H. Treisman, ImperialCancer ResearchFund).

Transient transfections. Monolayers of 2fTGH cells grown in 24-well plates to 50 to 70% confluence were transfected with 0.5 µg of DNA and 2 µl ofLipofectamine (Life Technologies Inc.) according to the manufacturer'sinstructions. After 16 h, the cells were or were not infectedwith SV5 and induced with 1,000 IU of rHuIFN- $alpha$ A/D per ml at 24h p.i. Four hours after induction by IFN, cells were harvestedand assayed for luciferase and $beta$ -galactosidase activity as describedpreviously (15). Relative expression levels were calculatedby dividing the luciferase values by the $beta$ -galactosidase values.The experiments were repeated several times with equivalentresults.

Electrophoretic mobility shift assay (EMSA). Whole-cell extracts (25) were prepared from mock-infected or SV5-infected cells that had or had not been treated with rHuIFN- $alpha$ A/Dfor 1 h prior to harvesting at 24 h p.i. Protein-DNA complexeswere formed by incubating 10 µg of protein for 15 min at 30°Cwith 1 ng of probe (labelled with [a ³²P]dATP by filling in the GATC 5' overhangs with Klenow enzymeon the otherwise double-stranded oligonucleotides 5' AGGAAATAGAAACTG3' [ISRE], or 5' TGATTTCCCCGAAATG 3' [GAS]) in a 20-µl reactionmixture containing 20 mM Tris (pH 8.0), 12% glycerol, 2 mM MgCl₂,0.6 mM dithiothreitol, and 375 ng poly(dI-dC) · poly(dI-dC). Complexeswere resolved on 6% native polyacrylamide (1:30 bisacrylamide/acrylamide)gels in 0.5× Tris-borate-EDTA, and the dried gels visualized byautoradiography.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

SV5 prevents the formation of ISGF3 and GAF complexes in human cells. Using luciferase reporter assays, we previously demonstrated that SV5 blocked IFN- $alpha$ / $beta$ signalling in human cells (Fig. 1a)but not murine cells (6). Using a similar approach, we showhere that SV5 also blocks IFN- $gamma$ signalling in human cells (Fig.1b) but not in murine cells (data not shown). To determine whetherSV5 inhibition of IFN- $alpha$ / $beta$ and IFN- $gamma$ signalling in human cellsreflected an inability to form the transcription complexes ISGF3and GAF, EMSAs were performed. In contrast to the induction ofISGF3 and GAF complexes in mock-infected cells treated with IFN,no ISGF3 and GAF complexes were detected in the SV5-infected cellextracts (Fig. 1c and d, respectively). (ISGF3 and GAF complexeswere readily detected in SV5-infected murine cells in the presenceof IFN [data not shown].)

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FIG. 1. SV5 inhibits IFN- $alpha$ / $beta$ (a) and IFN- $gamma$ (b) signalling and the formation of ISGF3 (c) and GAF (d) complexes in 2fTGH cells. Cells were transfected with either the IFN- $alpha$ / $beta$ (a)- or IFN- $gamma$ (b)-responsive plasmids together with pJATlacZ and at 16 h posttransfection were either mock infected or infected with SV5. At 24 h p.i. the culture medium was supplemented with rHuIFN- $alpha$ A/D (a) or IFN- $gamma$ (b) or left untreated. Four hours later, luciferase and $beta$ -galactosidase activities in the cellular lysates were measured. Luciferase activity, expressed in relative light units, was normalized to $beta$ -galactosidase activity. For the EMSAs, cells were mock infected or infected with SV5 for 24 h and then were (+) or were not ( $-$ ) treated with rHuIFN- $alpha$ A/D (c) or rHuIFN- $gamma$ (d) for 1 h. Extracts were prepared and analyzed by EMSAs using either ³²P-labelled ISRE (c) or GAS (d) probe.

Proteasome-mediated degradation of STAT1 in SV5-infected cells. Since STAT1 is the only common component of ISGF3 and GAF complexes, the levels of STAT1 in mock- or SV5-infected human cellswere examined by immunoblot blot analysis using antibodies reactiveto either the C (Fig. 2a) or N (Fig. 2b) terminus of STAT1. AlthoughSTAT1 was readily detectable in mock-infected cells (Fig. 2a andb), no STAT1 was detected in SV5-infected cells (Fig. 2a and b).(It should be noted that both STAT1 $alpha$ and STAT1 $beta$ were degradedin SV5 infected cells. The lower prominent band in Fig. 2b andsubsequent figures is not STAT1 $beta$ [see the legend to Fig. 2].)Immunoblot analysis using antisera reactive against the phosphotyrosine(701) and phosphoserine (727) forms of STAT1 showed that phosphorylatedforms of STAT1 were also degraded in SV5-infected cells (datanot shown). In contrast, the levels of STAT2 were comparable inmock- and SV5-infected cells (Fig. 2c).

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FIG. 2. STAT1, but not STAT2, is degraded in SV5-infected human cells. STAT1 and STAT2 were detected by immunoblot analysis in total-cell extracts of mock- or SV5-infected 2fTGH cells (harvested at 20 h p.i.), using antibodies reactive to the C terminus of STAT1 (a) or the N terminus of STAT1 (b) or STAT2 (c). It should be noted that both anti-STAT1 antibodies react with STAT1 $alpha$ and STAT1 $beta$ (they can be more clearly resolved on lower-percentage SDS-polyacrylamide gels). The lower prominent band, with an estimated molecular mass of 75 kDa, present in both mock-infected and SV5-infected cells (b) has not been identified.

No obvious degradation products of STAT1, such as those that might be expected for a sequence-specific endoprotease such asa caspase (16), were visible in the immunoblots of SV5-infectedcells. The failure to observe breakdown intermediates suggestedthat the proteins were being degraded by a processive proteasesuch as is seen for proteasome-mediated degradation. To test this,the levels of STAT1 were examined in cells treated with the proteasomeinhibitors MG132 and lactacystin (potent and structurally unrelatedinhibitors of proteasome action [8, 26, 35]). These results(Fig. 3a) clearly showed that in SV5-infected cells, STAT1 wasdegraded in the absence of MG132 (lanes 2 and 3); however, thiseffect was blocked by MG132 treatment (lanes 4 and 5). In thesame experiment, MG132 also prevented TNF- $alpha$ -induced degradationof I $kappa$ B $alpha$ (Fig. 3b; compare lanes 3 and 5), demonstrating that theinhibitor was effective at blocking proteasome-mediated degradationprocesses (1, 36). Lactacystin also inhibited the degradationof STAT1 in SV5-infected cells (data not shown).

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FIG. 3. The proteasome inhibitor MG132 blocks degradation of STAT1 in SV5-infected 2fTGH cells and of I $kappa$ B $alpha$ in TNF- $alpha$ -stimulated 2fTGH cells. Mock-infected cells (lanes 1) and SV5-infected cells (lanes 2 to 5) were incubated, from the time of infection, in medium that did (lanes 4 and 5) or did not (lanes 1 to 3) contain the proteasome inhibitor MG132 (10 µM). At 8 h p.i., the medium was (lanes 3 and 5) or was not (lanes 1, 2, and 4) further supplemented with TNF- $alpha$ ; 30 min later, the cells were harvested and the levels of STAT1 (a) and I $kappa$ B $alpha$ (b) were estimated by immunoblot analysis.

The V protein of SV5 targets STAT1 for proteasome-mediated degradation. We previously constructed a number of SFV vectors, including those that expressed the fusion (F) or V proteins of SV5. Todetermine whether either of these proteins might be responsiblefor the observed degradation of STAT1, we infected cells (at ahigh MOI) with these viruses or a virus that expressed $beta$ -galactosidaseand estimated the levels of STAT1 by immunoblot blot analysis(Fig. 4a). Negligible levels of STAT1 were present in cells infectedwith a recombinant SFV that expressed the V protein of SV5 (recSFV/V;Fig. 4a, lane 4). In contrast, levels of STAT1 similar to thatobserved in mock-infected cells (Fig. 4, lane 1) were presentin cells infected with a recombinant SFV that expressed eitherthe SV5 F protein (recSFV/F) (lane 2) or $beta$ -galactosidase (recSFV/lacZ)(lane 3).

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FIG. 4. The V protein of SV5 induces proteasome-mediated degradation of STAT1. (a) 2fTGH cells were mock infected (lane 1) or infected with recSFV/F (lane 2), recSFV/lacZ (lane 3), or recSFV/V (lane 4) for 8 h, and total-cell extracts were probed for STAT1 as previously described. (Immunofluorescence analysis confirmed that >95% of the cells were expressing the appropriate virus proteins at the time of harvest.) (b) 2fTGH cells were mock infected (lanes 1 and 2) or infected with recSFV/V (lanes 3 and 4). The proteasome inhibitor MG132 (10 µM) was (lanes 2 and 4) or was not (lanes 1 and 3) added to the culture medium at the time of infection. At 8 h p.i., cells were harvested and levels of STAT1 were estimated by immunoblot analysis.

To confirm that the mechanism of degradation of STAT1 induced by the V protein of SV5 was the same as that observed in SV5-infectedcells, the levels of STAT1 were examined in cells treated withthe proteasome inhibitor MG132. These results demonstrated thatMG132 inhibited the degradation of STAT1 in cells infected withrecSFV/V (Fig. 4b; compare lanes 3 and 4). In the same experiment,no degradation of STAT1 was observed in cells expressing eitherSV5 F or the $beta$ -galactosidase proteins in the presence or absenceof the inhibitor (data notshown).

The first 164 N-terminal amino acids are common between the V and P proteins of SV5, but V and P possess unique C termini.It was therefore important to ascertain whether P could also blockIFN signalling. To address this question, we cloned the P andV genes into the EF1 $alpha$ promoter vector pEFlink2 and measured theability of the expressed proteins to block the activation of theIFN- $alpha$ / $beta$ -responsive plasmid. It can clearly be seen from Fig. 5that expression of P and V had no effect on the TK control promoter(Fig. 5a). However, V, but not P, blocked activation of the IFN- $alpha$ / $beta$ -responsivepromoter (Fig. 5b).

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FIG. 5. The V protein of SV5, but not P, blocks activation of an IFN- $alpha$ / $beta$ -responsive promoter in human cells. 2fTGH cells were transfected with a mixture of plasmids that contained the luciferase gene under the control of either the herpes simplex virus TK promoter (a) or an IFN- $alpha$ / $beta$ -responsive promoter (b; 0.1 µg), together with 0.3 µg of pEFlink2 (control), pEF.SV5-P (expressing the SV5 P protein), or pEF.SV5-V (expressing the SV5 V protein). Also included in the transfection mix was 0.1 µg of plasmid pJATlacZ, in which the lacZ gene is under the control of the rat $beta$ -actin promoter. At 40 h posttransfection, the culture medium was (+) or was not ( $-$ ) supplemented with IFN. Four hours later, luciferase and $beta$ -galactosidase activities in cellular lysates were measured. Luciferase activity, expressed in relative light units, was normalized to $beta$ -galactosidase activity.

Infecting virus can induce the degradation of STAT1 in the absence of virus protein synthesis. Since the V protein is a structural component of the SV5 virion, it was of interest to determine how quickly STAT1 disappearedfollowing SV5 infection and whether virus protein synthesis wasrequired. In a time course experiment following infection of cellsat a high MOI (10 PFU/cell), there was a significant reductionin the amount of STAT1 by 4 h p.i. and complete loss of STAT1by 8 h p.i. (Fig. 6a, lanes 4 and 5, respectively). In contrast,STAT2 levels remained constant throughout the experiment (datanot shown). Furthermore, immunofluorescence analysis and immunoprecipitationof ³⁵S-labelled polypeptides showed that little virus protein synthesishad occurred by 4 h p.i. (data not shown), suggesting that STAT1might be degraded in the absence of virus protein synthesis. Todetermine whether this was the case, cells were infected withSV5 that had been inactivated by UV light such that the viruscould no longer synthesize detectable amounts of virus proteins.These results demonstrated that UV-inactivated virus also inducedthe degradation of STAT1 (data not shown; see also Fig. 6b).

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FIG. 6. STAT1 was rapidly degraded in SV5-infected cells in the absence of virus protein synthesis. (a) Total-cell extracts of 2fTGH cells that were mock infected (lane 1) or infected with SV5 for 1, 2, 4, or 8 h (lanes 2 to 5, respectively) were probed for STAT1 by immunoblot analysis. (b) 2fTGH cells were mock infected (lane 1) or infected with UV-inactivated SV5 (lanes 2 to 6). At 6 (lanes 1 and 2) and 24, 48, 72, and 96 (lanes 3 to 6, respectively) h p.i. total cell extracts were probed for STAT1 by immunoblot analysis. (At no time throughout the latter experiment were cells positive for virus antigens, as judged by immunofluorescence.)

To determine how long it took cells to recover normal levels of STAT1 in the absence of virus protein synthesis, cells wereinfected with UV-inactivated virus and harvested at various timesp.i., and levels of STAT1 were estimated (Fig. 6b). At 3 daysp.i., STAT1 protein levels remained negligible (Fig. 6b, lane5), and it took up to 4 days before substantial levels of STAT1could be detected (Fig. 6b, lane6).

The finding that virus (and cellular) transcription and protein synthesis were not required for the degradation of STAT1 inSV5-infected cells was confirmed by using actinomycin D and cycloheximide,inhibitors of transcription and protein synthesis, respectively.The levels of STAT1 in untreated mock-infected cells (Fig. 7a)were similar to that in mock-infected cells treated with eitheractinomycin D or cycloheximide for 8 h (Fig. 7a), thereby demonstratingthat there is a slow turnover of STAT1 in uninfected cells. Incontrast, STAT1 was rapidly degraded in SV5-infected cells thathad or had not been treated with actinomycin D or cycloheximidethroughout the infection (Fig. 7b).

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FIG. 7. Inhibition of transcription and protein synthesis did not prevent the degradation of STAT1 in SV5-infected cells. 2fTGH cells were untreated (Un) or treated with actinomycin D (Act. D; 10 µg/ml) or cycloheximide (Cx; 50 µg/ml) 1 h prior to being mock infected or infected with SV5. Actinomycin D or cycloheximide (as appropriate) was also present throughout infection period. Total-cell extracts were made at 6 h p.i., and the levels of STAT1 were detected by immunoblot analysis.

STAT1 is degraded in IFN-pretreated cells by infecting virus. Pretreatment of cells with IFN delays the onset of virus protein synthesis until between 24 and 48 h p.i., compared to about8 h p.i. in untreated cells (6). One explanation for this delaywould be that pretreatment of cells with IFN induced an antiviralstate which efficiently inhibited virus replication. However,in the absence of continued IFN signalling (due to the degradationof STAT1 by infecting virus), the antiviral state in these cellswas not maintained, thus permitting the infecting virus to eventuallyreplicate. Consistent with this model, infection with SV5 inducedthe degradation of STAT1 in IFN-pretreated cells. It can be seenfrom Fig. 8 that IFN stimulated STAT1 expression (the STAT1 geneis under the control of an IFN-responsive promoter), as the levelswere significantly higher in mock-infected cells pretreated withIFN than in untreated cells (Fig. 8; compare lanes 1 and 2). Nevertheless,in IFN-pretreated cells that had been infected with SV5, onlysmall amounts of STAT1 were detected at 6 h p.i., and no STAT1was detected at 24 h p.i. (Fig. 8, lanes 4 and 6, respectively).

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FIG. 8. STAT1 was degraded in IFN-pretreated cells. 2fTGH cells were (lanes 2, 4, and 6) or were not (1, 3, and 5) treated with rHuIFN- $alpha$ A/D for 24 h prior to mock infection (lanes 1 and 2) or infection with SV5 (lanes 3 to 6). Total-cell extracts were made from cells harvested at either 6 (lanes 1 to 4) or 24 (lanes 5 and 6) h p.i., and levels of STAT1 were detected by immunoblot analysis.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The potential effectiveness of the IFN response, if not blocked, can be judged by the rapid switch-off of SV5 protein synthesisin murine cells following the induction of IFN (SV5 does not blockIFN signalling in murine cells [6]). In contrast, human cellsinfected with SV5 can no longer respond to IFN and thereby switchoff virus protein synthesis once it has been established (6).In this report, we show that SV5 specifically targets STAT1 forproteasome-mediated degradation in human (but not murine) cells,thereby blocking both type I and type II IFN signalling by inhibitingthe formation of the ISGF3 and GAF transcription complexes. Wealso demonstrate that SV5 can induce the degradation of STAT1in human cells that have entered an antiviral state, and thismay be of significance in terms of virus pathogenesis. Presumably,in the absence of continued signalling (due to a loss of STAT1),cells cannot remain in an antiviral state and suppress virus replicationindefinitely. Thus there must be competition between intracellularvirus remaining viable and cells resynthesizing sufficient levelsof STAT1 to be able to respond to IFN and thus maintain theirantiviralstate.

There are clearly many potential advantages for SV5 in blocking both type I and type II IFN signalling. For example, in additionto blocking the autocrine effect of IFN- $alpha$ / $beta$ secreted from infectedcells, SV5-infected cells would be insensitive to both IFN- $alpha$ andIFN- $gamma$ released by activated leukocytes and T cells. Furthermore,as IFN can act as a leukocyte-activating cytokine, increasingNK cell activity and acting as a growth factor for memory CD8⁺ T cells, in the event of SV5 infection of these cells, cellularimmune responses may be adversely affected. The fact that SV5can lead to the degradation of STAT1 in the absence of virus proteinsynthesis may compound this situation. Furthermore, since V isa structural protein associated with the nucleocapsids of thevirion (~350 molecules per virion [28]), defective virus particlesmay also contribute to any effectsobserved.

Several properties have been ascribed to V, including its interaction with both viral NP (33) and cellular (21) proteins.However, it is clear that the interaction of V with NP is notrequired for either its ability to block IFN signalling or thetargeting of STAT1 for proteasome-mediated degradation. Thus,it remains likely that V is a multifunctional protein with a numberof independent roles in SV5 replication and pathogenesis. Whetherthe V protein of other members of the Paramyxovirinae family playexactly the same roles as that performed by the V protein of SV5remains to be established but seems unlikely. Thus, while thisreport was under review, Garcin et al. (9a) reported that itwas the C proteins of SeV, and not V, that counteract the IFN-inducedanti-viral state (SV5 and other rubulaviruses do not encode theC proteins). Since we had previously reported that SeV also blocksIFN signalling (6), it is probable that the molecular mechanismsemployed by SeV and SV5 to block the IFN signalling differ indetail. Indeed, it remains to be elucidated exactly how the Vprotein of SV5 targets STAT1 for proteasome-mediated degradation.V may interact directly with STAT1 and thereby somehow targetit for ubiquitination and degradation. Alternatively, V may activatea normal cellular pathway involved in STAT1 turnover. In thisrespect, it is of note that Kim and Maniatis (14) reported thatactivated (phosphorylated) STAT1 is degraded by a ubiquitin-proteasomepathway. However, there is some debate as to whether dephosphorylation/nuclearimport mechanisms are more important mechanisms of down-regulationof STAT1 than proteolytic degradation (10, 18). The key importmechanisms are more important mechanisms of down-regulation ofSTAT1 than proteolytic degradation (10, 18). The key differencein the observations reported here is that both phosphorylatedand nonphosphorylated forms of STAT1 are degraded in SV5-infectedcells.

There are other examples of viruses targeting cellular proteins for proteasome-mediated degradation. The E6 and E7 proteinsof human papillomaviruses target p53 and pRB, respectively, forproteasome-mediated degradation (2, 11, 38). Disruptionof nuclear structures known as ND10, or PML nuclear bodies, thathave been implicated in a number of cellular processes (e.g.,response to stress and IFNs, oncogenesis, and viral infection)also occurs during herpes simplex virus infection by a proteasome-dependentprocess (7). Thus, the targeting of important cellular controlproteins for proteasome-mediated degradation may be a generalmechanism employed by viruses to usurp cellularpathways.

	ACKNOWLEDGMENTS

L. Didcock is indebted to the MRC for a Ph.D. studentship and the Wellcome Trust for current support. S. Goodbourn is a recipientof a Wellcome Trust University award, and D. F. Young is supportedby theBBSRC.

We thank Ron Hay (University of St. Andrews) for reagents and helpfuladvice.

	FOOTNOTES

^* Corresponding author. Mailing address: Biomolecular Sciences Bldg., North Haugh, University of St. Andrews, Fife, ScotlandKY16 9TS, United Kingdom. Phone: 44 1334 463397. Fax: 44 1334462595. E-mail: rer{at}st-and.ac.uk.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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