Activation of TRAF5 and TRAF6 Signal Cascades Negatively Regulates the Latent Replication Origin of Epstein-Barr Virus through p38 Mitogen-Activated Protein Kinase

doi:10.1128/JVI.75.11.5059-5068.2001

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Journal of Virology, June 2001, p. 5059-5068, Vol. 75, No. 11
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.11.5059-5068.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Activation of TRAF5 and TRAF6 Signal Cascades Negatively Regulates the Latent Replication Origin of Epstein-Barr Virus through p38 Mitogen-Activated Protein Kinase

Masaki Shirakata,¹^,^* Ken-Ichi Imadome,¹ Kenji Okazaki,² and Kanji Hirai¹

Department of Tumor Virology, Division of Virology and Immunology, Medical Research Institute, Tokyo Medical and Dental University, Bunkyo, Tokyo 113-8510,¹ and Department of Molecular Biology, Biomolecular Engineering Research Institute (BERI), Suita, Osaka 565-0874,² Japan

Received 30 November 2000/Accepted 9 March 2001

	ABSTRACT

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Latent Epstein-Barr virus (EBV) is maintained by the virus replication origin oriP that initiates DNA replication with theviral oriP-binding factor EBNA1. However, it is not known whetheroriP's replicator activity is regulated by virus proteins or extracellularsignals. By using a transient replication assay, we found thata low level of expression of viral signal transduction activatorlatent membrane protein 1 (LMP1) suppressed oriP activity. Thebinding site of the tumor necrosis factor receptor-associatedfactor (TRAF) of LMP1 was essential for this suppressive effect.Activation of the TRAF signal cascade by overexpression of TRAF5and/or TRAF6 also suppressed oriP activity. Conversely, blockingof TRAF signaling with dominant negative mutants of TRAF5 andTRAF6, as well as inhibition of a downstream signal mediator p38MAPK, released the LMP1-induced oriP suppression. Furthermore,activation of TRAF6 signal cascade by lipopolysaccharides (LPS)resulted in loss of EBV from Burkitt's lymphoma cell line Akata,and inhibition of p38 MAPK abolished the suppressive effect ofLPS. These results suggested that the level of oriP activity isregulated by LMP1 and extracellular signals through TRAF5- andTRAF6-mediated signalcascades.

	INTRODUCTION

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Epstein-Barr virus (EBV) is related to Burkitt's lymphoma, T-cell lymphoma, gastric carcinoma, infectious mononucleosis, andopportunistic lymphoma in immunosuppressed patients (31), butresting memory B lymphocytes are normal cells infected latentlywith EBV in vivo (43, 44). During latent infection, the 170-kbEBV genome forms a circular plasmid DNA and is maintained by the2.2-kb region oriP containing an origin of bidirectional DNA replication(62, 64). oriP is comprised of two EBNA1-binding elements,dyad symmetry (DS) and family of repeats (FR), separated by 960bp. The DS element functions as a replication origin (16, 20,43, 55, 65), and the FR element plays a major role in nuclearretention of the genome (26, 41). DNA replication from oriP(DS-dependent replication) requires only the viral oriP-bindingprotein EBNA1 and occurs once in a single S phase through a mechanismof replication licensing (21, 56, 62, 63). However, itis not known whether oriP's replicator activity is regulated byvirus proteins or extracellularsignals.

In contrast to these studies, in some EBV-positive lymphoma cell lines, replication of the EBV genome is initiated mostlyin a broad initiation zone distant from oriP (DS-independent replication)(25). The occurrence of DS-independent replication was initiallyfound in Raji and Daudi by 2D gel analysis (38) and then wasdemonstrated using the oriP-containing plasmid in several celllines, including C33, HEK293, and P3HR1 (2, 35; unpublished data).Recently, Norio et al. (49) showed more direct evidence, usingrecombinant EBV virus, that the DS element is dispensable forEBV replication in BL30 and a P3HR1 clone. When DS-independentreplication occurs, the DS-dependent replication from oriP israre (38). The initiation region used for DS-independent replicationmay be preferentially used over oriP in lymphomas. Alternatively,the oriP activity may be negatively regulated by latent virusproteins expressing in these cell lines. To explore this possibility,we examined the effect of latent membrane protein 1 (LMP1) onoriP activity. LMP1 is an EBV integrated membrane protein thatplays an essential role in immortalization of human B lymphocytesby EBV (29, 34, 45) and transforms rodent fibroblasts (3,61). LMP1 induces activation of several signal mediators: NF- $kappa$ B(22, 42), c-Jun amino-terminal kinase (JNK) (12, 32),extracellular signal-regulated kinases (ERKs) (52), p38 mitogen-activatedprotein kinase (MAPK) (13), and Janus kinase 3 (17). LMP1has two C-terminal terminal activating regions, CTAR1/TES1 (aminoacids [aa] 187 to 232) and CTAR2/TES2 (aa 351 to 386), which areresponsible for activation of these signal mediators. CTAR1/TES1contains the PxQxT motif that is a binding site for the tumornecrosis factor receptor-associated factors (TRAFs) (9, 22,42, 46). TRAFs are the signal mediators of the cellular membranereceptors of TNFR and Toll/IR-1R superfamilies and initiate distinctbut overlapping signal cascades (7, 23, 46, 47). Amongthe six TRAFs identified to date, TRAF1, TRAF2, TRAF3, and TRAF5but not TRAF6 associate with the PxQxT motif of CTAR1/TES1 (5,9, 10, 46, 52). TRAF2 also associates indirectly withCTAR2/TES2 via TRADD and RIP and mediates signal cascades leadingto activation of NF- $kappa$ B and JNK (12, 14, 24, 25, 32,33, 58).

In this study, we showed that oriP activity is negatively regulated by the TRAF5-mediated signal initiated from LMP1 and theTRAF5- and TRAF6-mediated signals from cellular receptors. Wealso identified the p38 MAPK, a common downstream kinase in thesesignal cascades, as playing an important role in this negativeregulation of EBVreplication.

	MATERIALS AND METHODS

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Plasmids. The oriP plasmid (KORI) containing the oriP region, the DS plasmid (KD11), the SV40 plasmid, and the internal control plasmidwere described previously (55, 56). The expression plasmidsof the LMP1 deletion derivatives were constructed from the LMP1expression plasmid pNH-LMP1 (59). The plasmids expressing theLMP1 point mutants were described elsewhere (25). The expressionplasmids of TRAF and their dominant negative mutants were alsodescribed elsewhere (27). A cDNA clone of mouse p38 MAPK wasobtained by PCR from 15-day embryos using primers according tothe p38 sequence (19) and was inserted into the expression vectorpactEF (50). The dominant negative p38 mutant, p38^AGF, was prepared by replacing the wild-type Thr¹⁸⁰ (ACA) and Tyr¹⁸² (TAC) with an Ala (GCC) and a Phe (TTC), respectively, by oligonucleotide-directedmutagenesis.

Transient replication assay. The oriP plasmid (2 µg) was transfected into HeLa/EB1 cells (2 × 10⁶) (55) with the unmethylated control plasmid (1 µg) and theeffector plasmid(s) by the calcium phosphate method. Transfectionefficiency was estimated as 50% on average. After transfection,cells were cultured for 2 days in the experiments described inFig. 1, 2, and 3, and for 3 days in the experiments describedin Fig. 4, 5, and 6. DpnI digestion and Southern hybridizationanalysis were performed as described previously (56) using theoriP region (EcoRI-SacII) as a hybridization probe. The salt concentrationin the DpnI reaction buffer was lowered to 50 mM in this study.Aliquots of about 1/10 of the extracts were used for a singleDpnI assay. Radioisotope signals on Southern blots were analyzedquantitatively with a BAS2000 image analyzer (Fuji). The samemembranes were rehybridized to detect the control plasmid. Thehybridization signal of the DpnI-resistant oriP plasmid was normalizedwith the signal of the internal control plasmid in the same sampleand was represented relatively to that of the vector-transfectedsample. Expression of LMP1 and of EBNA1 was analyzed using a monoclonalantibody against LMP1 (S12) and a rabbit polyclonal antibody againstEBNA1.

[³H]thymidine incorporation of the LMP1/GFP expressing cells. The pNH-LMP1 (0 to 4 µg) was transfected with the green fluorescent protein (GFP) expression plasmid pEGFP-C1 (4 µg) intoHeLa/EB1 (2 × 10⁶) in 100-mm dishes. Transfection efficiency was determined bycounting GFP-expressing cells at 24 h after transfection. Then,cells were replated into 96-well plates (2,000 cells in 200 µl)and were cultured for 4 h in the presence of [³H]thymidine (1 µCi). Incorporation by the GFP/LMP1-expressingcells (2,000 cells) was calculated using the following equation:cpm^G = [cpm^S $-$ (1 $-$ f) × cpm^O]/f, where cpm^G is uptake by GFP-expressing cells; cpm^S is total uptake by cells transfected with the GFP plasmid andthe LMP1 plasmid; cpm^O is total uptake by cells transfected with the GFP plasmid alone;and f is the ratio of GFP-expressingcells.

NF- $kappa$ B activity. The NF- $kappa$ B reporter plasmid p $kappa$ B-tkLuc (27) (2 µg) was transfected with pSV- $beta$ -gal (1 µg) and pNH-LMP1 (1 µg) into HeLa/EB1(10⁶) in 60-mm dishes. Luciferase activity was determined 2 days aftertransfection, and $beta$ -galactosidase activity was used as internalcontrol.

Stimulation of Burkitt's lymphoma B cell lines. Bacterial lipopolysaccharide (LPS) (Difco) (5 mg/ml) was added at 10 µg/ml to growing B cells (15 ml; 10⁵ cells/ml). Two days after stimulation, cells (10 ml) were collected.Fresh culture medium containing LPS (10 ml) was added to the restof the cells (5 ml), which were then cultured again for 2 days.Total DNA was prepared from these LPS-stimulated cells and unstimulatedcells. The total DNA (4 µg) was digested with BamHI and analyzedby Southern hybridization methods using an EBV (B95-8) BamHI-Cfragment for a probe. Hybridized signals were analyzed quantitativelywith a BAS2000 imageanalyzer.

	RESULTS

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Expression of LMP1 induced suppression of oriP plasmid replication in HeLa/EB1 cells. We have previously demonstrated that when the dam-methylated oriP plasmid is transfected into HeLa/EB1 cells, the DpnI-resistantreplicated oriP plasmid is accumulated during 2 days after transfection(55, 56; Fig. 1A). When we analyzed the recovered oriP plasmidby DpnI digestion and Southern hybridization using the oriP regionfor a probe, we detected one linearized DpnI-resistant plasmid(5.0 kb) and five DpnI-digested fragments (2.5, 1.8, 1.3, 0.8,and 0.6 kb). The 0.8-kb and 0.6-kb fragments are not shown inthe figures. Among these DpnI-digested fragments, the 1.8-kb,0.8-kb, and 0.6-kb fragments were predicted from the restrictionsites. The 2.5-kb and 1.3-kb fragments were the products of replicationintermediates accumulated by a replication fork barrier at anFR element (16). Therefore, the amount of these replicationintermediates was less than that of the 1.8-kb DpnI-digested fragmentand related to the amount of replicated DpnI-resistant plasmid.To examine the effect of LMP1 expression on oriP activity, wecotransfected the LMP1 expression plasmid in this transient replicationassay and found that expression of LMP1 significantly suppressedreplication of the oriP plasmid (Fig. 1A). The amount of replicatedplasmid was normalized to the amount of the internal control plasmidin the same sample and then was compared. The replicated plasmidin the LMP1-transfected cells was about 5% of that of the vector-transfectedcells. We also examined the other latent membrane proteins LMP2Aand LMP2B but observed only a weak suppression of oriP activity.Western analysis confirmed that expression of LMP1 did not affectexpression of EBNA1, suggesting that insufficient expression ofEBNA1 was not a cause of oriP suppression (Fig. 1B). Like theoriP plasmid, the DS plasmid containing only the replication originwas also sensitive to LMP1 expression, indicating that the originelement was responsible for LMP1-induced suppression (Fig. 1C).Suppressive effects of LMP1 continued for at least 4 days, whileexpression of LMP1 was highest 1 day after transfection and thendecreased significantly at later time points (Fig. 1D). We thenexamined the dose dependency of the LMP1 plasmid for oriP suppressionand found that the lowest dose of LMP1 plasmid (0.0625 µg) wassignificantly effective for oriP suppression (Fig. 2A). The amountof LMP1 plasmid required for 50% inhibition was 0.0625 µg for2 × 10⁶ cells (Fig. 2C). Fig. 2E shows the amount of LMP1 expressed inthese transfected cells. When 0.5 µg of LMP1 plasmid was transfectedinto 2 × 10⁶ cells, the amount of LMP1 was about equal to that expressed inan EBV-positive lymphoma cell line, Raji (results not shown).

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FIG. 1. Expression of LMP1 suppressed replication of the oriP plasmid in HeLa/EB1 cells. (A) Transient replication assay of the oriP plasmid. The oriP plasmid (2 µg), the control plasmid (1 µg), and the expression plasmid of LMP1, LMP2A, or LMP2B (0.5 µg) were transfected. Total amounts of plasmids were adjusted to 3.5 µg with the vector plasmid. Hirt's extracts were prepared 2 days after transfection, and plasmids were analyzed by DpnI digestion and Southern blot hybridization. The linearized DpnI-resistant plasmid (5.0 kb) and three DpnI-digested fragments (2.5, 1.8, and 1.3 kb) are shown. Two fragments indicated by asterisks (2.5 and 1.3 kb) are products of replication intermediates that were accumulated by the replication fork barrier at the FR element of oriP. Amounts of the DpnI-resistant plasmid (replicated plasmid) are normalized with that of the control plasmid and shown below. Data represent averages of three experiments with the standard errors (SE). (B) Expression of LMP1 and EBNA1 in transfected cells. Short polypeptides reacted with LMP1 antibody were digested products of LMP1. As a control, a similar number of LCL cells were analyzed in a parallel lane. (C) Replication assay of the DS plasmid. Experimental conditions are described above for panel A. Data represent averages of three experiments with the standard errors (SE). (D) Time course of the oriP plasmid replication. Transfected plasmids were the same as in panel A, and cells were collected for DpnI assay at the days indicated. A summary of two experiments is shown. Expression of LMP1 in one experiment is shown at the bottom. The same amount of total proteins was loaded on each lane.

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FIG. 2. The LMP1 plasmid dose dependency of oriP suppression. (A) Transient replication assay of the oriP plasmid. The oriP plasmid (2 µg), the control plasmid (1 µg), and the LMP1 plasmid (0, 0.0625, 0.25, 1, and 4 µg) were transfected. Total amounts of plasmids were 7 µg. Two fragments indicated by asterisks are products of replication intermediates. (B) Transient replication assay of the SV40 plasmid. The SV40 plasmid (2 µg) was transfected with other plasmids as described above for panel A. (C) Summary of experiments described in panels A and B. Data represent averages of two experiments with standard errors (SE). (D) Expression of LMP1 and EBNA1 in the transfected cells. (E) [³H]thymidine incorporation of the LMP1/GFP expressing cells. The LMP1 plasmid was transfected with pEGFP-C1 (4 µg). Data represent averages of three experiments with standard errors (SE).

A low level of LMP1 expression that induced oriP suppression did not inhibit cell growth. Several studies have demonstrated that high levels of LMP1 expression inhibit cell growth (11, 18, 30). To monitor thegrowth inhibitory effect of LMP1 in our transient replicationassay, we used the SV40 plasmid containing SV40 origin and theT-antigen gene (56). The SV40 plasmid was transfected with theLMP1 plasmid and its replication was analyzed at 2 days aftertransfection (Fig. 2B). In contrast to the oriP plasmid, a lowerdose of the LMP1 plasmid (0.0625 and 0.25 µg) did not suppressthe SV40 plasmid replication. With a higher dose of LMP1 plasmid(1 and 4 µg), replication of the SV40 plasmid was suppressed by60 and 40%, respectively, suggesting that the growth inhibitoryeffect of LMP1 appeared at these doses. To confirm this resultby another assay, [³H]thymidine incorporation by LMP1-expressing cells was examined.We transfected the same amount of the GFP plasmid (4 µg) withseveral different amounts of the LMP1 plasmid (0 to 4 µg) intoHeLa/EB1. ³H incorporation by the GFP-expressing cells was estimated fromthe ratio of GFP-positive cells and ³H incorporation by total cells. ³H incorporation by GFP-positive cells was not affected with lowerdoses of LMP1 plasmid (0.0625 and 0.25 µg) but was reduced by71 and 46% with higher doses (1 and 4 µg) (Fig. 2E). Thus, a lowerlevel of LMP1 expression that induced oriP suppression did notinhibit cellgrowth.

The TRAF-binding motif of LMP1 was mostly responsible for induction of oriP suppression. To determine the signal cascade leading to oriP suppression, we examined the LMP1 domain responsible for induction of oriPsuppression. An LMP1 mutant, LMP1 $Delta$ (351-386), had a deletion ofCTAR2 (aa 351 to 386) but retained CTAR1 (aa 187 to 232). Expressionof LMP1 $Delta$ (351-386) suppressed oriP replication to the same extentas that of the wild-type molecule (Fig. 3A). Similarly, LMP1 $Delta$ (212-386),in which CTAR2 and most of CTAR1 were deleted but the PxQxT motif(aa 204 to 208) was retained, also showed the wild-type function.However, complete deletion of CTAR1 and CTAR2, including the PxQxTmotif in LMP1 $Delta$ (187-386), eliminated most of the suppressive effect,and the internal deletion of CTAR1 in LMP1 $Delta$ (187-351) showed onlya weak suppressive effect. This indicated the importance of thePxQxT motif for oriP suppression, which was further confirmedusing LMP1 point mutants. The LMP1 mutant LMP1(PQT $right-arrow$ AAA) had aminoacid substitutions Pro²⁰⁴ to Ala, Gln²⁰⁶ to Ala, and Thr²⁰⁸ to Ala in the PxQxT motif and did not bind TRAFs (32, 33).As shown in Fig. 3A, LMP1(PQT $right-arrow$ AAA) lost most of the suppressiveeffect.

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FIG. 3. Mutational analysis of LMP1 domains for oriP suppression. (A) Transient replication assay of the oriP plasmid. The oriP plasmid (2 µg), the control plasmid (1 µg), and the LMP1 plasmid (0.5 µg) were transfected. Total amounts of plasmids were 3.5 µg. The amino acid numbers in parentheses indicate the region deleted from LMP1. Amino acid substitutions in the LMP1 point mutants are also shown in parentheses. Normalized amounts of DpnI-resistant plasmid are shown below. Data represent averages of three experiments with standard errors (SE). Activation of NF- $kappa$ B activity by these LMP1 mutants was examined using the p $kappa$ B-Luc luciferase reporter plasmid. Data represent averages of two experiments with standard errors (SE). (B) Expression of LMP1 and its point mutants. The same amount of total protein was loaded in each lane. (C) Structure of LMP1.

We also examined Tyr³⁸⁴ in CTAR2, the amino acid residue important for binding of the TRADD-TRAF2 complex (14, 24, 33).Unexpectedly, the point mutant LMP1(Y384G) showed complete lossof the suppressive effect, although CTAR2 was not required formost of the LMP1's suppressive effect (Fig. 3A). Western analysisconfirmed expression of a similar level of LMP1 protein (Fig.3B). As the Y384G mutation abolishes the binding of the TRADD-TRAF2complex to the CTAR2 domain, this result suggested that the absenceof the TRADD-TRAF2 complex on the CTAR2 domain may have induceda large conformational change in LMP1 and interfered with thefunction ofCTAR1.

Overexpression of TRAF5 and TRAF6 suppressed oriP activity. TRAF1, TRAF2, TRAF3, and TRAF5 associate with the PxQxT motif of CTAR1 (5, 9, 10, 46, 53). To identify the TRAF-mediatedsignal cascade leading to oriP suppression, we overexpressed eachTRAF in the absence of LMP1 and examined its effect on oriP activity.TRAF expression vectors used in this experiment were constructedwith the same mammalian expression plasmid, and cells were collected3 days after transfection because transfection of a large amountof plasmids reduced the efficiency of oriP replication. By thistransient replication assay, we found that overexpression of TRAF5,but not of TRAF2 or TRAF3, reduced oriP activity by 60% (Fig.4A). We also examined TRAF6, although it did not bind to the PxQxTmotif, and found that overexpression of TRAF6 suppressed oriPactivity to a similar extent as TRAF5.

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FIG. 4. Effects of TRAF expression on oriP activity. Shown are the results of a transient replication assay of the oriP plasmid. (A) Effects of single expression of TRAF. The oriP plasmid (2 µg), the control plasmid (0.5 µg), and the TRAF expression plasmid (4 µg) were transfected. Total amounts of plasmids were 6.5 µg. (B) Effects of coexpression of TRAFs. The oriP plasmid (2 µg), the control plasmid (0.5 µg), and the TRAF expression plasmids (4 µg each) were transfected. Total amounts of plasmids were 10.5 µg. (C) Effects of coexpression of TRAF and the dominant negative TRAF mutants, TRAF5DN and TRAF6DN. Normalized amounts of DpnI-resistant plasmid are shown below. Data represent averages of three experiments with standard errors (SE). Two fragments indicated by asterisks are products of replication intermediates.

Because TRAF2 or TRAF3 might work synergistically with TRAF5 and TRAF6, we examined combinations of TRAFs in a similar assay.However, coexpression of TRAF2 with TRAF5 or TRAF6 showed suppressiveeffects similar to those of TRAF5 and TRAF6 alone, indicatingthat TRAF2 did not interfere with the functions of TRAF5 or TRAF6(Fig. 4B). Coexpression of TRAF3 reduced TRAF5-induced oriP suppressionbut it did not affect TRAF6-induced suppression. In contrast,when TRAF5 and TRAF6 were coexpressed, their suppressive effectswere added and the oriP activity was reduced by 10%. This additiveeffect was not observed when one of TRAF5 and TRAF6 had a deletionin the effector domain (Fig. 4C). We also examined expressionof TRAF1. Like TRAF2, expression of TRAF1 neither suppressed oriPactivity nor interfered with the suppressive effects of TRAF5and TRAF6 (results notshown).

oriP was activated by inhibition of the TRAF-mediated signaling in HeLa/EB1. Because overexpression of TRAF5 and TRAF6 induced oriP suppression, we next examined the effects of inhibition of the TRAF-mediatedsignaling. Under normal culture conditions, the TRAF-mediatedsignal cascade was activated at a low level. We inhibited thisbasal activity of TRAF signaling by expressing the dominant negativemutant of TRAF, TRAFDN, which had deletions in the amino-terminaleffector domain. When TRAF5DN or TRAF6DN was expressed, oriP replicationwas moderately activated, by 126 or 150% (Fig. 5A). Coexpressionof TRAF5DN and TRAF6DN showed further activation, by 242%, indicatingthat the effects of TRAF5DN and TRAF6DN were added like thoseof TRAF5 and TRAF6. This result confirmed that TRAF5- and TRAF6-mediatedsignal cascades negatively regulated oriP activity and also indicatedthat oriP was sensitive to even a basal level of signaling inHeLa/EB1 cells.

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FIG. 5. Effects of dominant negative TRAF expression on oriP activity. Shown are the results of a transient replication assay of the oriP plasmid. (A) Effects of dominant negative TRAF (TRAFDN) in the absence of LMP1 expression. The oriP plasmid (2 µg), the control plasmid (0.5 µg), and the expression plasmids of TRAFDN (4 µg each) were transfected. Total amounts of plasmids were 10.5 µg. (B) Effects of dominant negative TRAFDN on LMP1-induced suppression. The oriP plasmid (2 µg), the control plasmid (0.5 µg), the TRAF expression plasmids (4 µg each), and LMP1 $Delta$ (212-386) (0.25 µg) were transfected. Total amounts of plasmids were 10.75 µg. Normalized amounts of DpnI-resistant plasmid are shown at the bottom. Data represent averages of three experiments with standard errors (SE). Two fragments indicated by asterisks are products of replication intermediates.

Interestingly, expression of TRAF3DN also activated oriP replication by 150%, although overexpression of TRAF3 did not suppressoriP. Coexpression of TRAF3DN with TRAF5DN or TRAF6DN showed furtheractivation, by 215 and 325%, respectively. An in vitro study indicatedthat TRAF5 does not bind to the PxQxT motif directly, but thatTRAF3 forms TRAF3-TRAF5 hetero-oligomers through the amino-terminaleffector domain and mediates binding of TRAF5 to the motif (51).Because TRAF3DN lacked the effector domain, TRAF3DN competitivelyinhibited the binding of TRAF3-TRAF5 hetero-oligomers to the PxQxTmotif and inhibited TRAF5-mediated signaling. Therefore, TRAF3DNwas functionally similar toTRAF5DN.

We also examined the effects of TRAFDN on LMP1-induced suppression. Single expression of TRAF3DN or TRAF5DN did not affectthe LMP1 $Delta$ (212-386)-induced suppression of oriP activity, but coexpressionof both mutants partially released the suppression, confirmingthat TRAF5 mediated the LMP1-induced signal for oriP suppression(Fig. 5B). Although LMP1 does not bind TRAF6, TRAF6DN also partiallyreleased oriP suppression when it was coexpressed with TRAF3DNor TRAF5DN. This suggested that the LMP1-induced (TRAF5-mediated)signal and the TRAF6-mediated signal had a common downstream mediatorfor oriPsuppression.

The p38 MAPK regulated oriP activity. Because expression of LMP1, TRAF5, or TRAF6 induced activation of p38 MAPK in HeLa cells (4, 13; unpublished data), thekinase was a candidate common signal mediator for oriP regulation.We examined whether p38 MAPK was involved in the signal cascadeleading to oriP suppression. Under the condition that oriP replicationwas suppressed by about 35% with LMP1, expression of the dominantnegative mutant of p38 MAPK, p38^AGF, released the LMP1-induced oriP suppression by about 90% (Fig.6A). Similarly, treatment of cells with the specific inhibitorof p38 MAPK, SB203580 (20 µM), also released oriP suppression.In contrast, the wild-type p38 MAPK did not affect oriP replication.Because p38^AGF and SB203580 did not stimulate [³H]thymidine incorporation, these results suggested that p38 MAPKwas a downstream mediator of LMP1 for oriP suppression. Furthermore,in the absence of LMP1, expression of p38^AGF also activated oriP activity by 195%, and treatment with SB208530showed further activation, by 315%. This indicated that oriP activitywas negatively regulated by p38 MAPK and that its basal levelactivity in HeLa/EB1 cells reduced oriP replication by threefold.

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FIG. 6. Examination of the signal mediators that affect oriP activity. Shown are the results of a transient replication assay of the oriP plasmid. (A) The p38 MAPK. The oriP plasmid (2 µg), the control plasmid (0.5 µg), LMP1 $Delta$ (212-386) (0.25 µg), and the expression plasmid of p38 MAPK or the dominant negative mutant of p38 MAPK, p38^AGF (8 µg), were transfected. Total amounts of plasmids were 10.75 µg. The specific inhibitor for SB208350 was added into the culture medium at a concentration of 20 µM. (B) Ras and MEK. The oriP plasmid (2 µg), the control plasmid (0.5 µg), one of the expression plasmids of LMP1 (0.5 µg), c-H-ras (4 µg), the dominant active ras 12Vras (4 µg), or the constitutively active mutant of MEK1, MEK1^EE (4 µg), were transfected. Total amounts of plasmids were 6.5 µg. Normalized amounts of DpnI-resistant plasmid are shown at the bottom. Data represent averages of three experiments with standard errors (SE). Two fragments indicated by asterisks are products of replication intermediates.

We next examined the involvement of the ras-raf1-MEK-ERK signal pathway in oriP regulation (52). Expression of the dominantpositive mutant of H-ras, 12Vras, and the constitutively activemutant of MEK1, MEK1^EE, were reported to induce activation of ERKs. However, expressionof 12Vras and MEK1^EE did not suppress oriP activity (Fig. 6B). Thus, activation ofthe ERK signal pathway did not induce oriP suppression. We alsoanalyzed NF- $kappa$ B activation by LMP1 mutants and compared it withtheir ability to induce oriP suppression. LMP1 $Delta$ (351-386) and LMP1 $Delta$ (212-386)suppressed oriP replication as effectively as the wild type butthese mutants did not activate NF- $kappa$ B (Fig. 3). In contrast, LMP1 $Delta$ (187-351)and LMP1(PQT $right-arrow$ AAA) suppressed oriP only weakly but they activatedNF- $kappa$ B similarly to the wild-type LMP1. These results indicatedthat distinct domains of LMP1 induced activation of NF- $kappa$ B andoriP suppression. Similarly, CTAR2 and the region between CTAR1and CTAR2 were essential for activation of JNK and Janus kinase3, respectively (12, 17, 32), but both regions were dispensablefor oriP suppression (Fig. 3).

Activation of the TRAF6-mediating signal cascade by LPS resulted in loss of the EBV genome from Akata. Given the results suggesting that activation of TRAF5- and TRAF6-mediating signal cascades suppresses replication of the oriPplasmid in HeLa/EB1 cells, we next examined whether the same signalingsnegatively affected EBV replication in the infected cells. Tosee the suppression of oriP activity, it was essential that theEBV genome was maintained predominantly by the DS-dependent replicationfrom oriP in the infected cells. A Burkitt's lymphoma cell line,Akata, showed the latency type I phenotype and did not expressLMP1. In addition, the spontaneous loss of Akata EBV was alsoreported (54). Therefore it was very likely that Akata EBV wasmaintained by the DS-dependent replication from oriP. To activateTRAF-mediated signal cascades, we used LPS. It was shown thatLPS activated cells through Toll-like receptors, and TRAF6 wasthe signaling mediator from Toll-like receptors to NF- $kappa$ B and MAPKs(1, 28, 39, 40). We cultured growing Akata cells (10⁵ cells/ml) in the presence of 10 µg of LPS/ml for 2 or 4 days.To examine the copy number of the Akata EBV genome, total DNAwas prepared from these cells and was analyzed by Southern blothybridization using the same amount of DNA (4 µg) and a BamHI-Cfragment for a probe. As shown in Fig. 7A, Akata EBV decreasedsignificantly after LPS stimulation. Quantitative analysis indicatedthat EBV DNA was decreased by 28% during 4 days of LPS stimulation.In a control experiment, we examined another Burkitt's lymphomacell line, Raji. Raji EBV DNA was maintained by the replicationinitiated in a region out of oriP (DS-independent replication)(38), and oriP was not used for replication origin, presumablybecause the cell expressed LMP1. As we expected, activation ofthe TRAF6 signal cascade by LPS did not reduce the copy numberof Raji EBV, suggesting that LPS stimulation suppressed the oriPactivity in Akata. We also examined Daudi EBV replication foranother control. Like Akata, Daudi did not express LMP1 but DaudiEBV was replicated by both DS-dependent and DS-independent mechanisms(38). LPS stimulation resulted in only a little loss of DaudiEBV. These results suggested that activation of the TRAF6 signalcascade suppressed EBV replication in the infected cells whenEBV was maintained by the DS-dependent replication from oriP.To confirm that p38 MAPK mediated the signal cascade leading tothe suppression of Akata EBV replication, Akata cells were stimulatedwith LPS in the presence of SB208350. As shown in Fig. 7B, whenp38 MAPK was inhibited, Akata EBV was not lost by LPS stimulation.We also examined the effects of SB208350 on replication of theEBV genome in infected cells. In contrast to HeLa/EB1, in whichinitial accumulation of the replicated oriP plasmid was increasedby inhibiting the basal activity of p38 MAPK, similar treatmentof the EBV-infected cells for 4 days did not increase the copynumber of Akata and Raji EBV. Similar results were also obtainedwith LCLs and AG876 cell lines (data not shown).

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FIG. 7. LPS simulation resulted in loss of Akata EBV. (A) LPS stimulation of EBV-infected B cell lines. Cells (10⁵ cells/ml) were stimulated with 10 µg of LPS/ml for 2 or 4 days. Total DNA of these stimulated and unstimulated cells (4 µg) was digested with BamHI and was analyzed by Southern blot hybridization using an EBV(B95-8) BamHI-C fragment for a probe, which cross-hybridized with BamHI-W (3.1 kb). For the loading controls, EtBr-staining images of agarose gels are shown in the middle panel. Hybridization signals were measured and shown as a relative copy number in the lower panel. Raji and Daudi EBVs were replicated by the DS-independent mechanism (16). (B) The effects of SB208350 on EBV replication. EBV-infected B cell lines (10⁵/ml) were cultured in the presence of the specific inhibitor for p38 MAPK SB208350 (20 µM) with or without LPS stimulation (5 µg/ml) for 4 days. Total DNA (4 µg) was prepared and analyzed as described above for panel A. Hybridization signals of the BamHI-C fragment are shown in the left panels. EtBr-staining images of agarose gels are shown in the right panels.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We demonstrated that the replicator activity of oriP was negatively regulated by the TRAF5-mediated signal cascade from LMP1and the TRAF5 and TRAF6 signal cascades from cellular receptors.This negative regulation was shown in the transient replicationassay of the oriP plasmid and was also demonstrated in the analysisof Akata EBVreplication.

While the DS element of oriP initiates DNA replication, the FR element of oriP functions as a replication terminator wheretwo replication forks proceeding to opposite directions meet anda round of DNA replication is completed (16). After bidirectionalreplication is initiated from the DS element, one replicationfork proceeds through most of the EBV plasmid, and the other forkproceeds only a short distance, directly to the FR element inthe opposite direction. Two-dimensional gel analysis showed thatthis replication fork, after a short distance, was stopped bya replication fork barrier at the FR element, and the replicationintermediates were accumulated (16). In the transient replicationassay of the oriP plasmid replication, we found that two DpnI-digestedoriP fragments (2.5 and 1.3 kb) were not predicted from the DpnIsites in oriP. Amounts of these fragments are roughly relatedto that of the DpnI-resistant oriP plasmid. Longer enzyme digestionand use of excess enzymes did not reduce these products, indicatingthat the fragments were not products of incomplete digestion ofDpnI. Furthermore, these fragments were not detected in the sampleswhen the oriP plasmid was transfected into replication-incompetentHeLa cells (55) and the DS plasmid lacking the FR element wastransfected into HeLa/EB1 cells (Fig. 1B). From these results,we considered that these DpnI-sensitive fragments are productsof replication intermediates that were accumulated by the replicationfork barrier at the FRelement.

The LMP1 expression required to suppress 90% of oriP activity was almost equal to that in Raji cells. This indicated thatoriP activity was sensitive enough to be suppressed by LMP1 expressedin EBV-infected cells. TRAF1, TRAF2, TRAF3, and TRAF5 bind tothe PxQxT motif of LMP1 (5, 9, 10, 46, 53). TRAF1participates in the antiapoptotic activity of LMP1 (6, 60)and does not mediate regulation of oriP. TRAF2 and TRAF5 initiatesignal cascades which are overlapped in the activation of NF- $kappa$ Band JNK. However, only TRAF5 regulates oriP activity through p38MAPK. Thus, activation of the signal cascade leading to oriP suppressionis a TRAF5-specific function. TRAF3 facilitates the function ofTRAF5 by binding the TRAF3-TRAF5 hetero-oligomer to LMP1 (51).In addition, TRAF3 may mediate its own signal cascade, becauseoverexpression of TRAF3 reverses the TRAF5-induced oriP suppression.This suggests the importance of balance between TRAF3 and TRAF5in this signal transduction. TRAF6 binds to CD40, RANK, and p75NGFR and also associates with IL-1R indirectly. As with TRAF5,overexpression of TRAF6 activates NF- $kappa$ B, JNK, and p38 MAPK. Ourresults suggest that p38 MAPK is a common downstream mediatorfor oriP suppression in the signal cascades activated by LMP1,TRAF5, andTRAF6.

Eliopoulos et al. (13) showed that both CTAR1 and CTAR2 of LMP1 contribute to activation of p38 MAPK. In contrast, our resultsshowed that CTAR1 contributed mostly for oriP suppression andthe contribution of CTAR2 was only a part. There are four isozymesof p38 MAPK, p38 $alpha$ , p38 $beta$ , p38 $gamma$ , and p38 $delta$ . Among these isozymes,p38 $alpha$ and p38 $beta$ are sensitive to SB203580 and appear to mediatedistinct functions (15). A difference in the contribution ofCTAR1 and CTAR2 to p38 activation and oriP suppression may beexplained by identifying the p38 isozyme that is activated byLMP1 and suppresses oriP activity. The p38 MAPK is activated byphosphorylation by MAPK kinases (MAPKK) MAKK3 and MAKK6. TheseMAPKKs are activated by a group of MAPKK kinases (MAPKKK). SinceMAPKKKs also activate the signal pathways leading to JNK, theremay be cross-talk between the signal pathways leading to p38 MAPKand JNK (8). This suggests that the signal pathway initiatedfrom CTAR2 and leading to JNK activation may also contribute tooriP suppression. Our results showed that LMP1 mutants lackingCTAR1 but retaining CTAR2, LMP1 $Delta$ (187-351), induced oriP suppressionweakly. A mechanism by which p38 MAPK suppresses oriP activityis not yet known. The p38 MAPK may modify EBNA1 directly or indirectlyinnuclei.

We confirmed that TRAF-mediated signaling suppressed oriP activity in EBV-infected B cells (Fig. 7). Using EBV-positive Burkitt'slymphoma cell line Akata, we showed that activation of the TRAF6-mediatedsignal cascade with LPS decreased the copy number of EBV by 28%after stimulation for 4 days (Fig. 7). Loss of 72% of the genomecopy during three cell cycles corresponded to 74% suppressionof EBV replication in each cell cycle, indicating that suppressionwith LPS stimulation was significant. The specificity of thissuppression of EBV replication was shown by the result that LPSstimulation did not suppress replication of Raji EBV that wasmaintained by the DS-independent replication. Furthermore, weshowed that p38 MAPK was involved in suppression of both EBV andthe oriP plasmid replication, suggesting that the same mechanismregulated negatively the oriP activity of Akata EBV and the oriPplasmid in HeLa/EB1 cells. Consistent with these results, spontaneousloss of the EBV genome was observed in the EBV-positive Burkitt'slymphoma cell lines Akata and Mutu (54, 57).

In HeLa/EB1 cells, the p38 MAPK was activated at a low level under normal culture conditions, which was enough to suppressthe initial accumulation of the replicated oriP plasmid by 30%(Fig. 5 and 6). This negative pressure imposed on oriP activitymay cause constant loss of the oriP plasmid from transfected cellsfor longer cultures, which was reported in several studies (41,56, 62). In contrast to HeLa/EB1, inhibition of p38 MAPK bySB208350 under unstimulated conditions did not increase AkataEBV in a short time (4 days). We speculated that the basal activityof p38 MAPK was lower in Akata than in HeLa/EB1 and may suppressAkata EBV replication only slightly in normal culture conditions.This is also consistent with the observation that spontaneousloss of Akata EBV (54) was a relatively slow process comparedto LPS-induced loss (Fig. 7A).

Latently infected EBV appears to replicate by two distinct mechanisms, DS-dependent replication and DS-independent replication.The DS-dependent replication is initiated from the DS elementof oriP and requires EBNA1 for initiation of DNA replication (62,64). In contrast, DS-independent replication is initiated ina broad region out of oriP and EBNA1 functions only for maintenanceof the EBV chromosome (38). DS-independent replication appearsto be performed by cellular replication factors without EBNA1and is activated only in certain cell lines (unpublished data).DS-dependent and DS-independent mechanisms are not mutually exclusiveand occur simultaneously, as is observed in Daudi. Another significantdifference in these replication mechanisms is in their sensitivityto LMP1- and TRAF-induced signaling. As we showed in this study,activation of these signal cascades suppressed DS-dependent replicationbut not DS-independent replication. Based upon this knowledgeof EBV replication, it is possible to make several speculationsabout latent infection of EBV. When latent EBV is replicated mainlyby the DS-dependent mechanism, activation of TRAF5 and TRAF6 signalcascades or induction of LMP1 expression suppresses DS-dependentreplication and the copy number of the EBV genome in infectedcells may decrease. Normal cells infected latently with EBV invivo are resting memory B cells (43, 44), which are eventuallyactivated by CD4⁺ T cells. Upon activation, TRAF5- and TRAF6-mediated signalingare initiated from CD40, TNFRII, and IL-1R. Therefore, when theEBV-infected B cell is latency phenotype I (EBNA1-only cells),it is likely that oriP activity is suppressed in activated B cellsand EBV may be reduced or eventually lost from activated B cells.In contrast, when latent EBV is maintained predominantly by DS-independentreplication, expression of LMP1 does not suppress latent EBV replication.Therefore, this type of infected cell can express LMP1 continuously.In vitro experiments have shown that continuous expression ofLMP1 induced immortalization and the transformation phenotypein cultured cells (3, 34, 45, 61). Therefore, activationof DS-independent replication may facilitate lymphoproliferativedisorders. It is unknown why some cell lines activate DS-independentreplication of EBV but others do not. Because most B cell linesthat were infected with EBV in vitro are latency phenotype IIIand expressing LMP1, activation of DS-independent replicationmay be related to immortalization ofcells.

The DS-independent mechanism of EBV replication is apparently important in establishing the latent infection status in vitro,because LMP1 is expressed in both EBV-infected peripheral bloodmononuclear cells and immortalized LCL clones established later.However, EBV can promote cell growth without expression of LMP1by expressing virus-encoded poly(A) RNA EBER (36, 37). Interestingly, when EBV-infected celllines are prepared using normal gastric epithelial cells, theEBV-infected epithelial cells do not express LMP1 (48). Therefore,the DS-dependent replication from oriP may also play an importantrole during infection and establishing of the latent state innonlymphoidcells.

	ACKNOWLEDGMENTS

We thank E. Kieff for the S12 antibody and cDNA clones of TRAF1, TRAF2, and TRAF3, W. Hammerschmidt and A. Kieser for theLMP1 mutant plasmids, G. Mosialos for the TRAF1 clone, H. Nakanofor TRAF5 clones, J. Inoue for TRAF6 clone, and H. Kitayama forras mutantclones.

This work is supported in part by a Grant-in-Aid for Scientific Research from the Ministry of Education, Science, Sports andCulture ofJapan.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Tumor Virology, Division of Virology and Immunology, Medical ResearchInstitute, Tokyo Medical and Dental University, Yushima 1-5-45,Bunkyo, Tokyo 113-8510, Japan. Phone: (81)-3-5803-5815. Fax: (81)-3-5803-0241.E-mail: shirakata.creg{at}mri.tmd.ac.jp.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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52. Roberts, M. L., and N. R. Cooper. 1998. Activation of a ras-MAPK-dependent pathway by Epstein-Barr virus latent membrane protein 1 is essential for cellular transformation. Virology 240:93-99[CrossRef][Medline].

53. Sandberg, M., W. Hammerschmidt, and B. Sugden. 1997. Characterization of LMP-1's association with TRAF1, TRAF2, and TRAF3. J. Virol. 71:4649-4656[Abstract].

54. Shimizu, N., A. Tanabe-Tochikura, Y. Kuroiwa, and K. Takada. 1994. Isolation of Epstein-Barr virus (EBV)-negative cell clones from the EBV-positive Burkitt's lymphoma (BL) line Akata: malignant phenotypes of BL cells are dependent on EBV. J. Virol. 68:6069-6073[Abstract/Free Full Text].

55. Shirakata, M., and K. Hirai. 1998. Identification of minimal oriP of Epstein-Barr virus required for DNA replication. J. Biochem. 123:175-181[Abstract/Free Full Text].

56. Shirakata, M., K. Imadome, and K. Hirai. 1999. Requirement of replication licensing for the dyad symmetry element-dependent replication of the Epstein-Barr virus oriP minichromosome. Virology 263:42-54[CrossRef][Medline].

57. Srinivas, S. K., J. T. Sample, and J. W. Sixbey. 1998. Spontaneous loss of viral episomes accompanying Epstein-Barr virus reactivation in a Burkitt's lymphoma cell line. J. Infect. Dis. 177:1705-1709[Medline].

58. Sylla, B. S., S. C. Hung, D. M. Davidson, E. Hatzivassiliou, N. Malinin, D. Wallach, T. D. Gilmore, E. Kieff, and G. Mosialos. 1998. Epstein-Barr virus-transforming protein latent infection membrane protein 1 activates transcription factor NF- $kappa$ B through a pathway that includes the NF- $kappa$ B-inducing kinase and the I $kappa$ B kinases IKK $alpha$ and IKK $beta$ . Proc. Natl. Acad. Sci. USA 95:10106-10111[Abstract/Free Full Text].

59. Takanashi, M., J. Li, M. Shirakata, S. Mori, and K. Hirai. 1999. Tumorigenicity of mouse BALB/c 3T3 fibroblast cells which express Epstein-Barr virus-encoded LMP1 and show normal growth phenotypes in vitro is correlated with loss of transforming growth factor- $beta$ 1-mediated growth inhibition. Arch. Virol. 144:241-257[CrossRef][Medline].

60. Wang, C., M. W. Mayo, R. G. Korneluk, D. V. Goedel, and A. S. Baldwin, Jr. 1998. NF- $kappa$ B antiapoptosis: induction of TRAF1 and TRAF2 and c-IAP1 and c-IAP2 to suppress caspase-8 activation. Science 281:1680-1683[Abstract/Free Full Text].

61. Wang, D., D. Liebowitz, and E. Kieff. 1985. An EBV membrane protein expressed in immortalized lymphocytes transforms established rodent cells. Cell 43:831-840[CrossRef][Medline].

62. Yates, J. L., N. Wallen, and B. Sugden. 1985. Stable replication of plasmids derived from Epstein-Barr virus in various mammalian cells. Nature 313:812-815[CrossRef][Medline].

63. Yates, J. L., and N. Guan. 1991. Epstein-Barr virus-derived plasmids replicate only once per cell cycle and are not amplified after entry into cells. J. Virol. 65:483-488[Abstract/Free Full Text].

64. Yates, J. L. 1996. Epstein-Barr virus DNA replication, p. 751-773. In M. L. DePamphilis (ed.), DNA replication in eukaryotic cells. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

65. Yates, J. L., S. M. Camiolo, and J. M. Bashaw. 2000. The minimal replicator of Epstein-Barr virus oriP. J. Virol. 74:4512-4522[Abstract/Free Full Text].

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55.	Shirakata, M., and K. Hirai. 1998. Identification of minimal oriP of Epstein-Barr virus required for DNA replication. J. Biochem. 123:175-181[Abstract/Free Full Text].
56.	Shirakata, M., K. Imadome, and K. Hirai. 1999. Requirement of replication licensing for the dyad symmetry element-dependent replication of the Epstein-Barr virus oriP minichromosome. Virology 263:42-54[CrossRef][Medline].
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59.	Takanashi, M., J. Li, M. Shirakata, S. Mori, and K. Hirai. 1999. Tumorigenicity of mouse BALB/c 3T3 fibroblast cells which express Epstein-Barr virus-encoded LMP1 and show normal growth phenotypes in vitro is correlated with loss of transforming growth factor- $beta$ 1-mediated growth inhibition. Arch. Virol. 144:241-257[CrossRef][Medline].
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