Interferon Regulatory Factor 7 Is Induced by Epstein-Barr Virus Latent Membrane Protein 1

doi:10.1128/JVI.74.3.1061-1068.2000

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Journal of Virology, February 2000, p. 1061-1068, Vol. 74, No. 3
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Interferon Regulatory Factor 7 Is Induced by Epstein-Barr Virus Latent Membrane Protein 1

Luwen Zhang¹^,²^,^* and Joseph S. Pagano¹^,²^,³

Lineberger Comprehensive Cancer Center,¹ Department of Medicine,³ and Department of Microbiology and Immunology,² University of North Carolina, Chapel Hill, North Carolina 27599-7295

Received 12 July 1999/Accepted 26 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Infection by Epstein-Barr virus (EBV) generates several types of latency with different profiles of gene expression but withexpression of Epstein-Barr nuclear antigen 1 (EBNA-1) in common.The BamHI Q promoter (Qp) is used for the transcription of EBNA-1mRNA in type I latency, which is an EBV infection state exemplifiedby Burkitt's lymphoma (BL). However, Qp is inactive in type IIIlatency, and other promoters (C/Wp) are used for transcriptionof EBNA-1, which raises the question of how usage of these promotersis governed. Interferon (IFN) regulatory factor 7 (IRF-7) wasidentified first as a negative regulator of Qp. Expression ofIRF-7 is associated with EBV type III latency, where Qp is inactive,but not with type I latency, raising the possibility that a viralgene product(s) expressed in type III latency might induce IRF-7and repress Qp. Here, detailed analysis of the expression of IRF-7revealed that it is associated with the expression of EBV latentmembrane protein 1 (LMP-1) and that LMP-1 stimulates the expressionof IRF-7 in type III latency in which Qp is inactive. In contrast,LMP-1 is not expressed in type I latency cells in which Qp isactive. LMP-1 represses the constitutive activity of Qp reporterconstructs. Mutational analysis of Qp reporter constructs revealedthat the Qp IFN-stimulated response element (ISRE) is essentialfor the repression by LMP-1. Furthermore, LMP-1 reduced EBNA-1mRNA derived from Qp only in type I cells in which IRF-7 couldbe induced. Finally, IFN- $alpha$ , but not IFN- $gamma$ , repressed endogenousQp activity, which is consistent with the ability of IFN- $alpha$ toinduce IRF-7. Thus, IRF-7 may mediate repression of Qp by LMP-1.The induction of IRF-7 by LMP-1 may be relevant to the silencingof Qp in EBV type IIIlatency.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The biologic hallmark of Epstein-Barr virus (EBV) and its usual interaction with B lymphocytes is latency. Several types oflatency with distinct patterns of viral gene expression have beendescribed. Type I latency is exemplified by Burkitt's lymphomas(BL) in vivo and earlier passages of cultured cell lines derivedfrom BL tissues. EBV nuclear antigen 1 (EBNA-1), and in some caseslatent membrane protein 2A (LMP-2A), is expressed in this formof latency (7, 35, 36, 41, 59). Several reports suggestthat a type I-like form of latency exists in healthy carriersof EBV (7, 35, 36, 41, 59). Interestingly, cells intype I latency can escape host immune surveillance because EBNA-1can interfere with its peptide presentation on major histocompatibilitycomplex class I molecules (29), which might explain the lifelongreservoir of virus in immunocompetent, seropositive persons. TypeIII latency is represented by lymphoblastoid cell lines establishedafter EBV infection of adult primary B cells in vitro, by someBL lines, and in B-cell lymphomas in immunodeficient states. Nineviral proteins, including six nuclear proteins (EBNA-1, EBNA-2,EBNA-3A, EBNA-3B, EBNA-3C, and EBNA-LP) and three integral membraneproteins (LMP-1, LMP-2A, and LMP-2B), are expressed. In addition,in all three forms of latency, EBV-encoded RNAs (EBERs) are expressed(reviewed in references 25 and 43).

EBNA-1 is the sole viral protein needed for the replication of the EBV episome and maintenance of the latent infection state;both events are essential for cell immortalization (reviewed inreferences 25 and 43). The promoter usage for expression ofEBNA-1 differs in different types of latency. In type I latency,the BamHI Q promoter (Qp) is used for the transcription of EBNA-1mRNA. However, in type III latency, Qp is silent, and the BamHIC and/or BamHI W promoters (C/Wp) are used. The biological consequenceof the Qp-to-C/Wp switch and the conversion to type III latencyis the expression of the full spectrum of latency genes (reviewedin references 25 and 43), which confers enhanced cell survival,growth, and invasive potential (8, 17, 19, 22, 53,60, 65).

Since Qp usage not only relates to the survival of the virus in an immunocompetent host but also is associated with severaltumors, dissecting the regulation of Qp is essential for understandingthe viral program in EBV-associated malignancies. The functionalimportance of Qp for the EBV life cycle is underscored by thefacts that all EBV-positive tumor specimens collected from Africa,North America, and Asia have conserved Qp sequence (58) andthat conserved structural and functional cis elements (e.g., aninterferon [IFN]-stimulated response element [ISRE] and the Qlocus [see Fig. 4A]) also exist in the Old World primate lymphocryptoviruses,which are simian EBVs (47). Both EBNA-1 and host factors areinvolved in the transcriptional regulation of Qp. The downstreamelement of Qp, the Q locus (Fig. 4A), contains two binding sitesfor the EBNA-1 protein, which binds to and acts in an autoregulatorymanner to repress Qp transcription (48, 56). However, E2F-1overcomes EBNA-1-mediated repression of Qp in transient transfectionassays, and E2F-1 binds to the Q locus and displaces the bindingof EBNA-1 (55), so that the promoter is regulated in a cellcycle-dependent manner (10).

An ISRE immediately upstream of the transcriptional initiation site has been discovered and appears to be essential for Qpconstitutive activity (39, 49, 56, 67). IFN regulatoryfactors (IRFs), which are a group of transcription factors withmultiple functions (reviewed in reference 37), have the potentialto bind to the Qp ISRE and to regulate the activity of Qp. Althoughthe major positive regulator of Qp through the ISRE is disputed(39, 49, 68), both IRF-2 and the newly identified IRF-7have been reported to be negative regulators of Qp (67, 68).IRF-7 is predominately expressed in lymphoid tissues, and foursplicing forms (IRF-7A, IRF-7B, IRF-7C, and IRF-7H) have beenidentified (4, 67). IRF-7A is apparently the major form ofIRF-7 in peripheral blood leukocytes (67).

LMP-1 can induce a variety of cellular genes and enhance cell survival, adhesion, and invasive potential (13, 22, 34,62, 63, 65). LMP-1 expression is also necessary for B-celltransformation by EBV. Here, we report that LMP-1 stimulates theexpression of IRF-7. Furthermore, LMP-1 can repress Qp activity.Because IRF-7 is a negative regulatory of Qp and LMP-1 is expressedin type III latency, induction of IRF-7 by LMP-1 may provide anindirect pathway for the silencing of Qp in type IIIlatency.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture. DG75 is an EBV-negative BL cell line (5); BL30 and BL41 are EBV-negative BL lines with EBV-infected counterparts generatedby in vitro infection with the P3HR1 strain (BL30-P3HR1 and BL41-P3HR1)or the B95-8 strain (BL30-B95-8 and BL41-B95-8) of EBV (6).Akata, Eli-BL (gift from Alan Rickinson), and Rael (gift fromRichard Ambinder) are all EBV-positive type I BL cell lines (27,45, 57). Jijoye and its derivative P3HR1 are EBV-positivetype III BL cell lines (2, 42). The stable cell lines expressingeither LMP-1 or EBNA-2 in BJAB or BL41 cells were gifts from FredWang (63). All cell lines described were maintained in RPMI1640 plus 10% fetal bovine serum. Suitable selection drugs wereadded to the stable cell lines as reported elsewhere (63).

Plasmids and antibodies. IRF-7A and EBNA-2 expression plasmids and IRF-7 antibody have been described elsewhere (40, 54, 67). pcDNA/CD4 is ahuman CD4 expression plasmid (gift from Jenny Ting). The $beta$ -galactosidaseexpression plasmid, pCMV $beta$ (6177-1), was purchased from Clontech.pQ1-CAT and pQ2-CAT are described elsewhere (68). The LMP-1expression plasmid, pcLMP-1, was a gift from Tomakazu Yoshizaki.pQ2M-CAT ( $-$ 173 to +5) was made by cloning the corresponding PCRfragment with mutations in ISRE sequence into pBS-CAT (14).The IRF-1 (C-20) and IRF-2 (C-19) antibodies were purchased fromSanta Cruz Biotechnology, Inc. The EBNA-2 monoclonal antibody,PE-2, and LMP-1 monoclonal antibody, S12, were derived from theirrespective hybridoma cell lines (31, 66). IFN-stimulated gene15 (ISG-15) monoclonal antibody (11) was a gift from ErnestBorden.

Western blot analysis with enhanced chemiluminescence. Separation of proteins by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) was done according to standardmethods. After the proteins were transferred to a nitrocelluloseor Immobilon membrane, the membrane was blocked with 5% nonfatdry milk in TBST (50 mM Tris [pH 7.5], 200 mM NaCl, 0.05% Tween20) at room temperature for 10 min. It was then washed brieflywith water and incubated with a primary antibody in 5% milk inTBST for 1 to 2 h at room temperature or overnight at 4°C. Afterbeing washed with TBST for 10 min three times, the membrane wasincubated with the secondary antibody at room temperature for1 h. It was then washed three times with TBST as before, treatedwith enhanced chemiluminescence (Amersham) or SuperSignal (Pierce)detection reagents, and exposed to Kodak XAR-5film.

Transient transfection, CAT assays and isolation of transfected cells. For DG75 and Akata cells, 10⁷ cells in 0.5 ml of medium with 5 to 10 µg of DNA were used for transfection with the use of aBio-Rad Gene Pulser (320 V and 925 µF). For Eli-BL cells, 50 µgof DNA was used at 320 V and 975 µF. Two days after transfection,cells were collected for chloramphenicol acetyltransferase (CAT)assay or for isolation of transfected cells. The CAT and $beta$ -galactosidaseassays were essentially the same as described elsewhere (16).The CAT assay results were analyzed on a Molecular DynamicsPhosphorImager.

For isolation of transfected cells, cells were collected after transfection and enrichment for CD4 positive cells was performedwith the use of anti-CD4 antibody conjugated to magnetic beadsas recommended by the manufacturer (Dynal, Inc.). The isolatedcells were used for the extraction of totalRNA.

RNA extraction and RPA. Total RNA was isolated from cells with the use of RNease total RNA isolation kit (Qiagen). RNase protection assays (RPA) wasperformed with total RNA with the use of an RNase Protection KitII (Ambion Inc.). The hybridization temperature was 45°C. Theglyceraldehyde-3-phosphate dehydrogenase (GAPDH) probe was suppliedby U.S. Biochemicals, Inc. The IRF-7 probe was generated withthe use of ApaLI-digested pBS-IRF7A as a template and T7 RNA polymerase.The protected region is nucleotides 1671 to 1890 of IRF-7A (67).This probe cannot distinguish various splicing forms of IRF-7.The EBNA-1 probe was described previously (68). Molecular weightmarkers were made with the use of a $gamma$ -³²P-labeled DNA marker, (ØX174 DNA/HinfI;Promega).

IFN. IFN- $alpha$ -2a was purchased from Hoffman La Roche Inc.; IFN- $gamma$ was from Genzyme. For IFN treatments, cells were treated with eitherIFN- $alpha$ (500 U/ml) or IFN- $gamma$ (500 U/ml) for 48 h and were collectedfor further analysis. The same amounts of H₂O or 1× phosphate-bufferedsaline were used as mocktreatments.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Expression of IRF-7 is associated with LMP-1 protein in type III latency. We have shown that high levels of IRF-7 and IRF-2 are associated with type III, but not type I, latency (67, 68), whichraises the possibility that a viral gene(s) may regulate the expressionof IRF-7 or IRF-2. Because only EBNA-1, and possibly LMP-2A, isexpressed in type I latency, but all of the latency proteins (EBNA-1,-2, -3A, -3B, and -3C, and LMP-1, -2A, and -2B) are expressedin type III latency, one or more viral genes expressed in typeIII latency may be responsible for the upregulation of IRF-2 andIRF-7.

To select a candidate gene(s), paired cell lines infected by EBV P3HR1 virus or the prototype B95-8 strain were examined.BL30-P3HR1 and BL30-B95-8 lines were established by infectingthe EBV-negative BL30 line with P3HR1 and B95-8 viruses, respectively.The BL41-P3HR1 and BL41-B95-8 lines were established similarly(6). B95-8 virus has all of the latency genes in its viralgenome, whereas the P3HR1 virus genome lacks the EBNA-2 gene anda portion of the EBNA-LP gene (2). The cell lines infectedwith P3HR1 virus did not express EBNA-2 and had a much lower levelof LMP-1, whereas both cell lines infected with B95-8 virus expressedhigh levels of LMP-1 because EBNA-2 can transactivate the LMP-1promoter (1, 15, 61, 64) (Fig. 1 and data not shown).The expression of IRFs in these lines was examined by Westernblotting with specific antibodies. IRF-7 was shown to be expressedat high levels in the two cell lines infected with B95-8 virus,both of which have a high level of LMP-1 (Fig. 1, lanes 3 and6). The levels of IRF-1 and IRF-2, on the other hand, did notcorrelate with the high levels of LMP-1 expression. The IRF-1level was high in all cell lines tested. These experiments wererepeated several times, and consistent results were obtained.Furthermore, the type III Jijoye cell line, which has high-levelexpression of LMP-1 and is the parental line for P3HR1 cells,has a higher level of IRF-7 than P3HR1 cells, which have a lowerLMP-1 level (data not shown).

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FIG. 1. Association between the expression of IRF-7 and LMP-1. Equal amounts of protein lysates from the indicated cell lines were separated by SDS-PAGE (10% gel) and stained with Ponceau S red after transfer of protein to the membrane. Western blotting with IRF-7, IRF-1, IRF-2, and LMP-1 antibodies was performed.

These data strongly suggest that high-level expression of IRF-7 in type III latency is associated with the expression of LMP-1.In contrast, an association of IRF-1 and IRF-2 with EBV proteinexpression was notapparent.

LMP-1 stimulates the expression of IRF-7 protein. Since there was a consistent association between high levels of LMP-1 in type III latency and IRF-7, whether LMP-1 could directlystimulate IRF-7 was examined in stable cell lines expressing eitherLMP-1 or EBNA-2 (Fig. 2). MMLM-6 and MMLM-18 are EBV-negativeBJAB lines expressing LMP-1 protein constitutively, whereas pZu2-4and pZu2-5 express EBNA-2 protein. pZ-3, gpt-1, and gpt-2 arevector control lines for the EBNA-2 (pZ-3) and LMP-1 (gpt-1 andgpt-2) lines (63). The expression of EBNA-2 and LMP-1 was confirmedby Western blot analysis with EBNA-2 or LMP-1 antibody. As shownin Fig. 2, expression of IRF-7 is higher in LMP-1-expressing lines(lanes 3 and 4) than it is in the negative control lines (lanes1 and 2). However, IRF-2 was not affected by LMP-1 expression.Neither the IRF-7 nor the IRF-2 level was stimulated in the EBNA-2-expressingcell lines (lanes 5 to 7).

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FIG. 2. LMP-1 increases levels of endogenous IRF-7 protein. Western blotting with IRF-7, IRF-2, LMP-1, and EBNA-2 antibodies was performed. Lanes 1 to 7, stable cell lines established from the EBV-negative BJAB cell line; lanes 3 and 4, LMP-1 expression lines (MTLM-6 and MTLM-18); lanes 6 and 7, EBNA-2 expression lines (pZu2-4 and pZu2-5); lanes 1 and 2, vector control lines for LMP-1 (gpt-1 and gpt-2); lane 5, vector control line for EBNA-2 (pZ-3); lanes 8 and 9, LMP-1 expression line in BL41 (BL41-MTLM c11; lane 9) and its control cell line (BL41-gpt-3; lane 8). n.s., nonspecific band in lane 5.

To address further whether LMP-1 could stimulate IRF-7, we used BL41-MTLM c11, a BL41 line stably transfected with an LMP-1expression plasmid (63). As shown in Fig. 2, expression of IRF-7is also higher in this LMP-1-expressing line than in its controlline, BL41-gpt-3 (lanes 8 and 9). These results suggest that LMP-1,but not EBNA-2, can stimulate the expression of IRF-7protein.

LMP-1 stimulates the expression of IRF-7 mRNA. Whether LMP-1 can increase IRF-7 mRNA was examined by RPA with a specific probe (see Materials and Methods for details). Ina pair of genetically identical lines, the IRF-7 mRNA level washigher in the type III line (Sav III), where LMP-1 is expressed,than in the type I line (Sav I), where there is no LMP-1 expression(Fig. 3, lanes 3 and 4). The difference in IRF-7 mRNA betweenthe two lines is more than 10-fold (Fig. 3). Also, the level ofIRF-7 mRNA is low in Eli-BL, Akata, and Rael cells (type I lines)but higher in Jijoye and CB95 cells (type III lines) (data notshown). Therefore, IRF-7 mRNA expression is also associated withtype III latency, in agreement with previous reports (39, 67).

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FIG. 3. LMP-1 increases endogenous IRF-7 mRNA. (A) IRF-7 and GAPDH probes were labeled with [ $alpha$ -³²P]UTP and used for RPA. Lanes 1 and 2, undigested IRF-7 and GAPDH probes; lanes 3 and 4, RNAs from Sav I and Sav III cells, respectively; lane 5, yeast tRNA; lanes 6 to 11, RNAs from transfected and concentrated DG75 cells; lanes 7 and 8, an LMP-1 expression plasmid was used for transfection; lanes 10 and 11, EBNA-2 expression plasmid; lanes 6 and 9, control vectors. Specific protection of IRF-7 and GAPDH mRNAs and undigested probes is indicated. (B) Short time exposure for GAPDH-protected areas. The IRF-7 mRNA in Sav III was 10.4-fold ± 1.9-fold higher than in Sav I. The enhancement of IRF-7 mRNA by LMP-1 was 2.4-fold ± 0.4-fold, whereas enhancement by EBNA-2 was 0.63-fold ± 0.2-fold. Data were obtained by normalizing IRF-7 levels to the GAPDH level with the use of a PhosphorImager.

Whether LMP-1 could increase IRF-7 mRNA was examined by transient transfection of LMP-1 and a CD4 expression plasmid intoDG75 cells, which is an EBV-negative line, and selecting transfectedcells by the use of anti-CD4 antibody-conjugated magnetic beads(see Materials and Methods for details). As shown in Fig. 3, LMP-1expression causes an increased level of IRF-7 mRNA (lanes 7 and8) compared with vector alone (lane 6). In contrast, EBNA-2 didnot stimulate the expression of IRF-7 mRNA (lanes 9 to 11). Westernblot analysis confirmed that IRF-7A protein was greater in amountin LMP-1-transfected cells than in pcDNA3-transfected cells (datanot shown). The mRNA data are also consistent with results fromWestern blot analyses of LMP-1- and EBNA-2-expressing lines (Fig.2). The data together suggest that LMP-1 stimulates the expressionof IRF-7mRNA.

LMP-1 represses the constitutive activity of Qp reporter constructs. Because IRF-7 has been shown to be a negative regulator of Qp (67, 68), the stimulation of IRF-7 by LMP-1 predicts thatLMP-1 might act indirectly as a negative regulator of Qp. To testthis idea, an LMP-1 expression plasmid and a Qp reporter constructwere cotransfected into DG75 cells, and CAT activity was assayed2 days later, with $beta$ -galactosidase activity as an internal transfectionefficiency control. The pQ2CAT construct was chosen to assay Qpactivity because the constitutive activity of pQ2CAT correlateswith endogenous Qp activity and is more responsive to IRF-7 (68).As shown in Fig. 4B, LMP-1 repressed activity of the Qp reporterconstruct (columns 1 to 3). EBNA-2 protein expression did notrepress Qp (column 4), which is consistent with the fact thatEBNA-2 does not induce IRF-7 (Fig. 2 and 3). Overexpression ofIRF-7 repressed Qp as expected (column 5). Furthermore, mutationsin the ISRE of Qp (Fig. 4A) prevented the repression by LMP-1or by IRF-7A (Fig. 4C). It should be noted that ISRE mutationgreatly reduced the constitutive activity of Qp as reported previously(39, 49, 56, 67).

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FIG. 4. Repression of Qp reporter constructs by LMP-1. (A) Schematic diagram of Qp and Qp reporter constructs. Open rectangle, ISRE; solid bars, E2F binding sites; ovals, EBNA-1 sites (Q locus). The RNA start site for Qp is indicated by an arrow (50). The mutations in the Qp ISRE are shown. (B) Repression of Qp by LMP-1 in B cells. DG75 cells were transfected with the reporter construct pQ2-CAT along with the pcDNA-3 vector (column 1), with 0.2 and 0.4 µg of LMP-1 expression plasmid pcLMP-1 (columns 2 and 3, respectively), with an EBNA-2 expression plasmid (column 5), or with pcDNA-IRF-7A (column 6). (C) Mutations in ISRE abolish the repression of Qp by LMP-1 and by IRF-7. DG75 cells were transfected with reporter construct pQ2M-CAT and pcDNA-3 (column 1), pcLMP-1 (column 2), or pcDNA-IRF-7A (column 3). (D) LMP-1 did not repress Qp reporter construct in Akata cells. Akata cells were transfected with the reporter construct pQ2-CAT and with pcDNA-3 vector (column 1) or with 0.2 and 0.4 µg of LMP-1 expression plasmid pcLMP-1 (columns 2 and 3, respectively). CAT assay results were normalized by $beta$ -galactosidase activity. CAT activity is expressed relative to the vector control level. Standard deviations are shown.

It is interesting that we did not detect any stimulation of IRF-7 expression after overexpression of LMP-1 in Akata cells(Fig. 5B). Therefore, whether LMP-1 could repress Qp reporterconstructs in these cells was tested. As shown in Fig. 4D, LMP-1failed to repress Qp in Akata cells. The Akata line is unusualin that some LMP-1-inducible genes cannot be induced in thesecells, and anti-human immunoglobulin G can trigger lytic replicationof EBV (46, 57). However, LMP-1 could activate NF- $kappa$ B in thisline (data not shown).

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FIG. 5. LMP-1 reduces the endogenous EBNA-1 mRNA transcribed from Qp in type I cells. (A) Reduction of endogenous EBNA-1 mRNA in cells transfected with an LMP-1 expression plasmid. RPA was performed with GAPDH and EBNA-1 probes with various RNAs. Lane 1, yeast RNA; lane 2, total RNA from DG75, an EBV-negative cell line; lanes 3 to 5, RNAs from Eli-BL cells transfected with pcDNA3, pcLMP1 (5 µg), and pcLMP1 (10 µg), respectively; lanes 6 and 7, RNAs from Akata cells transfected with pcDNA3 and pcLMP1, respectively. The relative EBNA-1 mRNA levels are shown. Data were analyzed by normalizing EBNA-1 mRNA levels to the GAPDH level with the use of a PhosphorImager. In LMP-1-transfected cells, the average EBNA-1 mRNA level (and standard deviation) relative to pcDNA3-transfected cells from four experiments was 0.52 ± 0.09. One representative experiment is shown. (B) Stimulation of IRF-7 by LMP-1 in Eli-BL cells. RPA was performed with GAPDH and IRF-7 probes with various RNAs. Lane 1, yeast RNA; lanes 2 to 4, RNAs from Eli-BL cells transfected with pcDNA3, pcLMP1 (5 µg), and pcLMP1 (10 µg), respectively; lanes 5 and 6, RNAs from Akata cells transfected with pcDNA3 and pcLMP1 respectively. One representative experiment is shown.

Since high-level expression of LMP-1 has been reported to have a toxic effect on some cells (12, 20), whether the reductionin Qp constitutive activity by LMP-1 was due to toxicity was examinedcarefully. First, there were no obvious differences in $beta$ -galatosidaseactivity with or without LMP-1. Second, an NF- $kappa$ B reporter constructwas activated with the expression of LMP-1 as expected (data notshown and references 28 and 46). Third, endogenous IRF-7 mRNAwas enhanced by LMP-1 in DG75 cells under the same transfectionconditions (Fig. 3). Therefore, the data suggest that LMP-1 canrepress Qp activity, and the repression is associated with IRF-7stimulation.

LMP-1 reduces endogenous EBNA-1 mRNA in type I latency cells. To test if LMP-1 represses endogenous Qp activity, the LMP-1 and CD4 expression plasmids were transfected into Eli-BL, a typeI cell line in which Qp is active. The RNA from the transfectedcells was isolated, and RPA with an EBNA-1-specific probe wasperformed. The Eli-BL line was chosen because LMP-1 could stimulatethe expression of IRF-7 in this line (Fig. 5B). As shown in Fig.5A, LMP-1 indeed reduced the level of EBNA-1 mRNA in Eli-BL cells(compare lanes 4 and 5 with lane 3). However, LMP-1 did not induceIRF-7 (Fig. 5B, lane 6) or reduce EBNA-1 mRNA in Akata cells (Fig.5A, lane 10). The EBNA-1 mRNA level in Akata cells is lower thanit is in Eli-BL cells, possibly because the EBV genome is lostin subpopulations of Akata (52), resulting in differences inviral genome copy numbers. The reduced level of EBNA-1 mRNA producedin Eli-BL cells by LMP-1 is most likely due to the repressionof Qp activity, because LMP-1 could repress the activity of Qpreporter constructs to a similar extent (Fig. 4B). These datasuggest that LMP-1 can repress the endogenous activity of Qp,and the repression is associated with the ability of LMP-1 toinduce the expression of IRF-7.

Repression of Qp by IFN is associated with the induction of IRF-7. Because IFN has been shown to induce the expression of IRF-7 (4, 32, 39), whether IFN can repress endogenous Qp wastested in the type I latency cells, Eli-BL and Rael; in both celllines, endogenous Qp is active. IFN- $alpha$ could induce the expressionof IRF-7 in Eli-BL cells but not in the Rael cell line (Fig. 6B,lanes 2 and 5). The reason that IFN- $alpha$ fails to induce IRF-7 inRael cells is unknown; however, the signal transduction pathwayfor IFN- $alpha$ in Rael cells is at least partially functional becausethe expression of ISG-15 could be greatly induced (Fig. 6C, lanes2 and 3; reference 11). IFN- $gamma$ could not induce IRF-7 in eithercell line (Fig. 6B, lanes 3 and 6), which is consistent with aprevious report (4). However, IFN- $gamma$ could enhance the expressionof Tap-2 (transporter associated with antigen processing 2), suggestingthat IFN- $gamma$ was functional as reported (data not shown; references30 and 44). Whether IFN represses the endogenous Qp was addressedwith the use of RPA with an EBNA-1-specific probe. Figure 6A showsthat IFN- $alpha$ indeed reduced the Qp-derived EBNA-1 mRNA in the Eli-BLcells (lane 4). In contrast, IFN- $alpha$ failed to repress Qp in theRael line, in which IFN- $alpha$ did not induce the expression of IRF-7(Fig. 6A, lane 7). The reduced level of EBNA-1 mRNA in Eli-BLcells is most likely due to the repression of Qp activity, becauseIFN- $alpha$ could repress the activity of Qp reporter constructs (datanot shown and reference 39). IFN- $gamma$ did not repress Qp in eithercell line, as expected (Fig. 6A, lanes 5 and 8). These data suggestthat IFN- $alpha$ can repress the endogenous activity of Qp. This effectis associated with the ability of IFN- $alpha$ to induce the expressionof IRF-7.

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FIG. 6. IFN- $alpha$ can repress endogenous Qp activity in type I cells. (A) Repression of endogenous Qp by IFN- $alpha$ in Eli-BL cells. Lanes 1 and 2, undigested GAPDH and EBNA-1 probes, respectively; lanes 3 to 8, RNAs from Eli-BL (lanes 3 to 5) or Rael (lanes 6 to 8) cells were used for RPA; lanes 3 and 6, mock treatment; lanes 4 and 7, IFN- $alpha$ treatment (500 U/ml, 48 h); lanes 5 and 8, IFN- $gamma$ treatment (500 U/ml, 48 h). The reduction of EBNA-1 mRNA by IFN- $alpha$ was 53%. Data were obtained by normalizing EBNA-1 levels to the GAPDH level with the use of a PhosphorImager. One representative experiment of two independent experiments performed is shown. (B) IFN- $alpha$ induces the expression of IRF-7 in Eli-BL cells. Protein lysates from Rael (lanes 1 to 3) or Eli-BL (lanes 4 to 6) cells from the same experiment as shown in panel A were separated by SDS-PAGE (8% gel) and stained with Ponceau S red after transfer of protein to the membrane. Lanes 1 and 4, mock treatment; lanes 2 and 5, IFN- $alpha$ treatment; lanes 3 and 6, IFN- $gamma$ treatment. Western blots with IRF-7 and $gamma$ -tubulin antibodies were performed. (C) IFN- $alpha$ induces ISG-15 expression in Rael cells. Equal amounts of protein lysates from Rael with IFN- $alpha$ treatment (lanes 2 and 3) or mock treatment (lane 1) were separated by SDS-PAGE (12% gel) and stained with Ponceau S red after transfer of protein to the membrane. Western blotting with ISG-15 antibody was performed. ns, nonspecific band.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

EBV can deregulate B-cell growth through activation of endogenous programs of cellular gene expression. At the same time,these deregulated cellular genes can modulate the program of viralgene expression. The switch from Qp to C/Wp usage, which allowstranscription of other EBNA proteins (EBNA-2, EBNA-3A, EBNA-3B,EBNA-3C, and EBNA-LP), produces a phenotypic conversion from typeI to type III latency. We previously identified a novel regulatorfor Qp, IRF-7, which is highly expressed in type III latency.In this work, LMP-1, a key type III latency protein, is identifiedas an inducer of IRF-7. First, IRF-7 is associated with type IIIlatency, in which LMP-1 is expressed (67). Second, high levelsof IRF-7 are associated with LMP-1 expression in EBV-infectedBL-30 and BL-41 cell lines (Fig. 1). Third, stable expressionof LMP-1 in EBV-negative BJAB as well as BL41 cell lines increasesthe endogenous expression of IRF-7 protein (Fig. 2). Fourth, transienttransfection of LMP-1 into DG75 or Eli-BL cells could increasethe endogenous expression of IRF-7 mRNA (Fig. 3 and 5). Fifth,a physiological level of LMP-1 seems also able to stimulate IRF-7mRNA expression (Fig. 3). More work is needed to dissect the domainsof LMP-1 required for induction of IRF-7.

Interestingly, it has been argued that the induction of bcl-2 by LMP-1 may be due to the selection of a cell population withhigh endogenous expression of bcl-2 (33). Since transient expressionof LMP-1 in DG75 or Eli-BL cells could stimulate the expressionof IRF-7, LMP-1 is more likely able to enhance IRF-7 expressiondirectly, rather than to select for a cell population with a highlevel of IRF-7. All of these data suggest that LMP-1 is a factornecessary for the stimulation of the expression of IRF-7 in EBV-infectedcells but not sufficient, as in the case of Akata cells. Akatacells may have a mutation(s) in the signal transduction pathwayof LMP-1.

The fact that LMP-1 can stimulate the expression of IRF-7, which is a negative regulator of Qp, predicts that LMP-1 may beable to repress Qp through IRF-7. First, there is no LMP-1 expressionin type I latency in which Qp is active; however, LMP-1 expressionin type III latency is associated with inactivation of Qp andinduction of IRF-7. Second, LMP-1 could repress the activity ofQp reporter constructs in DG75 cells and reduce the endogenousEBNA-1 mRNA from Qp in a type I cell line, Eli-BL (Fig. 4 and5). In both cell lines, IRF-7 could be induced by LMP-1 (Fig.3 and 5). Third, overexpression of IRF-7 could repress the activityof Qp reporter construct to an extent similar to that exhibitedby LMP-1 (Fig. 4B) and marginally reduce the endogenous EBNA-1mRNA derived from Qp (data not shown). Fourth, in Akata cellsLMP-1 could not induce the expression of IRF-7, and LMP-1 failedto repress activity of a Qp reporter construct and to reduce theendogenous EBNA-1 mRNA (Fig. 4B and 5). Fifth, mutations in theISRE of Qp abolished the repression by LMP-1 or IRF-7 (Fig. 4C).Also, EBNA-2 could not stimulate the expression of IRF-7 in DG75cells and did not repress Qp activity (Fig. 2 to 4). These datastrongly suggest that LMP-1 is a negative regulator of Qp andthat the repression may be mediated by IRF-7 through the Qp ISRE.However, since in IRF-7A-transfected cells the average EBNA-1mRNA level (and standard deviation) relative to pcDNA3-transfectedcells from five experiments was 0.68 ± 0.15 (data not shown),an additional factor(s) may cooperate with IRF-7 to repress Qpefficiently (68).

Interestingly, in type II latency, LMP-1 expression and an active Qp can coexist (for a review, see reference 43). One possibleexplanation is that LMP-1 in type II cells cannot induce IRF-7and thus fails to repress Qp. Preliminary results suggest thatthis scenario may be correct (data not shown and reference 68).More work is needed to address the relations among LMP-1, IRF-7,and Qp activity in type II latencycells.

It is apparent that Qp activity is a balanced outcome of positive and negative regulators, with IRFs strongly implicated inits regulation. In type III latency, Qp may be turned off by acombination of LMP-1, IRF-7, IRF-2, and higher levels of EBNA-1(9, 18, 51, 67, 68). The contribution of each repressorto the inactivation of Qp in type III latency needs to be addressedfurther. In contrast, in type I latency when Qp is active, lowlevels or absence of these negative factors plus some unidentifiedpositive regulator(s) presumably cause the activation of Qp. IRF-2has been proposed as a primary activator of Qp (39, 49), butthat conclusion is disputed (68), and the identity of the ISRE-mediatedactivator(s) is stilluncertain.

Finally, IFN- $alpha$ , but not IFN- $gamma$ , has been shown to induce the expression of IRF-7 (Fig. 6B; references 4, 32, and 39).As expected, IFN- $alpha$ , but not IFN- $gamma$ , could repress endogenous Qpactivity in type I cells (Fig. 6A). The repression seems to beassociated with the ability of IFN to induce IRF-7 as exemplifiedby Eli-BL cells. In contrast, Qp activity in Rael cells, in whichIRF-7 could not be induced by IFN- $alpha$ , was not repressed by IFN- $alpha$ (Fig. 6A). Thus, the data overwhelmingly support the idea thatIRF-7 is a mediator of Qp repression. Also, it is interestingthat primary EBV infection could apparently induce IFN- $alpha$ (26)and that proliferation of type III latency cells is resistantto IFN (3, 24). These observations together with the datareported here and in a previous report (67) suggest that IFN- $alpha$ by induction of IRF-7 silences Qp and favors usage of C/Wp andfacilitates expression of the EBV oncoproteins. This scenariocould function in primaryinfection.

LMP-1 is essential for the viral transformation process. Interestingly, some IRFs have oncogenic capability (21, 23, 38).Since the cellular function (especially oncogenic potential) ofIRF-7 is unknown, it is premature to speculate on the relationbetween the induction of IRF-7 by LMP-1 and the transformationprocess in B cells. Whether IRF-7 is involved in the pathogenesisof EBV-associated diseases and malignancies remains to bedetermined.

The present results expand the role of LMP-1 as a pleiotropic molecule in effecting deregulation of cellular genes. LMP-1has been shown to induce numerous cellular genes with a varietyof functions. LMP-1 is now presented as a stimulator of IRF-7that, in turn, mediates the repression of the principal type Ilatency promoter for EBNA-1, Qp, thus favoring the switch to theuse of type III latency promoters, C/Wp. The complexity of regulationof EBV's latency states is illustrated by the fact that the principalproduct transcribed from C/Wp is EBNA-2, which in turn amplifiesthe transcription of LMP-1. Thus, both viral and IRF pathwaysmay converge to determine latencystate.

	ACKNOWLEDGMENTS

We thank Fred Wang, Alan Rickinson, Richard Ambinder, and Ernest Borden for providing valuable reagents for this work. Wealso thank Shannon Kenney and Nancy Raab-Traub for critical readingof the manuscript, Matt Davenport and Val Zacny for editorialhelp, and Lihong Wu for technicalwork.

This work was supported in part by grants from the National Institute of Allergy and Infectious Diseases (AI 42372-01) andfrom the National Cancer Institute (CA 19014). L.Z. was supportedby NIH Individual National Research Service Award 5F 32CA67433.

	FOOTNOTES

^* Corresponding author. Mailing address: Lineberger Comprehensive Cancer Center, University of North Carolina, Campus Box 7295,Chapel Hill, NC 27599. Phone: (919) 966-1183. Fax: (919) 966-9673.E-mail: luzhang{at}med.unc.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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