Characterization of the CBF2 Binding Site within the Epstein-Barr Virus Latency C Promoter and Its Role in Modulating EBNA2-Mediated Transactivation

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J Virol, January 1998, p. 693-700, Vol. 72, No. 1
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Characterization of the CBF2 Binding Site within the Epstein-Barr Virus Latency C Promoter and Its Role in Modulating EBNA2-Mediated Transactivation

Ezequiel M. Fuentes-Pananá and Paul D. Ling^*

Division of Molecular Virology, Baylor College of Medicine, Houston, Texas 77030

Received 25 August 1997/Accepted 8 October 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The Epstein-Barr virus (EBV) EBNA2 protein is a transcriptional activator that regulates viral and cellular gene expressionand is also essential for EBV-driven immortalization of B lymphocytes.The EBNA2-responsive enhancer in the viral latency C promoter(Cp) binds two cellular factors, CBF1 and CBF2. The precise roleof the CBF2 protein for Cp enhancer function is presently unclear.CBF2 does not appear to interact with EBNA2 and binds just downstreamof CBF1 between positions $-$ 339 and $-$ 368 in the Cp EBNA2 enhancer.Within this region an 8-bp sequence, CAGTGCGT, can be found, anda similar sequence is also located downstream of CBF1 bindingsites in other EBNA2-responsive promoters. Previous studies haveindicated that mutations and methylation in this sequence affectEBNA2 responsiveness. To investigate the requirements for CBF2binding, we synthesized a series of oligonucleotides carryingdouble transversion mutations spanning both the conserved coresequence and outside flanking sequences. Surprisingly, mutationsoutside of the conserved core sequence in 4 bases immediatelyflanking the 5' end, GGTT, had the most deleterious effect onCBF2 binding. Mutations in the conserved core had a gradient effect,with those near the 5' end having the most deleterious effectson CBF2 binding. In addition, the affinities of CBF2 for bindingto the LMP-1, LMP-2, and CD23 promoters were also measured. Thesepromoters contain the conserved core but lack the 5' flankingGGTT motif and bound CBF2 weakly or not at all. Using Cp reporterplasmids containing CBF2 mutant binding sites, we were also ableto show that at lower doses of EBNA2, Cp transactivation requireda functional CBF2 binding site but that higher doses of EBNA2transactivated CBF2 mutant promoters to 40% of wild-type levels.These assays indicate that CBF2 is important for EBNA2-mediatedtransactivation of the viral latency Cp. In addition, CBF2 activitywas found to be associated with two polypeptides of 27 and 33kDa.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Epstein-Barr virus (EBV) has been consistently associated with a variety of B-cell malignancies, including endemic Burkitt'slymphomas, immunoblastic lymphomas of the immunosuppressed, anda proportion of Hodgkin's disease (33). EBV infection of primaryB cells results in the establishment of a latent infection, inwhich only 11 of potentially more than 80 viral proteins are expressed(17). These gene products include EBNAs 1, 2, 3A, 3B, 3C, and5 (leader protein); latent membrane proteins (LMP) 1, 2A, and2B; and the small noncoding EBERs 1 and 2. EBV infection of primaryB cells also leads to immortalization and outgrowth of continuouslyproliferating lymphoblastoid cell lines (LCL). Following EBV infection,the latency W promoter (Wp) is active initially and the firstviral genes expressed are EBNA-LP and EBNA2 (1, 2, 39,52). After EBNA2 expression, transcription initiation switchesfrom the Wp to the upstream latency C promoter (Cp), which inturn leads to expression of the other members of the EBNA family:EBNA1, -3A, -3B, and -3C (1, 2, 31, 39, 52, 53).Cp activation is dependent on a functional EBNA2 protein (41,52). In addition to activating expression of the Cp, EBNA2 activatesexpression of the viral LMP-1 and LMP-2 promoters, as well asthe cellular CD23 and the c-fgr proto-oncogene promoters (11,18, 27, 49, 51, 57).

EBNA2 is a transcriptional activator that does not directly bind DNA and interacts with target promoters through contact withthe ubiquitous cellular Cp binding factor 1 (CBF1), also calledRBPJ $kappa$ (13, 14, 23, 55). CBF1 binding sites have been observedin all of the EBNA2-responsive enhancers (13, 14, 22, 23,27, 55). Except for the viral LMP-1 promoter, all known EBNA2-responsivepromoters require interaction between EBNA2 and CBF1 for activationin transient-transfection assays (14, 16, 22, 23, 56).EBNA2 possesses an acidic activation domain located at the carboxyterminus of the protein (7, 24) and functions at least inpart through interactions with the basal transcription factorsTFIIB, TAF40, TFIIH, and a novel protein, p100 (45-47). Recombinantviruses expressing a gene encoding a mutant EBNA2 protein unableto interact with CBF1 or containing a deletion of the transactivationdomain fail to immortalize B cells, thus linking EBNA2 transactivationand immortalization functions (6, 54).

Regulation of Cp activity may be important for governing latency gene expression patterns established in the infected cell(26, 43). This idea is supported by the fact that in infectiousmononucleosis, during primary infection, and in most EBV-positivecell lines (lymphoblastoid cell lines), Cp is active (44). Underthese conditions EBV infection of B cells is characterized bylatency group III gene expression. Latency group III is normallycharacterized by the activity of the Cp and expression of thecomplete set of viral latent proteins, including those of theEBNA family. In contrast, tumor cells associated with Burkitt'slymphoma, nasopharyngeal carcinoma, and Hodgkin's disease usuallycontain an inactive Cp. Cell lines or tissues from these EBV-associatedmalignancies display group I or II patterns of latent gene expression.Latency group I is characterized by expression of only EBNA1,with transcripts initiated primarily from the Q promoter, whilelatency group II is characterized by expression of EBNA1, LMP-1,and LMP-2, with transcripts initiating from the Q promoter andLMP promoters. Recently, a number of studies have demonstratedthat the majority of EBV-infected cells in the peripheral bloodof healthy, persistently infected individuals are resting in G₀(CD23 B7) and express LMP-2A mRNA, but not other latency mRNAs, includingthose derived from Cp (9, 29, 30). Repression of Cp activitymay be important to reduce EBNA expression and avoid immune surveillancemechanisms of the host. In contrast, the ability to reactivateto latency group III, inducing lymphocyte proliferation, for example,may also be important for transient expansion of the pool of infectedlymphocytes as an important mechanism for EBV persistence. Consistentwith this notion, several mechanisms that both positively andnegatively regulate Cp activity have been described. In additionto EBNA2, glucocorticoids positively modulate Cp activity throughglucocorticoid response elements located upstream of the EBNA2-responsiveenhancer (19). In contrast, sequence-specific methylation maycontribute to silencing of Cp activity (28, 37). EBNA3 alsodownregulates EBNA2-mediated transactivation of the Cp (and alsothe LMP-1 and LMP-2 promoters) through competition for CBF1 (25,34, 50).

The EBNA2-responsive enhancer sequences from the LMP-1 and LMP-2 promoters have also been characterized. These enhancer sequencesbind many cellular factors in addition to CBF1 (16, 40, 55).Deletion and point mutation analysis of the LMP-1 promoter havesuggested that other cellular factors in addition to CBF1 maymediate or enhance EBNA2 transactivation. One of these factors,PU.1, has been proposed to mediate EBNA2 interaction with theLMP-1 promoter (16, 21, 40, 55). A proposed role for aPOU domain protein required for EBNA2-mediated transactivationhas also been suggested (40).

The Cp EBNA2 enhancer is structurally simple, interacting with only two cellular activities (23). A 100-bp sequence from $-$ 330 to $-$ 430 bases from the Cp transcription initiation site hasbeen mapped as the EBNA2-responsive element (15). The two cellularactivities associated with this fragment have been called CBF1and CBF2 (23). Whereas CBF1 has been extensively investigated,the identity of CBF2 and its role in EBNA2-mediated transactivationhave not been determined. Several lines of evidence suggest animportant role for CBF2 in EBNA2 transactivation. First, clusteredmutations between $-$ 340 to $-$ 360 in the Cp, where CBF2 binds, greatlyreduces EBNA2 transactivation (15). Second, synthetic promoterscontaining both CBF1 and CBF2 binding sites respond to EBNA2 transactivationsignificantly more strongly than promoters containing CBF1 bindingsites alone (23). Third, examination of the EBNA2 enhancer regionsin the Cp and the LMP-1 and -2 promoters reveals that sequencescontributing to EBNA2 transactivation have a common 5-bp sequence,CAGTG, or a similar expanded 8-bp sequence, CAGTG(C/T)G(T/G/C).Finally, some studies have suggested that the inactivity of theCp in some EBV cell lines correlates with CpG methylation of theCBF2 binding site and that cell lines in which Cp was active lackedCpG methylation of this site (23, 35, 37, 38). DNase protectionassays also showed that CBF2 binding is sensitive to methylationand that the methylated residue maps to position 6 in the 8-bpconserved sequence CAGTGCGT (37). In addition, a synthetic reporterplasmid containing a C-to-T change in this residue results ina 50-fold reduction in the ability of this enhancer to respondto EBNA2 transactivation (37).

In this study, we further define the sequence required for CBF2 binding and we evaluate the contribution of CBF2 towards EBNA2-mediatedtransactivation. These experiments provide further support foran important role for CBF2 in EBNA2-mediated transactivation.The data also indicates that the most important sequences thatdetermine CBF2 binding lie outside of a conserved 8-bp sequencefound in several EBNA2-responsive enhancers. Dissecting CBF2 participationin this process will further enhance our understanding of themechanism by which EBNA2 controls latent gene expression and B-cellimmortalization.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Cell culture. DG75 and CA46, EBV-negative Burkitt's lymphoma cell lines, were maintained in RPMI 1640 supplemented with 10% fetal bovineserum and incubated in 5% CO₂ at 37°C.

Plasmids. Reporter plasmids containing EBV sequences from nucleotides 10312 to 11336, which correspond to nucleotides $-$ 1021 to +3 relativeto the start site of the BamHI Cp, were constructed (Fig. 1).A reporter vector, pPDL3, was constructed by subcloning a SalIfragment containing the chloramphenicol acetyltransferase (CAT)reporter gene (also contains a polyadenylation element) from thepCATB' plasmid into the SalI site of pUC18. Plasmid pPDL5 carriesthe wild-type Cp sequence $-$ 1021 to +3 cloned as a KpnI/Sau3A fragmentinto the KpnI and BamHI sites in plasmid pPDL3. Mutations in theCp (see Fig. 3B) were generated by site-directed mutagenesis asdescribed by Chen and Przybyla (4). Briefly, PCR was performedwith a 5' primer that carries the desired mutation and a 3' primerthat binds downstream of the mutagenic site. The Cp amplifiedfragment was agarose gel purified and used as a primer togetherwith another 5' primer (upstream from the first 5' primer) ina second PCR. This second product was agarose gel purified, digestedwith SacI and EagI, and cloned into the same sites in the wild-typeCp $-$ 1021-to-+3 fragment. Plasmid MA1 carries the wild-type Cp $-$ 1021-to-+3 fragment cloned as a KpnI/Sau3A fragment into theKpnI and BglII sites of the pGL2-Basic vector (Promega). The Sau3A/BglIIjunction results in retention of the BglII site. MA1 was usedas the template for construction of most of the mutant fragments,except for pEFP 56 (mutant 12), in which pEFP 46 (mutant 3) wasused as the template (see Fig. 1 and 3 for illustrations of constructions).Mutant promoters were digested with KpnI and BglII and insertedinto the same sites of plasmid pPDL3. The following primers, withchanges introduced into the wild-type sequence underlined, wereused: OPL67 (mutant 3 primer), 5'-GGGAAAAAATTTATGGGGCAGTGCGTCGAGTGC-3'(for construction of pEFP 46; Cp $-$ 1021-to-+3 mutant 3); OPL126(mutant 11 primer), 5'-AATTTATGGTTCAGTGTGTCGAGTGCTATC-3' (forconstruction of pEFP 52; Cp $-$ 1021-to-+3 mutant 11); OPL207 (mutant12 primer), 5'-GTAAACACGCCGTGGGAAAAAATTTATTTGGCAGTGCGTCGAGTG-3'(for construction of pEFP 56; Cp $-$ 1021-to-+3 mutant 12); and OPL213(CBF1 mutant primer), 5'-GGTGTAAACACGCCGTTTGAAAAAATTTATGGTTC-3'(for construction of pEFP 76; Cp $-$ 1021-to-+3 CBF1 mutant). Thedownstream 3' primer used in the first round of PCR was OPL108,5'-ACGTTGCTCCACCTCTAAGG-3', and the upstream 5' primer used inthe second round of PCR was OPL109, 5'-CCTTGCGAACAATTATTAGT-3'.

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FIG. 1. Structure of Cp reporter constructions. A schematic illustration of the EBV genomic region containing the Cp and upstream sequences is shown at the top. Indicated are the episomal origin of replication (ori P), glucocorticoid response element (GRE), EBNA2 response element (E2RE), and the KpnI and Sau3A restriction sites. The arrow indicates the site of transcription initiation. Below are shown the Cp sequences cloned into reporter vectors (Cp $-$ 1021 to +3) and a multimerized version of the EBNA2 response element corresponding to positions $-$ 330 to $-$ 430 also cloned into a reporter vector (8X Cp E2RE).

The mutagenized Cp fragments were sequenced with the OPL109 and OPL108 primers to confirm the presence of the mutation andto confirm that no other changes were introduced.

Construction of plasmids carrying eight copies of the Cp EBNA2 enhancer region have been described previously (24). PlasmidpPDL84A contains eight copies of the wild-type Cp EBNA2-responsiveelement, which directs the expression of the CAT reporter (Fig.1). DNA fragments containing mutants 3, 11, and 12 (plasmids pEFP32, pEFP 63, and pEFP 68) were generated by PCR with primers thatamplify the sequence from $-$ 330 to $-$ 430. The templates used werederived from the Cp $-$ 1021-to-+3 promoter constructions containingthe appropriate mutation. Mutant CBF1 (GTCCGAA [with changes fromthe wild-type sequence underlined]) was generated by PCR, as previouslydescribed (4). The PCR product was digested with BglII andBamHI and cloned into the same sites of plasmid pGH56. Plasmidconstructions with one copy of the Cp sequence $-$ 330 to $-$ 430 weresequenced with the forward universal primer. The Cp fragmentscontaining sequence from $-$ 330 to $-$ 430 were then oligomerized aspreviously described (24), digested with BglII and BamHI, andcloned into the BglII site of the CAT expression vector pGH262.pPDL151 expresses EBNA2 and has been previously described (23).

EMSA. Nuclear extracts were prepared from CA46 cells as previously described (23). Nuclear extracts from 30 liters of culturewere fractionated by application to a heparin-Sepharose columnand were eluted with a linear 0.1- to 1.0-M KCl gradient. Thedifferent fractions were tested for CBF2 activity by electrophoreticmobility shift assay (EMSA). For the EMSA, the protein-DNA complexeswere formed as previously described (23). Two different DNAsequences from the Cp were used as probes: (i) the Cp EBNA2 enhancer,extending from $-$ 330 to $-$ 430 bases from the transcription initiationsite, which was excised from pDL63 with BglII and BamHI, and (ii)the 30-bp oligonucleotide duplex corresponding to bases $-$ 339 to $-$ 368 of the Cp. The probe containing the sequence from $-$ 339 to $-$ 368 has been shown previously to bind CBF2 in gel mobility shiftassays (23). Both fragments were end labeled with the Klenowfragment of DNA polymerase. The reaction mixtures were resolvedunder nondenaturing conditions on 4.5% polyacrylamide gels.

For competition assays, we synthesized a series of 30-mer oligonucleotides (and their complementary pairs) containing doubletransversion mutations in their sequences from $-$ 339 to $-$ 368. Inaddition to Cp sequences, these oligonucleotides contain BglIIand BamHI overhangs that increase their overall length to 36 bp.These oligonucleotides carried mutations across the conserved8-bp sequence and in the flanking regions (see Fig. 3B). Unlabeledmutant oligonucleotides were annealed and added to the bindingreaction mixture at 2.5, 5.0, 25, and 125 molar excesses relativeto the molarity of the labeled wild-type oligonucleotide probe.After EMSA, the amount of bound CBF2 activity was quantified witha Betascope 603 blot analyzer.

UV cross-linking. An oligonucleotide containing the CBF2 binding site of the Cp ( $-$ 339 to $-$ 368) and a 17-bp 3' sequence homologous to the M13forward sequencing primer was synthesized and annealed with theM13 forward universal primer. The sequence of the CBF2/M13 primeris 5'-AATTTATGGTTCAGTGCGTCGAGTGCTATGACTGGCCGTCGTTTTAC-3'. Theoligonucleotide was converted to fully duplex form, radiolabeled,and purified as described previously (22). Binding reactionmixtures were prepared essentially as described above for EMSA,but 200,000 cpm of probe was used. After 30 min of incubation,samples were irradiated on a model TMW-20 transilluminator (UVP,Inc.) for 1 h. Digestion with 12 U of DNase I (Boehringer Mannheim)and 1 U of microccocal nuclease (Pharmacia) was then carried outfor 15 min in the presence of a solution containing 7 mM Tris-HCl(pH 7.5), 7 mM MgCl₂, and 7 mM CaCl₂. Reaction products were electrophoresedon sodium dodecyl sulfate-12% polyacrylamide gels and visualizedby autoradiography. Competition reactions were done with a 50-Mexcess of competitor.

Transfections and CAT assays. DNA transfections were carried out by a DEAE-dextran method (24). Cells were transfected with the amounts of target andeffector plasmids indicated in the figures. Transfections wereharvested after 3 days of incubation, cells were lysed with reporterlysis buffer (Promega), and CAT assays were carried out as previouslydescribed (24). Acetylated forms of chloramphenicol in the chromatographicplates were detected by autoradiography and quantitated by excisingthe spot and counting in a liquid scintillation counter. A reportervector constitutively expressing luciferase (GL3 control; Promega)was used as an internal control for transfections, and the valuesfrom CAT assays were normalized to the luciferase activity.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

The CBF2 recognition element requires sequences that are unique to the Cp. In gel mobility shift assays the Cp EBNA2 enhancer binds CBF1 and CBF2. By competition analysis the CBF2 binding element mapsto sequences between $-$ 368 and $-$ 339 from the Cp transcription initiationsite (Fig. 2A) (23). Comparison of these essential sequenceswith the EBNA2-responsive sequences of the viral LMP-1 and LMP-2Apromoters and the cellular CD23 promoter reveals that all of thesepromoters have a common pentanucleotide, CAGTG, or a similar 8-bpsequence, CAGTGCGT (Fig. 2B). In addition, clustered mutationsin this region of the Cp have been shown to decrease the responsivenessof this promoter to EBNA2-mediated transactivation (15). Therefore,this conserved 8-bp sequence represented a potential CBF2 recognitionelement. To map more precisely the sequences required for CBF2binding in the Cp EBNA2 enhancer, we synthesized a series of oligonucleotidescontaining sequences from $-$ 368 to $-$ 339. Double transversion mutationswere introduced into some of these oligonucleotides across theputative CBF2 binding site and in the 5' and 3' flanking regions(Fig. 3B). The affinity of each oligonucleotide for CBF2 was measuredby its ability to compete for CBF2 binding with the wild-typesequence as evaluated by gel mobility shift assay. The wild-typeoligonucleotide was radiolabeled, and its ability to bind CBF2was measured in the presence of increasing amounts of the unlabeledwild type or mutant oligonucleotides. An example of the competitorassays is shown in Fig. 3A. A summary of data accumulated withall the mutant oligonucleotide competitors is shown in Fig. 3B.From this analysis we expected to find that regions flanking theconserved 8-bp sequence would have a moderate effect on CBF2 bindingbut that the most important sequences would be present in theconserved 8-bp conserved sequence. However, this analysis showedthat although the conserved 8-bp sequence is important for binding,the changes that affected CBF2 binding the most lie in the 5'flanking region, in sequences that are unique to the Cp (Fig.2B). Paired mutations across the 4 bases flanking the 5' sideof the conserved core GGTT eliminated CBF2 binding (mutants 2and 3), while mutant 1, which contains mutations even furtherupstream, reduced CBF2 binding by fivefold relative to that ofthe wild-type sequence. Each of the paired mutations introducedinto the 3' flanking region does not affect CBF2 binding, andsome of the mutants in this region seem to be even better competitorsthan the wild type.

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FIG. 2. CBF1 and CBF2 bind distinct sequences in the Cp EBNA2 enhancer which are conserved in other EBNA2-responsive promoters. (A) Nuclear extracts from CA46 cells were incubated with a radiolabeled Cp sequence from positions $-$ 330 to $-$ 430 in the presence or absence of competitor oligonucleotides and analyzed by EMSA. Lanes: 1, probe only; 2, CA46 extract; 3, CA46 extract and cold 30-mer oligonucleotide competitor from positions $-$ 359 to $-$ 388 (CBF1 binding element); 4, CA46 extract and cold 30-mer oligonucleotide competitor from positions $-$ 339 to $-$ 368 (CBF2 binding element). (B) Comparison of the nucleotide sequences of EBNA2-responsive promoters and locations of their putative conserved CBF2 binding sequences. Shown also is the location of the CBF1 binding sites previously characterized in these promoters. The LMP-1 promoter (LMP-1p) contains in its natural context the consensus CBF1 binding site in the antisense orientation and is shown on top as the reverse complement strand to aid in the comparison of similarities. LMP-2Ap, LMP-2A promoter; CD23p, CD23 promoter.

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FIG. 3. Mutagenesis analysis of the conserved 8-bp sequence in the Cp and identification of residues crucial for CBF2 binding. Nuclear extracts were mixed with 0-, 2.5-, 5-, 25-, and 125-fold molar excesses of the different unlabeled mutant oligonucleotides. A fixed amount of ³²P-wild-type (wt) oligonucleotide was then added to the shift reaction mixture. The reaction mixtures were separated on 4.5% nondenaturing polyacrylamide gels, dried, and autoradiographed. Amounts of CBF2 complex were quantified with a Betascope 603 blot analyzer. (A) The EMSA gel shows binding of nuclear extract containing CBF2 to a 30-mer oligonucleotide probe from positions $-$ 339 to $-$ 368 alone or with increasing (triangle) amounts of cold competitor oligonucleotide of the same sequence (the wild type [wt]) or mutant 11 (mut. 11) or mutant 12 (mut. 12) oligonucleotide. The asterisk denotes a nonspecific band that does not compete with the CBF2-specific oligonucleotide probes and appears in lanes containing probe only. (B) Summary of competition results. The sequences shown represent the central 30 bp of the 36-mer oligonucleotide. The 8-nucleotide conserved sequence is shaded. The mutations consist of double transversion mutations, and they are shown in boldface type and underlined. The numbers in column a are concentrations of unlabeled mutant oligonucleotides required for 50% competition. The numbers in column b are percentages representing the ability of each oligonucleotide to compete for CBF2 relative to that of the wt element, which was set at 100%. Results are averages from three independent experiments.

Mutations inside the conserved 8-bp sequence do not completely abolish CBF2 binding, and the ability to compete for CBF2 isdiluted as the paired changes are located farther from the 5'flanking region. Mutant 4, the one with the greatest effect, liesin the 5' border of the conserved 8-bp sequence. This mutant has23-fold decreased affinity for CBF2. Mutations downstream of thissite decreased activity by seven- to threefold.

We also tested other mutations that have been previously reported to affect the activity of the enhancer. The 4ch mutant (CGGCCGGT)contains four changes in the central part of the core and hasa sixfold reduction in binding (data not shown), while mutant11 has a sevenfold reduction. The result with mutant 11 is inagreement with that with mutant 6, whose affinity was also reducedsevenfold. Jin and Speck (15) reported that the 4ch mutant reducedthe ability of the enhancer to respond to EBNA2 approximatelyeightfold in transient-transfection assays, but binding activitiesfor this mutant were not reported. These results contrast withthose of Robertson et al. (37), who reported that mutant 11abolishes CBF2 binding. The differences for those results arenot known, but CBF2 binding in the study by Robertson et al. wasobserved through direct binding to mutant DNA, a method whichmay not be as sensitive as our assays. Our results show that mutant11 has an intermediate affinity for CBF2 (Fig. 3B; see below).On the other hand, mutations that lie in the 5' flanking regionwere not able to compete with the wild-type oligonucleotide evenat a concentration of 125-fold molar excess.

To confirm the competition results, mutant oligonucleotides 2, 3, 8, 10, and 11 were tested for their ability to directlybind CBF2 in a gel shift mobility assay. As expected, mutants2 and 3 were unable to bind CBF2 while mutants 8 and 10 showedwild-type levels of binding. Mutant 11 retained some binding activity(data not shown). The full-length sequence of the EBNA2 enhancerwas also tested for its ability to bind CBF2 in the presence ofincreasing amounts of some of the unlabeled mutant oligonucleotides,and results similar to those obtained with the 30-mer oligonucleotideprobe were observed (data not shown).

CBF2 activity is associated only with the Cp and not with other EBNA2 enhancers. In addition to that of the Cp, EBNA2 upregulates the expression of other viral and cellular promoters in EBV-immortalizedB cells. The putative CBF2 binding sites present in the LMP-1and LMP-2A viral promoters and the distal and proximal sites ofthe cellular CD23 promoter are shown in Fig. 2B. Although thesepromoters contain the conserved 8-bp sequence, their 5' flankingregions are highly divergent from those of the Cp. We measuredthe ability of oligonucleotides containing the putative CBF2 recognitionelement from these other promoters for CBF2 binding by competitionassays (Fig. 4). The results of these competitions show that thesequences from the other promoters fail to detectably bind CBF2.LMP-1 was able to compete at a very low level (37-fold-reducedaffinity), while the other promoters could not compete even atthe highest concentration of competitor tested. These sequenceswere also tested for their ability to directly bind CBF2 in agel mobility shift assay, and CBF2 binding was undetectable (datanot shown). This result is consistent with the result of our previousmutagenesis of the Cp, which indicated that the 5' sequences flankingthe conserved 8-bp sequence are crucial for CBF2 binding.

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FIG. 4. The LMP-1, LMP-2A, and CD23 promoters fail to bind CBF2. Competitions were carried out as described for Fig. 3. The sequences shown represent the central 30 bp of the 36-mer oligonucleotide. The 8-bp putative CBF2 binding sites are shaded. The natural changes between the sequences of the LMP-1, LMP-2A, and CD23 promoters and Cp are shown in boldface type and underlined. The numbers in column a are concentrations of unlabeled mutant oligonucleotides required for 50% competition. The numbers in column b are percentages representing the ability of each oligonucleotide to compete for CBF2 relative to that of the wild-type element, which was set at 100%. Results are averages from three independent experiments.

Activation of the Cp by EBNA2 is strongly dependent on CBF2. To evaluate the importance of CBF2 for EBNA2-mediated transactivation of the Cp, we tested the ability of EBNA2 to transactivatewild-type and mutant Cp constructions in transient-transfectionassays. Two different sequences from the Cp were used for thisanalysis (Fig. 1): (i) the 100-bp EBNA2 enhancer from $-$ 330 to $-$ 430 and (ii) a larger fragment spanning $-$ 1021 to +3 from theCp. The 100-bp fragments containing $-$ 430 to $-$ 330 were multimerizedto eight copies and cloned upstream of the adenovirus E1b TATAbox in the reporter plasmid E1b CAT. The larger $-$ 1021-to-+3 fragmentcontains the natural TATA box and transcription initiation sitesfrom the Cp, and they were cloned upstream of the CAT reportergene.

The results of these transfections are shown in Fig. 5 and summarized in Table 1. For transfection of plasmids with eightcopies of the EBNA2 enhancer, 0.5 µg of EBNA2-expressing plasmidand 2 µg of each of the target plasmids were used. Fold inductionsafter addition of effector plasmid could not be calculated dueto the low basal activity of these constructions, which was nothigher than the background level given by the CAT expression vectoralone, and transfections were performed with single doses of effectorplasmid. Under these conditions, mutant 11 had no effect on responsivenessof the enhancer (Fig. 5A). Both mutant 3 and mutant 12, whoseaffinities for CBF2 are significantly weaker than that of thewild type, were transactivated by EBNA2 to 23 and 36% of wild-typelevels, respectively.

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FIG. 5. Analysis of the EBNA2 responsiveness of wild-type (wt) and CBF2 Cp mutants. (A) Results of single-dose transfections to compare levels of EBNA2 transactivation of reporter plasmids containing eight tandem copies of the EBNA2 enhancer. DG75 cells were cotransfected with 2 µg of the target plasmid and 0.5 µg of the effector EBNA2-expressing plasmid. Results are averages from two independent experiments. mut., mutant. (B) Dose responses for comparison of levels of EBNA2 transactivation of reporter plasmids containing the Cp $-$ 1021-to-+3 sequence. Cells were transfected with 2 µg of target plasmid and 0.2, 0.4, 0.8, and 1.6 µg of effector EBNA2-expressing plasmid. Results are averages from five independent experiments. Standard errors of the means are indicated with T bars.

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TABLE 1. Summary of levels of transactivation of the wild-type and mutant Cps

Figure 5B shows the results of transfections with the Cp $-$ 1021-to-+3 constructions. Table 1 shows the range of activitiesobtained with these plasmids in response to the different concentrationsof EBNA2. In general, the activities of the mutants correlatedwell with the CBF2 binding affinities. Mutant 11 had an intermediateeffect (up to 63% of the activity of the wild-type promoter),while mutant 3 was a slightly worse responder, with its maximalactivity being 45% of wild-type levels. Interestingly, mutant12 was not responsive at the lowest concentrations tested, butwith increasing amounts of EBNA2, it was activated to 36% of wild-typelevels. As expected, the CBF1 mutant was the one with the lowestactivity and was not activated to a significant degree at anyEBNA2 concentration tested. The results of these transfectionexperiments indicate that CBF2 binding contributes significantlyto EBNA2 transactivation.

Two polypeptides of 33 and 25 kDa are associated with the Cp CBF2 recognition element. In order to identify proteins that specifically associate with the CBF2 site of the Cp, bromo-dUTP-containing oligonucleotideprobes representing the sequences from $-$ 368 to $-$ 339 were incubatedwith the CA46 nuclear extracts under conditions similar to thoseemployed in the shift assays. The samples were irradiated withUV light to cross-link the DNA-protein complexes formed duringthe binding reaction and digested with nucleases to remove unboundDNA. Figure 6A shows two polypeptides of 33 and 25 kDa specificallyassociated with the Cp DNA probe containing sequence $-$ 368 to $-$ 339.Competition with a 75-fold molar excess of unlabeled mutant 3probe did not affect the binding of these peptides, while competitionwith only a 25-fold molar excess of the unlabeled wild-type probewas sufficient to abolish binding to the CBF2 response element.In an independent experiment, 50-fold molar excesses of mutants2, 3, and 10 were also tested (Fig. 6B). As expected, while mutant10 resembled the wild-type oligonucleotide probe in binding, mutant2 and 3 oligonucleotides did not compete for binding. This resultconfirms the importance of the 5' flanking sequences for CBF2binding. These results suggest that the 33- and 25-kDa polypeptidesare candidates for nuclear factors that may bind and mediate CBF2activity.

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FIG. 6. UV-cross-linking analysis demonstrating that the CBF2 binding site specifically interacts with two polypeptides of 33 and 25 kDa. (A) Competition with different amounts of unlabeled competitors. Reaction mixtures containing UV-cross-linked proteins were resolved on sodium dodecyl sulfate-12.5% polyacrylamide gels, dried, and autoradiographed. To some cross-linking reaction mixtures cold competitor oligonucleotides were added as indicated. Lanes 1 to 3, competition with 75-, 50-, and 25-fold molar excesses, respectively, of mutant 3 (mut.3); lanes 4 to 6, competition with 75-, 50-, and 25-fold molar excesses, respectively, of the wild-type (wt) sequence; lane 7, no competition. (B) Competition with 50-fold molar excesses of wild-type, mutant 10, mutant 2, and mutant 3 oligonucleotides. Asterisks indicate specific bands of 33 and 25 kDa interacting with the CBF2 probe. Lane 1 contains no competitor.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Understanding the mechanisms of EBNA2-regulated gene expression during viral latency is essential to understanding EBV-drivenB-cell immortalization. The viral latency Cp provides a simplemodel to study EBNA2-transactivating mechanisms. This enhancerbinds two cellular proteins, CBF1 and CBF2. CBF1 is responsiblefor tethering EBNA2 to promoter DNA, and as such, CBF1 bindingelements have been identified in all known EBNA2 enhancer elements.

In contrast, CBF2 has not been well-characterized. Sequence comparisons reveal similar 8-bp sequences, CAGT(C/T)G(T/G/C),in all known EBNA2-responsive promoters. The 8-bp conserved sequencein the Cp is protected in DNase I footprinting analysis with nuclearextracts from B lymphocytes (15, 23, 37). In addition, somemutations in the 8-bp conserved sequence affect transactivationby EBNA2 (15). Based on these observations we hypothesized (i)that several of the known EBNA2-responsive promoters bind CBF2,(ii) that the 8-bp conserved sequence is responsible for thisbinding, and (iii) that CBF2 plays a general role in EBNA2-transactivatingfunction. Surprisingly, although we found that the conserved 8-bpcore influenced binding, mutations adjacent to and upstream ofthis conserved region produced more-dramatic effects on CBF2 binding.

These results were obtained in both EMSA and UV-cross-linking analyses. These analyses identified the sequence GGTTCA as thebasic core element required for CBF2 binding. Transversion changesin these sequences eliminated CBF2 binding. The sequences thatflank GGTTCA were also found to decrease binding affinity up tosevenfold (e.g., mutations in the 5' AT and those in the 3' GTGC).Our data is also consistent with the results of the footprintinganalysis by Jin and Speck (15), where the GGTTCA sequence wasprotected in the absence of CBF1 binding. Database searches withthe basic hexanucleotide GGTTCA, the extended sequence ATGGTTCAGTGC,or the conserved core sequence have not been informative in determiningwhether other DNA binding proteins identified so far will recognizethis sequence. The UV-cross-linking results also identified thatCBF2 activity is associated with two polypeptides of 25 and 33kDa. It is unclear whether CBF2 is a heterodimer of two proteinsor if the smaller 25-kDa protein is a degradation product or somespliced variant of the larger 33-kDa protein. Alternatively, thetwo proteins may be differentially modified species of the sameprotein.

The putative binding sites present in other EBNA2 enhancers were not able to bind CBF2. Although these promoters contain theconserved 8-bp sequence, their 5' flanking regions diverge fromthose of the Cp sequences. Because the conserved core is not sufficientto confer CBF2 binding activity and these enhancers do not containcrucial sequences required for CBF2 binding, we predict that CBF2does not play a significant role in the EBNA2-mediated transcriptionalactivation of these promoters. Consistent with this hypothesis,Meitinger et al. introduced clustered mutations into the LMP-2Apromoter, some of which overlap the conserved 8-bp core (27).These mutations had only small effects on EBNA2 transactivationof the LMP-2A promoter.

The level of EBNA2 transactivation of the Cp $-$ 1021-to-+3 reporter correlated with the relative affinity of the CBF2 bindingsite for CBF2. Mutant 11 reduced competitor efficiency to 86%of wild-type levels. Cp $-$ 1021-to-+3 promoter constructions containingthis mutation were activated by EBNA2 to 40 to 60% of wild-typelevels (Table 1). Mutants 3 and 12 reduced competitor efficiencyby greater than 98%. Cp $-$ 1021-to-+3 promoter constructions containingthese mutations were activated to 37 to 47% and 0 to 36%, respectively(Table 1). Interestingly, the requirement for a functional CBF2element was most apparent at low concentrations of EBNA2 in thetransient-transfection assays.

Optimal transactivation of the multimerized enhancer constructions also required a functional CBF2 binding site. Both mutants3 and 12 were transactivated to 23 and 36% of wild-type levels,respectively. Mutant 11 activity, however, resembled that of thewild-type enhancer construction. This mutation only partiallyreduced the affinity for CBF2. The deleterious effect predictedfor this mutant may be masked due to the presence of several copiesof the enhancer and the number of EBNA2 molecules that can bindthis artificial promoter, which results in high levels of activity.Our results differ from those of a previous publication that demonstratevirtual loss of activity from an identical construction (37).Recent studies, however, now confirm that a multimerized versionof an EBNA2 response element containing mutant 11 and cloned intoa reporter vector may have only small effects on EBNA2-mediatedtransactivation (3). Methylation of the natural cytosine inthis position has been suggested to regulate Cp expression indifferent types of EBV-driven lymphomas (35, 36). In the morenatural context of the Cp $-$ 1021-to-+3 construction, mutant 11causes a reduction in EBNA2 transactivation of 47 to 60%. Methylationat this site together with methylation at other positions or thepresence of additional inhibitory factors may be working togetherto inactivate Cp in the lymphoma-derived cell lines. Also, EBNA2is expressed from the Cp and mechanisms that reduce Cp activitywill reduce the concentration of EBNA2. Under these conditions,the Cp may be more sensitive to the presence of CBF2.

The regulatory mechanism of CBF2 action is at present unclear. Previous studies have been unable to demonstrate an interactionwith EBNA2 (23). Multimerized CBF2 binding sites also had noeffect on transcriptional activity of a basal promoter (23).Stabilizing interactions between CBF1 and CBF2 also remain a possibility.However, due to the low concentrations of CBF2 derived from nuclearextracts, it has thus far not been possible to obtain sufficientquantities of pure CBF2 to test this hypothesis (unpublished observations).Recent work has revealed a distinct class of proteins termed architecturaltranscription factors (20). Examples of such factors are thehigh-mobility-group proteins that include LEF-1 (48). Like CBF2,multimerized LEF-1 binding sites were unable to activate transcriptionof a basal promoter element. In the context of the T-cell receptor $alpha$ enhancer, LEF-1 DNA bending appears to facilitate interactionof other promoter-bound factors and to further activate enhanceractivity (48). Whether CBF2 is an architectural factor or targetsan interaction of other important transcription factors awaitsthe identification of the gene product.

The presence of the 8-bp sequence conserved among the EBNA2 enhancers may be explained by several reasons. First, this coremay represent the remains of a lost regulatory element. It ispossible that CBF2 was required for the activation of these enhancers(e.g., LMP-1, LMP-2A, and CD23) but that binding to CBF2 was notnecessary as the enhancers gained the ability to bind other cellularfactors that could substitute for CBF2. As evidence for this,the LMP-2A promoter region of the closely related herpesviruspapio does not contain the conserved core (12). Alternatively,there may be cellular or viral activities, different from thatof CBF2, that associate with the conserved 8-bp sequence. Thisactivity may be present only under a given condition or stageof viral infection that has heretofore been undetected.

The role of the EBNA2-responsive enhancer for Cp expression has recently been challenged. Viral recombinants containing mutationsin the Cp CBF1 binding site were viable, and some clones retainedalmost wild-type Cp activity (10). One possibility for thisresult is that the activity of the EBNA2-responsive enhancer wasnot sufficiently reduced by mutation of the CBF1 binding sitealone and may require additional mutations, for example, in theCBF2 element. In vitro, viral recombinants containing large deletionsin Cp are also immortalizing competent and use Wp (42). WhileCp usage may not be required for immortalization in vitro, transcriptsinitiating from Cp in EBV-infected lymphocytes in vivo are detectedin individuals with both primary and persistent infection (5,32, 44). Several studies are also consistent with CBF2 havinga significant role in Cp activation. Contreras-Brodin et al. (8)showed that Cp activity is restricted to B cells. Unlike CBF1,which is constitutively expressed in almost all cell types, CBF2appears to be expressed only in lymphocytes (15, 52). It isintriguing to speculate that CBF2 may be an important factor requiredfor Cp activity in lymphoid cells. In addition, site-specificmethylation that prevents CBF2 binding but not CBF1 binding alsocorrelates with Cp silencing in a Burkitt's lymphoma cell line(28, 37). Treatment with 5-azacytidine results in demethylation,CBF2 binding, and activation of Cp. Future studies involving theintroduction of mutations in the CBF2 binding element in the contextof the viral genome will be informative in confirming the roleof CBF2 for Cp activity.

Overall, mutagenesis of the CBF2 response element permitted us to determine that the sequence GGTTCA is essential for CBF2binding, with the immediately flanking sequences influencing theaffinity for this element. Furthermore, the transient-transfectionanalysis provided evidence for the importance of CBF2 functionin the Cp EBNA2 enhancer. Further characterization and identificationof the CBF2 gene will contribute to a better understanding ofthe mechanisms controlling Cp activity during latent infections.

	ACKNOWLEDGMENTS

We thank R. T. Javier and A. P. Rice for their critical reading of the manuscript.

This work was supported by NIH grant R29 CA69437 to P.D.L. and a Leukemia Society Special Fellowship to P.D.L.

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Molecular Virology, Baylor College of Medicine, One Baylor Plaza, Houston,TX 77030. Phone: (713) 798-8474. Fax: (713) 798-3586. E-mail:pling{at}bcm.tmc.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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	Articles by Ling, P. D.

1.	Alfieri, C., M. Birkenbach, and E. Kieff. 1991. Early events in Epstein-Barr virus infection of human B lymphocytes. Virology 181:595-608[Medline].
2.	Allday, M. J., D. H. Crawford, and B. E. Griffin. 1989. Epstein-Barr virus latent gene expression during the initiation of B cell immortalization. J. Gen. Virol. 70:1755-1764[Abstract/Free Full Text].
3.	Ambinder, R. F. Personal communication.
4.	Chen, B., and A. E. Przybyla. 1994. An efficient site-directed mutagenesis method based on PCR. BioTechniques 17:657-659. [Medline]
5.	Chen, F., J. Z. Zou, L. di Renzo, G. Winberg, L. F. Hu, E. Klein, G. Klein, and I. Ernberg. 1995. A subpopulation of normal B cells latently infected with Epstein-Barr virus resembles Burkitt lymphoma cells in expressing EBNA-1 but not EBNA-2 or LMP1. J. Virol. 69:3752-3758[Abstract].
6.	Cohen, J. I. 1992. A region of herpes simplex virus VP16 can substitute for a transforming domain of Epstein-Barr virus nuclear protein 2. Proc. Natl. Acad. Sci. USA 89:8030-8034[Abstract/Free Full Text].
7.	Cohen, J. I., and E. Kieff. 1991. An Epstein-Barr virus nuclear protein 2 domain essential for transformation is a direct transcriptional activator. J. Virol. 65:5880-5885[Abstract/Free Full Text].
8.	Contreras-Brodin, B., A. Karlsson, T. Nilsson, L. Rymo, and G. Klein. 1996. B cell-specific activation of the Epstein-Barr virus-encoded C promoter compared with the wide-range activation of the W promoter. J. Gen. Virol. 77:1159-1162[Abstract/Free Full Text].
9.	Decker, L. L., L. D. Klaman, and D. A. Thorley-Lawson. 1996. Detection of the latent form of Epstein-Barr virus DNA in the peripheral blood of healthy individuals. J. Virol. 70:3286-3289[Abstract].
10.	Evans, T. J., P. J. Farrell, and S. Swaminathan. 1996. Molecular genetic analysis of Epstein-Barr virus Cp promoter function. J. Virol. 70:1695-1705[Abstract].
11.	Fahraeus, R., A. Jansson, A. Ricksten, A. Sjoblom, and L. Rymo. 1990. Epstein-Barr virus-encoded nuclear antigen 2 activates the viral latent membrane protein promoter by modulating the activity of a negative regulatory element. Proc. Natl. Acad. Sci. USA 87:7390-7394[Abstract/Free Full Text].
12.	Franken, M., B. Annis, A. N. Ali, and F. Wang. 1995. 5' coding and regulatory region sequence divergence with conserved function of the Epstein-Barr virus LMP2A homolog in herpesvirus papio. J. Virol. 69:8011-8019[Abstract].
13.	Grossman, S. R., E. Johannsen, X. Tong, R. Yalamanchili, and E. Kieff. 1994. The Epstein-Barr virus nuclear antigen 2 transactivator is directed to response elements by the J kappa recombination signal binding protein. Proc. Natl. Acad. Sci. USA 91:7568-7572[Abstract/Free Full Text].
14.	Henkel, T., P. D. Ling, S. D. Hayward, and M. G. Peterson. 1994. Mediation of Epstein-Barr virus EBNA2 transactivation by recombination signal-binding protein J kappa. Science 265:92-95[Abstract/Free Full Text].
15.	Jin, X. W., and S. H. Speck. 1992. Identification of critical cis elements involved in mediating Epstein-Barr virus nuclear antigen 2-dependent activity of an enhancer located upstream of the viral BamHI C promoter. J. Virol. 66:2846-2852[Abstract/Free Full Text].
16.	Johannsen, E., E. Koh, G. Mosislos, X. Tong, E. Kieff, and S. R. Grossman. 1995. Epstein-Barr virus nuclear protein 2 transactivation of the latent membrane protein 1 promoter is mediated by J $kappa$ and PU.1. J. Virol. 69:253-262[Abstract].
17.	Kieff, E. 1996. Epstein-Barr virus and its replication, p. 107-172. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Virology, 3rd ed. Lippincott-Raven Publishers, Philadelphia, Pa.
18.	Knutson, J. C. 1990. The level of c-fgr RNA is increased by EBNA-2, an Epstein-Barr virus gene required for B-cell immortalization. J. Virol. 64:2530-2536[Abstract/Free Full Text].
19.	Kupfer, S. R., and W. C. Summers. 1990. Identification of a glucocorticoid-responsive element in Epstein-Barr virus. J. Virol. 64:1984-1990[Abstract/Free Full Text].
20.	Landy, A. 1989. Dynamic, structural, and regulatory aspects of lambda site-specific recombination. Annu. Rev. Biochem. 58:913-949[Medline].
21.	Laux, G., F. Dugrillon, C. Eckert, B. Adam, S. U. Zimber, and G. W. Bornkamm. 1994. Identification and characterization of an Epstein-Barr virus nuclear antigen 2-responsive cis element in the bidirectional promoter region of latent membrane protein and terminal protein 2 genes. J. Virol. 68:6947-6958[Abstract/Free Full Text].
22.	Ling, P. D., J. J. Hsieh, I. K. Ruf, D. R. Rawlins, and S. D. Hayward. 1994. EBNA-2 upregulation of Epstein-Barr virus latency promoters and the cellular CD23 promoter utilizes a common targeting intermediate, CBF1. J. Virol. 68:5375-5383[Abstract/Free Full Text].
23.	Ling, P. D., D. R. Rawlins, and S. D. Hayward. 1993. The Epstein-Barr virus immortalizing protein EBNA-2 is targeted to DNA by a cellular enhancer-binding protein. Proc. Natl. Acad. Sci. USA 90:9237-9241[Abstract/Free Full Text].
24.	Ling, P. D., J. J. Ryon, and S. D. Hayward. 1993. EBNA-2 of herpesvirus papio diverges significantly from the type A and type B EBNA-2 proteins of Epstein-Barr virus but retains an efficient transactivation domain with a conserved hydrophobic motif. J. Virol. 67:2990-3003[Abstract/Free Full Text].
25.	Marshall, D., and C. Sample. 1995. Epstein-Barr virus nuclear antigen 3C is a transcriptional regulator. J. Virol. 69:3624-3630[Abstract].
26.	Masucci, M. G., and I. Ernberg. 1994. Epstein-Barr virus: adaptation to a life within the immune system. Trends Microbiol. 2:125-130[Medline].
27.	Meitinger, C., L. J. Strobl, G. Marschall, G. W. Bornkamm, and U. Zimber-Strobl. 1994. Crucial sequences within the Epstein-Barr virus TP1 promoter for EBNA2-mediated transactivation and interaction of EBNA2 with its responsive element. J. Virol. 68:7497-7506[Abstract/Free Full Text].
28.	Minarovits, J., L. F. Hu, K. S. Minarovits, G. Klein, and I. Ernberg. 1994. Sequence-specific methylation inhibits the activity of the Epstein-Barr virus LMP1 and BCR2 enhancer-promoter regions. Virology 200:661-667[Medline].
29.	Miyashita, E. M., B. Yang, G. J. Babcock, and D. A. Thorley-Lawson. 1997. Identification of the site of Epstein-Barr virus persistence in vivo as a resting B cell. J. Virol. 71:4882-4891[Abstract].
30.	Miyashita, E. M., B. Yang, K. M. Lam, D. H. Crawford, and D. A. Thorley-Lawson. 1995. A novel form of Epstein-Barr virus latency in normal B cells in vivo. Cell 80:593-601[Medline].
31.	Puglielli, M. T., N. Desai, and S. H. Speck. 1997. Regulation of EBNA gene transcription in lymphoblastoid cell lines: characterization of sequences downstream of BCR2 (Cp). J. Virol. 71:120-128[Abstract].
32.	Qu, L., and D. T. Rowe. 1992. Epstein-Barr virus latent gene expression in uncultured peripheral blood lymphocytes. J. Virol. 66:3715-3724[Abstract/Free Full Text].
33.	Rickinson, A. B., and E. Kieff. 1996. Epstein-Barr virus, p. 2397-2446. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Virology, 3rd ed. Lippincott-Raven Publishers, Philadelphia, Pa.
34.	Robertson, E. S., S. Grossman, E. Johannsen, C. Miller, J. Lin, B. Tomkinson, and E. Kieff. 1995. Epstein-Barr virus nuclear protein 3C modulates transcription through interaction with the sequence-specific DNA-binding protein J $kappa$ . J. Virol. 69:3108-3116[Abstract].
35.	Robertson, K. D., and R. F. Ambinder. 1996. Regulation of the Epstein-Barr virus BamHI-C promoter by DNA methylation. Epstein-Barr Virus Rep. 3:115-121.
36.	Robertson, K. D., and R. F. Ambinder. 1997. Mapping promoter regions that are hypersensitive to methylation-mediated inhibition of transcription: application of the methylation cassette assay to the Epstein-Barr virus major latency promoter. J. Virol. 71:6445-6454[Abstract].
37.	Robertson, K. D., S. D. Hayward, P. D. Ling, D. Samid, and R. F. Ambinder. 1995. Transcriptional activation of the Epstein-Barr virus latency C promoter after 5-azacytidine treatment: evidence that demethylation at a single CpG site is crucial. Mol. Cell. Biol. 15:6150-6159[Abstract].
38.	Robertson, K. D., L. J. Swinnen, J. C. Zong, M. L. Gulley, and R. F. Ambinder. 1996. CpG methylation of the major Epstein-Barr virus latency promoter in Burkitt's lymphoma and Hodgkin's disease. Blood 88:3129-3136[Abstract/Free Full Text].
39.	Rooney, C., J. G. Howe, S. H. Speck, and G. Miller. 1989. Influence of Burkitt's lymphoma and primary B cells on latent gene expression by the nonimmortalizing P3J-HR-1 strain of Epstein-Barr virus. J. Virol. 63:1531-1539[Abstract/Free Full Text].
40.	Sjoblom, A., A. Jansson, S. Yang, S. Lain, T. Nilsson, and L. Rymo. 1995. PU box-binding transcription factors and a POU domain protein cooperate in the Epstein-Barr virus (EBV) nuclear antigen 2-induced transactivation of the EBV latent membrane protein 1 promoter. J. Gen. Virol. 76:2679-2692[Abstract/Free Full Text].
41.	Sung, N. S., S. Kenney, D. Gutsch, and J. S. Pagano. 1991. EBNA-2 transactivates a lymphoid-specific enhancer in the BamHI C promoter of Epstein-Barr virus. J. Virol. 65:2164-2169[Abstract/Free Full Text].
42.	Swaminathan, S. 1996. Characterization of Epstein-Barr virus recombinants with deletions of the BamHI C promoter. Virology 217:532-541[Medline].
43.	Thorley-Lawson, D. A., E. M. Miyashita, and G. Khan. 1996. Epstein-Barr virus and the B cell: that's all it takes. Trends Microbiol. 4:204-208[Medline].
44.	Tierney, R. J., N. Steven, L. S. Young, and A. B. Rickinson. 1994. Epstein-Barr virus latency in blood mononuclear cells: analysis of viral gene transcription during primary infection and in the carrier state. J. Virol. 68:7374-7385[Abstract/Free Full Text].
45.	Tong, X., R. Drapkin, D. Reinberg, and E. Kieff. 1995. The 62- and 80-kDa subunits of transcription factor IIH mediate the interaction with Epstein-Barr virus nuclear protein 2. Proc. Natl. Acad. Sci. USA 92:3259-3263[Abstract/Free Full Text].
46.	Tong, X., R. Drapkin, R. Yalamanchili, G. Mosialos, and E. Kieff. 1995. The Epstein-Barr virus nuclear protein 2 acidic domain forms a complex with a novel cellular coactivator that can interact with TFIIE. Mol. Cell. Biol. 15:4735-4744[Abstract].
47.	Tong, X., F. Wang, C. J. Thut, and E. Kieff. 1995. The Epstein-Barr virus nuclear protein 2 acidic domain can interact with TFIIB, TAF40, and RPA70 but not with TATA-binding protein. J. Virol. 69:585-588[Abstract].
48.	Travis, A., A. Amsterdam, C. Belanger, and R. Grosschedl. 1991. LEF-1, a gene encoding a lymphoid-specific protein with an HMG domain, regulates T-cell receptor alpha enhancer function. Genes Dev. 5:880-894[Abstract/Free Full Text].
49.	Tsang, S. F., F. Wang, K. M. Izumi, and E. Kieff. 1991. Delineation of the cis-acting element mediating EBNA-2 transactivation of latent infection membrane protein expression. J. Virol. 65:6765-6771[Abstract/Free Full Text].
50.	Waltzer, L., M. Perricaudet, A. Sergeant, and E. Manet. 1996. Epstein-Barr virus EBNA3A and EBNA3C proteins both repress RBP-J $kappa$ -EBNA2-activated transcription by inhibiting the binding of RBP-J $kappa$ to DNA. J. Virol. 70:5909-5915[Abstract].
51.	Wang, F., H. Kikutani, S. F. Tsang, T. Kishimoto, and E. Kieff. 1991. Epstein-Barr virus nuclear protein 2 transactivates a cis-acting CD23 DNA element. J. Virol. 65:4101-4106[Abstract/Free Full Text].
52.	Woisetschlaeger, M., X. W. Jin, C. N. Yandava, L. A. Furmanski, J. L. Strominger, and S. H. Speck. 1991. Role for the Epstein-Barr virus nuclear antigen 2 in viral promoter switching during initial stages of infection. Proc. Natl. Acad. Sci. USA 88:3942-3946[Abstract/Free Full Text].
53.	Woisetschlaeger, M., C. N. Yandava, L. A. Furmanski, J. L. Strominger, and S. H. Speck. 1990. Promoter switching in Epstein-Barr virus during the initial stages of infection of B lymphocytes. Proc. Natl. Acad. Sci. USA 87:1725-1729[Abstract/Free Full Text].
54.	Yalamanchili, R., X. Tong, S. Grossman, E. Johannsen, G. Mosialos, and E. Kieff. 1994. Genetic and biochemical evidence that EBNA 2 interaction with a 63-kDa cellular GTG-binding protein is essential for B lymphocyte growth transformation by EBV. Virology 204:634-641[Medline].
55.	Zimber-Strobl, U., E. Kremmer, F. Grasser, G. Marschall, G. Laux, and G. W. Bornkamm. 1993. The Epstein-Barr virus nuclear antigen 2 interacts with an EBNA2 responsive cis-element of the terminal protein 1 gene promoter. EMBO J. 12:167-175[Medline].
56.	Zimber-Strobl, U., L. J. Strobl, C. Meitinger, R. Hinrichs, T. Sakai, T. Furukawa, T. Honjo, and G. W. Bornkamm. 1994. Epstein-Barr virus nuclear antigen 2 exerts its transactivating function through interaction with recombination signal binding protein RBP-J kappa, the homologue of Drosophila Suppressor of Hairless. EMBO J. 13:4973-4982[Medline].
57.	Zimber-Strobl, U., K. O. Suentzenich, G. Laux, D. Eick, M. Cordier, A. Calender, M. Billaud, G. M. Lenoir, and G. W. Bornkamm. 1991. Epstein-Barr virus nuclear antigen 2 activates transcription of the terminal protein gene. J. Virol. 65:415-423[Abstract/Free Full Text].