Cells Expressing the Epstein-Barr Virus Growth Program Are Present in and Restricted to the Naive B-Cell Subset of Healthy Tonsils

doi:10.1128/JVI.74.21.9964-9971.2000

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Journal of Virology, November 2000, p. 9964-9971, Vol. 74, No. 21
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Cells Expressing the Epstein-Barr Virus Growth Program Are Present in and Restricted to the Naive B-Cell Subset of Healthy Tonsils

Alexandra M. Joseph, Gregory J. Babcock, and David A. Thorley-Lawson^*

Department of Pathology, Tufts University School of Medicine, Boston, Massachusetts 02111

Received 5 May 2000/Accepted 8 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

In this paper we demonstrate, for the first time, that Epstein-Barr virus (EBV)-infected cells expressing the lymphoblastoidgrowth program are present in healthy carriers of the virus. Previouslywe observed that latently infected naive B cells are present intonsils only when viral replication is detected, suggesting thatthese may represent newly infected B cells. We have tested thisidea by performing a reverse transcription-PCR analysis for theexpression of latent genes (EBNA2 and the EBNA3s) that are characteristicallyexpressed only by newly infected cells expressing the growth latencyprogram. EBNA2 expression is regularly detected in purified naive(IgD⁺) tonsillar B cells (13 of 16 tonsils tested) but was never foundin the IgD population (0 of 16). More detailed analysis revealed that themRNAs for the latent genes EBNA1 (3 of 3 tonsils tested), EBNA3a(3 of 5), EBNA3b (3 of 5), EBNA3c (3 of 5), LMP1 (6 of 6), andLMP2 (5 of 6) were also present in the IgD⁺ population, but the EBNA1Q-K transcript, characteristic of nonlymphoblastoidforms of latency, was never detected (0 of 6). Finally, we demonstratethat the latently infected naive (IgD⁺) cells express CD80 (B7.1), a marker characteristically expressedon activated naive lymphoblasts but absent from resting naiveB cells. The infected naive (IgD⁺) population in the tonsil therefore has the viral and cellularphenotype of a B-cell directly infected with EBV $---$ an activatedlymphoblast expressing the growthprogram.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Epstein-Barr virus (EBV) is a human, B-lymphotropic herpesvirus that is best known for its capacity to immortalize normalB cells in vitro and for its association with a number of humanneoplasias, including both lymphomas and carcinomas (for reviewssee references 14 and 27). EBV immortalizes B cells in vitroby infecting them and driving them to become proliferating lymphoblasts(34) through the expression of nine latent proteins under thecontrol of the transcription factor EBNA2 (38, 39, 42).This state of infection is referred to as the growth program (35)or latency 3 (27), and EBNA2 expression is a specific characteristicof EBV-infected B cells using this program. Like other membersof the herpesvirus family, EBV also has the capacity to establisha life-long, persistent infection. Despite the pathogenic potentialof the virus, life-long infection is benign in the overwhelmingmajority of the infectedpopulation.

Recent studies have begun to unravel the mechanism of persistent infection in healthy individuals, which is at variance withthe pathogenic behavior classically associated with EBV. In theperipheral blood of healthy carriers, the virus is tightly restrained,being found only in resting memory B cells (4, 19). The onlylatent gene to be consistently expressed in the peripheral bloodis LMP2 (5, 26, 36), and there is evidence to suggest thateven this gene may not be expressed in the majority of the infectedcells (3). We have referred to this state as the latency program(35) and proposed that these cells are the site of long-termpersistent infection because they are not a pathogenic threatto the host and are probably not subject to immunosurveillance.If true, then EBV, in its site of persistence, is much like theother herpesviruses in that it persists in a transcriptionallyquiescent state in a long-lived, resting cell. The ability ofEBV to establish a latent infection in a resting B cell raisesthe question of what the role of the EBV growth program may beinvivo.

Cells expressing the growth program have been detected in the blood during acute infectious mononucleosis (36) but havenever been found in healthy, persistently infected individuals(19, 36), even when immunosuppressed (3). It is now wellestablished that all healthy carriers have large numbers of cytotoxicT cells (CTL) that recognize epitopes from latent proteins thatare uniquely expressed during the growth program, namely, EBNA2and the EBNA3s (reviewed in reference 13). The suggestion hasbeen made that the lymphoblastoid form of latency is undetectablein healthy carriers because the cells are immediately destroyedby CTL. This led to the proposition that the growth program maybe required to establish a latent infection before the CTL responsearises, but thereafter it is not required for life-long maintenanceof the persistent infection (15, 18, 28).

It is believed that EBV establishes infection through exposure of the mucosal lymphoepithelium to saliva containing infectiousvirus. Similarly, it is believed that the virus is shed from themucosal lymphoepithelium into saliva (2). Recently we observedthat, in tonsils, unlike the peripheral blood, there are significantnumbers of latently infected, naive B cells, and their presenceis associated with ongoing viral replication (4). In rare caseswhen we were unable to detect viral replication, infected, naiveB cells were absent. This led to the suggestion that naive B cellsin the tonsil are being infected with EBV to produce proliferatinglymphoblasts driven by the growth program (4). These infectednaive B cells would either be killed by CTL or differentiate withinthe tonsil to become resting memory B cells (32, 33). Thelatently infected cells could then leave the tonsil, accountingfor the restriction of EBV to memory cells in theperiphery.

In this study, we have used reverse transcription-PCR (RTPCR) analysis for EBNA2 expression to screen B-cell subsets froma panel of healthy tonsils, to test for cells expressing the growthprogram. We found that EBNA2 was consistently expressed but onlyin the naive B-cell subset, as predicted from our previous studies.Furthermore, the latently infected, naive B cells express allof the growth program latent proteins expected for B cells thathave been directly infected withEBV.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells and cell lines. An in vitro-immortalized, EBV-positive lymphoblastoid cell line was used as a positive control for DNA PCR and RTPCR for EBNA1(U-K), EBNA2, EBNA3a, EBNA3b, EBNA3c, LMP1, and LMP2a. Rael (giftof S. Speck), an EBV-positive Burkitt's lymphoma cell line, wasused as a positive control for EBNA1 (Q-K) RTPCR. The cell lineswere maintained in 5% CO₂ in RPMI 1640 with 10% fetal bovine serumand penicillin andstreptomycin.

Tonsils were obtained from patients undergoing routine tonsillectomies, primarily for obstructed-breathing disorders, at theNew England Medical Center and the Massachusetts General Hospital.Tonsils were minced in PBSA (phosphate-buffered saline [PBS] with0.5% bovine serum albumin), and the resulting suspension was passedthrough a silkscreen to remove any connective tissue. The cellsuspension was diluted to 10⁸ cells/ml, layered onto Ficoll-Hypaque (Pharmacia), and centrifugedat 2,000 rpm for 30 min at 25°C. Buffy coats were removed, washedtwice with PBSA, and centrifuged at 1,200 rpm for 15 min. Theisolated lymphocytes were then either stored frozen in aliquotsfor future study or fractionated into immunoglobulin D-positive(IgD⁺) and IgD subsets. The frequency of virus-infected cells was estimatedfor each subpopulation by limiting-dilution DNA PCR as describedbelow. Lymphocytes from EBV-negative tonsils were used as negativecontrols for all RTPCR experiments and were also used to bringthe cell number up to 5 × 10⁶ when necessary prior to mRNAisolation.

Magnetic bead separations. Tonsillar mononuclear cells were resuspended to 2 × 10⁷ cells/ml in PBSA as 1-ml aliquots. To positively select the naive (IgD⁺) population, biotinylated anti-IgD antibody (0.015 µg) (SouthernBiotech catalog no. 2030-08) was added to each tube and incubatedon a rotator at 4°C for 30 min. All tubes were washed two timeswith PBSA and resuspended to 180 µl in the same buffer. Then 20µl of streptavidin-coated microbeads (Miltenyi) was added to eachtube and incubated for 10 min at 4°C. Cells were again washedand resuspended in 500 µl for separation using a magnetic cellseparation column (Miltenyi) and kept at 4°C at all times. TheMACS column (AS or CS, depending on the cell number) was preparedby rinsing with 5 column volumes of PBSA and then inserted intoa VarioMACS magnet. The flow rate of the column was adjusted byattaching a 25- (AS) or 23 (CS)-gauge needle to the base of thestopcock. Cells were then loaded onto the column, and the negativefraction was collected. The cells were washed through by applying3 column volumes of PBSA to the column while still attached tothe magnet. The retained population was then washed by removingthe column from the magnet and injecting 1 column volume of PBSAfrom the bottom of the column using the side syringe supplied.The needle was then replaced with a 23- (AS) or 21 (CS)-gaugeneedle, the column was reinserted into the magnet, and cells wereallowed to flow through. These cells were collected as the washfraction and discarded. The column was again rinsed with 3 columnvolumes of PBSA as before to remove any remaining nonspecificallybound cells. The column was then removed from the magnet, theneedle was removed, and the column was washed with 5 column volumesof PBSA to elute the retained cells. The resulting IgD⁺ fraction was set aside, and the IgD B-cell fraction was isolated from the whole IgD fraction by positive selection for the pan-B-cell marker CD19.The biotinylated anti-CD19 antibody was prepared in our own laboratoryand was used at 0.072 µg/ml pertube.

FACS cell sorting. To isolate CD80-positive and -negative IgD⁺ B cells, whole tonsillar lymphocyte populations were resuspended to 5 × 10⁷ cells/ml in PBSA as 1-ml aliquots. The cells were then labeledby incubating each tube with 0.09 µg of phycoerythrin (PE)-conjugatedanti-CD80 (Pharmingen) and fluorescein isothiocyanate (FITC)-coupledanti-IgD (1:100 dilution of stock [Southern Biotech]) or 0.55µg of FITC-coupled anti-CD80 (Pharmingen) and PE-conjugated anti-IgD(Southern Biotech). After the cells were labeled and washed, theywere fractionated with either a FACStar (Becton Dickinson) orMoFLo (Cytomation) cell sorter for fluorescence-activated cellsorting(FACS).

FACS analysis and antibodies. All fractionated populations were analyzed using a Becton Dickinson FACScan or FACSCalibur. After separations, all columnfractions were stained with a PE-conjugated anti-IgD (SouthernBiotec) as well as anti-CD20-FITC (Dako) for reanalysis to assesspurity and recovery. As negative controls, MOPC21 (IgG1 isotypecontrol; Sigma), 1a2 (IgG2a isotype control; this laboratory),and MOPC121 (IgG2b isotype control; Sigma) wereused.

Limiting-dilution DNA PCR. The absolute frequency of virus-infected cells in a given population was estimated by limiting-dilution DNA PCR analysis witha DNA PCR assay that can detect the presence of a single viralgenome in as many as 10⁶ uninfected cells. The quantitative and technical aspects of thisassay have been detailed elsewhere (12). Isolated populationswere serially diluted, and replicates, usually eight, of eachdilution were prepared in a 96-well V-bottomed microtiter plate(Immulon). The plate was centrifuged at 1,500 rpm for 15 min at4°C, and the supernatant was aspirated. Then, 10 µl of a lysissolution containing 0.45% Tween 20, 0.45% NP-40, 2 mM MgCl₂, 50mM KCl, 10 mM Tris (pH 8.3), and 0.5 mg of proteinase K per mlwas added to each well, and the plate was incubated for at least2 h at 55°C. After incubation, the plate was centrifuged quicklyto remove condensation from the lid of the plate. PCR was performedin a final volume of 50 µl per reaction; 5 µl of cell lysate wasadded to each PCR. The PCR and Southern blotting conditions havebeen described in detail previously (20).

Poisson statistics were used to determine the absolute number of infected cells from the limiting-dilution analysis as describedpreviously (12, 20). To exclude the possibility of externalcontamination of the DNA PCR, we included eight negative DNA samplesper analysis. Furthermore, the lack of contamination could beconfirmed since the PCR signals always fractionate consistently,for example, into the IgD subset of peripheral blood cells, and the signals titrated out,i.e., they were weaker and less frequent with fewercells.

cDNA synthesis. Cells (usually 5 × 10⁶) were pelleted in a microcentrifuge tube, resuspended in 1 ml of Trizol reagent (Gibco-BRL), and incubatedat room temperature for 5 min. Then, 200 µl of chloroform wasadded, and the tube was shaken vigorously for 10 s. The suspensionwas incubated at room temperature for 5 min and centrifuged at11,500 rpm in an Eppendorf microcentrifuge for 15 min at 4°C.The top aqueous layer was transferred to a fresh microcentrifugetube containing 500 µl of isopropyl alcohol and incubated for10 min at room temperature. The tube was centrifuged at 11,500rpm for 10 min at 4°C, and the supernatant was aspirated. Then,1 ml of 75% ethanol was added, and the tube was vigorously vortexed,and again centrifuged at 9,200 rpm for 5 min at 4°C. The supernatantwas aspirated, and the pellet was allowed to dry for 10 min atroom temperature. The pellet was resuspended in 7 or 14 µl ofhigh-pressure liquid chromatography water (HPLC H₂O) at 55°C for15min.

To synthesize cDNA from purified RNA, 7 µl of RNA suspension was transferred to a 200-µl Microamp reaction tube, and 5 µlof random primers (50 ng/µl; Gibco-BRL) was added to the RNA suspension.The mix was heated at 68°C for 8 min, followed by a 2-min incubationon ice. The tubes were rapidly centrifuged to remove condensation,and 7 µl of a mix containing 1 µl of 10 mM deoxynucleoside triphosphates(dNTPs), 4 µl of 5× Superscript II buffer (375 mM KCl, 250 mMTris [pH 8.4], 15 mM MgCl₂), and 2 µl of 100 mM dithiothreitolwas added. The reaction was incubated at room temperature for10 min, followed by the addition of 50 U of Superscript reversetranscriptase (Gibco-BRL catalog no. 18064-014) and incubationat room temperature for an additional 10 min. Next, the tube wasincubated at 42°C for 50 min, and the reaction was stopped byincubation at 68°C for 15 min. The volume was made up to 100 µlby addition of 80 µl of HPLC H₂O, and 20 µl was used for eachPCR.

PCR of latent gene products. PCR was performed on the synthesized cDNA for EBNA1 (U-K), EBNA1 (Q-K), EBNA2, EBNA3a, EBNA3b, EBNA3c, LMP1, and LMP2a. Reactionconditions for each were 50 mM KCl, 20 mM Tris (pH 8.4), 0.2 mMdNTPs, and 20 pM each of the amplimers. MgCl₂ was 2 mM for EBNA1(U-K), EBNA3a, EBNA3b, EBNA3c, and LMP2a, 2.5 mM for EBNA1 (Q-K),and 3.0 mM for EBNA2 and LMP1. The amplimers were as follows:EBNA1 (U-K): E1U (5'-AGCTTCCCTGGGATGAGCGT-3') and E1K (5'-TCTTCCCCGTCCTCGTCCAT-3')(26); EBNA1 (Q-K), RT3 (5'-TGGCCCCTCGTCAGACATGATT-3') and Qb(5'-AGCGTGCGCTACCGGAT-3') (gift from Sam Speck); EBNA2, E2F (5'-CATAGAAGAAGAAGAGGATGAAGA-3')and E2R (5'-GTAGGGATTCGAGGGAATTACTGA-3') (26); EBNA3a, L1 (5'-TCTTCCATGTTGTCATCCAGGG-3')and U1 (5'-CTTAGGAAGCGTTTCTTGAGCTT-3'); EBNA3b, E3B-S (5'-TTCCATGTTGCAATCGGACC-3')and E3B-AS (5'-AAAGTGACCTAGCACGACGT-3') (gift from Robert Touitou);EBNA3c, E3C-S (5'-GGGCTGTCAAGCAATCGCAC-3') and E3C-AS (5'-GTGGTGCATTCCACGGGTAA-3')(gift from Robert Touitou); LMP1, L1F (5'-TTGGTGTACTCCTACTGATGATCACC-3')and L1R (5'-AGTAGATCCAGATACCTAAGACAAGT-3') (26); and LMP2a,L2F (5'-ATGACTCATCTCAACACATA-3') and L2R (5'-CATGTTAGGCAAATTGCAAA)(26).

Master mixes with the indicated conditions were aliquoted to 200-µl Microamp reaction tubes, and 20 µl of the cDNA suspensiondescribed above was added to give a final volume of 50 µl. Thereforeit was possible to perform RTPCR for up to five different latentgenes from one cDNA pot. Reactions were incubated at 95°C for5 min, and 1 U of Taq DNA polymerase (Perkin Elmer) was addedto each tube. The tubes were loaded in a Geneamp 9600 thermocyclerand the following conditions were run: for EBNA1 (Q-K), EBNA3a,EBNA3b, EBNA3c, and EBNA2, 95°C for 15 s, 62°C for 30 s, and 72°Cfor 30 s, repeated for 40 cycles; for EBNA1 (U-K) and LMP1, 95°Cfor 15 s, 65°C for 30 s, and 72°C for 30 s, repeated for 40 cycles;for LMP2a, 95°C for 15 s, 55°C for 30 s, and 72°C for 1 min, repeatedfor 40cycles.

All reactions were concluded with a 5-min incubation at 72°C to complete the extension of all synthesized products. PCR productswere electrophoresed on agarose gels, blotted, and probed as describedabove.

RTPCR products were analyzed in the same manner as the DNA PCRs except the PCR products were detected by probing Southernblots with ³²P-random-primed PCR products isolated from an EBV-positive lymphoblastoidor Rael cell line. An EBV-positive lymphoblastoid cell line wasused as a positive control for RTPCR for EBNA1 (U-K), EBNA2, EBNA3a,EBNA3b, EBNA3c, LMP1, and LMP2a, and the Rael Burkitt's lymphomacell line was used as a positive control for EBNA1 (Q-K) RTPCR.These protocols detect the mRNA from 1 EBV-positive cell in thepresence of 5 × 10⁶ EBV-negative tonsil cells (see Fig. 2).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Naive (IgD⁺) but not IgD B cells from the tonsil express EBNA2, the latent gene characteristic of the lymphoblastoid growth program. When EBV newly infects resting B cells, EBNA2 is the first gene to be expressed (1, 29), and it regulates the expressionof all the other latent genes (38, 39, 42). The result isan activated lymphoblast proliferating under the control of thegrowth program. Thus, EBNA2 expression is a specific marker forthe lymphoblastoid growth program. To test if the infected IgD⁺ population from the tonsil bore the hallmarks of direct infection,we have screened a panel of tonsils for EBNA2expression.

Tonsillar B cells were fractionated into IgD⁺ (naive) and IgD (memory plus germinal center) B cells using biotinylated antibodiesand the MACS system (Fig. 1). The cells were then split into twoaliquots. The first aliquot was used to generate a limiting-dilutionseries for DNA PCR analysis to estimate the absolute frequencyof virus-infected cells in the two populations. The second aliquotwas used to isolate mRNA from the two populations of cells forcDNA preparation and PCR analysis for EBNA2 expression.

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FIG. 1. FACS analysis of tonsillar lymphocytes before and after purification of the naive (IgD⁺) and IgD populations. Naive (IgD⁺) and IgD B cell subsets were isolated from whole tonsils using the MACS system as described in Materials and Methods. IgD⁺ cells were first isolated by positive selection with biotinylated antibodies to IgD. The remaining cells were then positively selected for the IgD B cells using a biotinylated antibody to CD19. The resulting populations were stained with a FITC-coupled antibody to the pan-B-cell marker CD20 and a PE-coupled antibody to IgD. The left-hand panel shows whole tonsillar lymphocyte staining prior to separation; the middle panel shows IgD⁺ B cells (96% pure); and the right panel shows IgD B cells (97% pure).

The results of the RTPCR analysis from five such tonsils are shown in Fig. 2A, and a summary of results from 16 tonsils aregiven in Table 1. EBNA2 was detected in the IgD⁺ population (13 of 16) but never in the IgD population (0 of 16). For each tonsil, multiple negative controlsand a sensitivity control of the type shown in Fig. 3 were performed.The failure to detect EBNA2 in the IgD⁺ cells from 3 of the 16 tonsils could genuinely reflect a lackof EBNA2 expression; however, we suspect it is more likely a consequenceof a technical failure. Although the overall quality of the cDNAin these samples appeared good, the number of infected cells isso small that relatively minor variations in the cell fractionationor cDNA synthesis protocol could cause a false-negative result.Due to limited amounts of material, it was not possible to reanalyzethe cells from these three tonsils. The failure to detect EBNA2in any of the IgD population, however, was consistent even when sufficient cellswere available to confirm the negative result. Furthermore, fortonsils for which sufficient cells were available, we have preformedspiking experiments in which 5 or 1 infected cell from an in vitro-transformedlymphoblastoid cell line was added to the purified IgD B cells prior to mRNA extraction. An example of one such experimentis shown in Fig. 2B. This result confirms that the EBNA2 transcriptwas detectable in the IgD⁺ but not the IgD cells. However, EBNA2 was detected when the EBV lymphoblastswere spiked into the IgD sample.

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FIG. 2. EBNA2 is expressed by latently infected naive but not IgD B cells in the tonsil. IgD⁺ (naive) and IgD B cells were isolated from tonsils using biotinylated antibodies and MACS columns as described in the legend to Fig. 1. RTPCR was then performed on 5 × 10⁶ cells from each population. The PCR products were fractionated on agarose gels, Southern blotted, and probed with a sequence-specific probe. For details see the text. The expected position of the PCR product is indicated by the arrow. (A) Examples from five different EBV-positive tonsils. D+, surface IgD⁺ B-cell population; D $-$ , surface IgD B-cell population. (B) Results from a single tonsil with spiking and negative controls. Either five or one cell from an EBNA2-positive lymphoblastoid cell line (LCL) was spiked into the IgD population prior to mRNA extraction for EBNA2 RTPCR. The negative controls are B cells from tonsils that were EBV negative in the DNA PCR assays used to derive the frequencies shown in Table 1.

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TABLE 1. EBNA2 latent gene expression in latently infected naive and IgD B cells from tonsils^a

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FIG. 3. Sensitivity of the RTPCR assays used. cDNA prepared from EBV-positive cell lines was serially diluted into cDNA from EBV-negative tonsils to generate 100, 10, and 1 cell equivalents. The negative controls are B cells from EBV-negative tonsils alone. The expected positions of the PCR products are indicated by the arrows. Similar sensitivity and negative controls were performed for all experiments. An EBV-positive lymphoblastoid line was used for all RTPCRs except EBNA1 (Q-K), for which Rael cells were used. All of the assays could detect a single cell equivalent, although the EBNA3a assay was significantly less sensitive than the others. D+, surface IgD⁺ B-cell population; D $-$ , surface IgD B-cell population.

The failure to detect an EBNA2 transcript in the IgD population was not a consequence of lower levels of virus infection inthis subset. The estimated frequencies of virus-infected cellsin the naive (IgD⁺) and IgD populations, shown in Table 1, demonstrate that for any giventonsil there were as many, if not more, infected cells in theIgD population as in the IgD⁺ population. We conclude, therefore, that EBNA2 is reproduciblyexpressed in the naive (IgD⁺) but not the IgD population fromtonsils.

Naive but not IgD B cells from the tonsil also express the EBNA3 family of latent genes. In addition to EBNA2, the other latent genes that are restricted in their expression to the growth program are EBNA3a, -b,and -c (reviewed in reference 27). Therefore, we analyzed EBNA2,EBNA3a, EBNA3b, and EBNA3c expression in IgD⁺ and IgD cells from an additional five tonsils. The results for two representativetonsils are shown in Fig. 4, and a summary of the results forall five tonsils are presented in Table 2. We found that EBNA2,EBNA3a, EBNA3b, and EBNA3c expression was restricted to the IgD⁺ subset; none were found in the IgD population (Fig. 4A). However, the EBNA3s were not detected intwo of five of the tonsils tested (Fig. 4B) even though EBNA2expression was reproducibly detected in all five. The reason forthese negative results is unclear. They were not due to technicalfailures, since both tonsils were retested for EBNA3 expressionin at least three independent experiments and were uniformly negative,while control and spiking experiments were positive, and the samecDNA preparations were positive for EBNA2. It is possible thata subset of tonsils contain infected IgD⁺ cells that express EBNA2 without the EBNA3s, but it is unclearwhy this would happen in some tonsils and not others, unless itwas caused by differential and transient gene expression in subsetsof IgD⁺ cells. This seems unlikely, given the tight linkage between expressionof EBNA2 and the EBNA3s. Technical explanations seem more likely.All of the RTPCR assays we have used readily detect gene expressionin a single cell infected in vitro (Fig. 3). The exception isEBNA3a, for which 10 or more cells are required to obtain a strongsignal. Therefore, failure to detect EBNA3a may simply reflectthe lack of sensitivity of the assay. A more likely explanationfor the discrepancy between EBNA2 and EBNA3 detection is thatthe transcript copy number for the EBNA3s may be significantlylower in the in vivo-infected cells than in the cell lines, whereasthe EBNA2 transcript level may be similar. It is also conceivablethat our EBNA3 primers do not detect all of the viral isolatesdue to sequence variation in the EBNA3 genes.

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FIG. 4. EBNA3 proteins are expressed by latently infected naive but not IgD B cells in the tonsil. IgD⁺ (naive) and IgD B cells were isolated from tonsils using biotinylated antibodies and MACS columns as described in the legend to Fig. 1. cDNA was prepared from 5 × 10⁶ cells of each population and divided for DNA PCR detection of EBNA2, EBNA3a, EBNA3b, and EBNA3c. The PCR products were fractionated on agarose gels, Southern blotted, and probed with sequence-specific probes. For details, see the text. The expected positions of the PCR products are indicated by the arrows. (A) Representative example of tonsils that express EBNA2 and all of the EBNA3 family. (B) Representative example of tonsils that express EBNA2 but lack detectable EBNA3s.

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TABLE 2. EBV latent gene expression in latently infected naive and IgD B cells from tonsils^a

Combining the results in Tables 1 and 2, we found EBNA2 expressed in IgD⁺ B cells from 13 of 16 tonsils and in the IgD population from 0 of 16. EBNA3a, -b, and -c were found in IgD⁺ cells from three of five tonsils and in the IgD population from zero offive.

Expression of other latent genes in the IgD⁺ population. The growth program is characterized by expression of the EBNA2 and EBNA3 genes. EBNA1 and the latent membrane proteins (LMPs)are also expressed, but they are not unique to the growth program.They are also present in the more restricted forms of latencyfound in tumors such as Hodgkin's lymphoma (10, 21, 23,24) and nasopharyngeal carcinoma (6, 8, 41). In thesetumors, EBNA2 and the EBNA3s are not expressed. The only EBNAfound is EBNA1, and it is expressed from a unique promoter (Qp)(22, 30, 37) that is not used in the growth program. Toassess if the overall pattern of latent gene expression in latentlyinfected, naive B cells was consistent with the growth program,we screened IgD⁺ B cells from a panel of six tonsils for expression of the EBNA1(U-K) and EBNA1 (Q-K) transcripts and the LMP1 and LMP2 genes.An example of the results obtained with three tonsils is shownin Fig. 5A, and a summary of all the results obtained is shownin Table 3. Typical sensitivity and negative controls are shownin Fig. 3. As expected, from the studies already described, EBNA2was detected in all of the samples of IgD⁺ cells tested. In addition, LMP1 and LMP2 were also expressedin the IgD⁺ cells from six of six tonsils. We were unable to detect the presenceof the Qp-derived form of the EBNA1 transcript in six of six tonsils,although EBNA1 itself was being produced, since three of threetonsils negative for EBNA1 (Q-K) were positive for EBNA1 (U-K).This RTPCR detects all of the known splice variants of the EBNA1transcript. To test if the failure to detect EBNA1 (Q-K) was dueto technical difficulties with our assay, we spiked differentnumbers of Rael cells into the tonsillar B-cell preparations.Rael is a Burkitt's lymphoma line that expresses the EBNA1 (Q-K)transcript. As shown in Fig. 5B, we readily detected EBNA1 (Q-K)when as few as 1 Rael cell was spiked into the tonsillar B cell.Thus, the pattern of latent genes found in the IgD⁺ population is EBNA1⁺, EBNA2⁺, EBNA3a⁺, EBNA3b⁺, EBNA3c⁺, LMP1⁺, and LMP2⁺ but EBNA1 (Q-K) negative. This is precisely the expected patternfor the growth program associated with the lymphoblastoid formof latency found in directly infected cells in vitro.

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FIG. 5. Naive (IgD⁺) B cells express all of the latent genes expected for the growth program. IgD⁺ (naive) B cells were isolated from tonsils using biotinylated antibodies and MACS columns as described in the legend to Fig. 1. cDNA was prepared from 5 × 10⁶ cells and divided for DNA PCR detection of EBNA1 (U-K), EBNA1 (Q-K), EBNA2, LMP1, and LMP2. The PCR products were fractionated on agarose gels, Southern blotted, and probed with sequence-specific probes. For details, see the text. The expected positions of the PCR products are indicated by the arrows. (A) Results from three tonsils. (B) Spiking control, in which cells from the EBNA1 (Q-K)-positive Rael cell line were diluted into naive tonsillar B cells prior to mRNA extraction for RTPCR detection of EBNA1 (Q-K).

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TABLE 3. EBV latent gene expression in latently infected naive B cells from tonsils

Latently infected naive (IgD⁺) tonsillar B cells express an activated surface phenotype. Resting naive B cells are negative for expression of the costimulatory molecule B7.1 (CD80). This molecule is expressed athigh levels when naive B cells become activated lymphoblasts througheither antigen activation or EBV infection (9). To test ifEBV-infected, naive (IgD⁺) B cells were phenotypically activated, we isolated tonsilarlymphocytes and stained for IgD and CD80 expression. The cellswere then fractionated into IgD⁺ CD80⁺ (activated naive) and IgD⁺ CD80 (resting naive) B cells using MoFlo FACS. An example of the stainingprofile and sort gates is shown in the left-hand panel of Fig.6A, and reanalysis of the purified populations is shown in themiddle and right panels. The frequency of virus-infected cellsin each population was then estimated using the limiting-dilutionDNA PCR assay. The PCR results for one experiment are shown inFig. 6, and the quantitation from two such experiments is summarizedin Table 4. It can readily be seen that separation on the basisof CD80 expression resulted in a marked enrichment of the virus-infectedcells into the CD80⁺ fraction. The percentage of IgD⁺ cells expressing CD80 could be estimated from the FACS analysisprior to sorting. From these numbers, it is possible to backcalculatethe absolute numbers of virus-infected cells residing in eachfraction. For experiment number 1, >90% of the infected cellscould be accounted for in the CD80⁺ fraction, whereas in experiment 2, approximately 80% were inthe CD80⁺ fraction. These represent rough estimates; nevertheless, overallthe experiments are consistent with most if not all of the infectedIgD⁺ naive B cells expressing an activated cell surface phenotype.

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FIG. 6. Limiting-dilution DNA PCR analysis of activated (CD80⁺) and resting (CD80) naive (IgD⁺) tonsillar B cells. (A) Whole tonsils were stained with a FITC-coupled antibody to CD80 and a PE-coupled antibody to IgD. The presort staining and the sort gates are shown in the dot plot to the left, taken from a Cytomation MoFlo cell sorter. Reanalysis of the isolated population is shown in the middle (93% pure CD80⁺ IgD⁺ cells) and right (99% pure CD80 IgD⁺ cells) panels analyzed on a FACSCalibur. (B) The cells were serially diluted, and EBV-specific DNA PCR was performed on replicates of each cell dilution. The PCR products were fractionated on an agarose gel, Southern blotted, and probed with a sequence-specific probe. The fraction of negative samples at each dilution was then estimated, and the fractions were used to calculate an absolute frequency of infected cells using Poisson statistics. Only a limited amount of the whole dilution series is shown. The expected positions of the PCR products are indicated with arrowheads.

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TABLE 4. EBV-infected naive B cells from tonsils are CD80 positive^a

EBV-infected naive (IgD⁺) B cells are not always detected in EBV-positive tonsils. We have developed a quantitative, limiting-dilution assay that allows the measurement of absolute numbers of EBV-infectedcells within a given population of cells (12, 20). With thisassay, we have shown previously that peripheral blood, a siteof persistent infection, contains infected IgD B cells but completely lacks infected IgD⁺ (naive) B cells (4). In comparison, tonsils contain both infectedIgD⁺ and IgD B cells. We noted, however, that there were rare tonsils thatlacked infected IgD⁺ cells. Infected IgD B cells were found in 100% of the samples tested for both (59of 59) tonsils and peripheral blood (16 of 16) (Table 5). However,infected IgD⁺ (naive) cells were only found in 90% of the tonsils (52 of 59)and were never found in the peripheral blood (0 of 16). None ofthe tonsils contained infected IgD⁺ B cells in the absence of infected IgD B cells. In an analysis of a limited number of tonsils, we showedpreviously (4) that five of five tonsils with infected IgD⁺ B cells contained linear viral DNA characteristic of infectiousvirus, whereas two of two tonsils that lacked infected IgD⁺ cells lacked linear DNA. We interpret these results to mean thatthe virus persists within IgD B cells throughout the lymphoid system, but the IgD⁺ cells are being directly infected by the virus in the tonsilsand are either killed or differentiate into IgD B cells before they can leave the tonsil.

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TABLE 5. Tonsils always contain infected IgD B cells, but some tonsils lack infected naive (IgD⁺) B cells^a

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this paper, we report that the tonsillar lymph nodes of healthy carriers of EBV contain infected lymphoblastoid cells thatexpress the growth latency program. We further show that thesecells are all IgD⁺ (naive) B cells. In a previous study, we demonstrated a directcorrelation between the detection of these infected IgD⁺ cells and the presence of viral replication. Since the naive,infected lymphoblasts are not found when infectious virus is absent(4), we conclude that they are not a self-sustaining compartmentof viral persistence. Instead, they are being continuously generatedby direct infection with the virus and then removed, either throughdifferentiation (see below) or through the actions ofCTL.

The lymphoblastoid growth program has already been characterized extensively because it is the program used when the virusestablishes latency in vitro. However, lymphoblastoid cells expressingthe growth latency program have only been detected before in vivoduring acute infectious mononucleosis (36). These cells stimulatea rapid and potent CTL response that is particularly focused onthe EBNA2 and EBNA3 latent proteins (13), which are uniquelyexpressed by the growth program. The CTL response is thought toeliminate infected cells, driven to proliferate by the growthprogram, before they develop into a pathogenic threat. This threatis revealed in immunosuppressed individuals who are at risk fordeveloping life-threatening lymphomas derived from B cells expressingthe growth program (31, 40).

The oncogenic risk to the host posed by proliferating, EBV-infected lymphoblasts has led to the suggestion that the EBV-encodedgrowth program is essential for the establishment of latency duringacute infection, before the CTL response arises. Thereafter, theproliferating lymphoblasts are killed as soon as they are producedand play no role in the maintenance of persistent latent infection.This view now appears too simple. The frequency of infected IgD⁺ cells in the tonsil is comparable to that of infected IgD cells in the periphery $---$ a population that is presumably underless immunosurveillance because the major CTL target antigens,EBNA2 and the EBNA3s, are not expressed (5, 26, 36). Itappears, therefore, that the CTL response is not particularlyeffective in eliminating the naive, infected lymphoblasts. Furthermore,it is noteworthy that the lymphomas that arise in allograft patients,in whom the CTL response is suppressed iatrogenically, are notIgD⁺ (11). This implies that CTL are not required to regulate theIgD⁺ cells expressing the growth program in thetonsil.

The key to understanding why latently infected, naive B cells in the tonsil express the growth program but may not requireimmunosurveillance lies, we believe, in the specificity of theinfection process for the naive compartment and in our model ofEBV persistence. It is well known that EBV has no specificityfor naive B cells in vitro; it can equally well infect and growth-transformmemory B cells. Yet we have shown in this study that only naiveIgD⁺ B cells are being infected by EBV and driven to express the growthprogram. The explanation must be that infectious virus is restrictedto regions of the tonsil that contain only naive B cells. Theonly region of the tonsil that is highly enriched for naive IgD⁺ B cells and lacks other B cell types is the mantle zone thatsurrounds the follicles (16, 25). It would be a reasonablescenario to suggest that latently infected memory B cells fromthe periphery extravasate in the marginal zones of the tonsiland reactivate the virus in response to signals that they receiveas they migrate to the mantle zone. Thus, infectious virus wouldonly be produced in regions where IgD⁺, naive B cells werepresent.

We have proposed that EBV-infected, naive B cells in vivo are able to recapitulate B-cell differentiation driven by antigen(4, 32, 33). They do not remain lymphoblasts, but ratherdifferentiate through a germinal center-type reaction (16, 17)to enter the peripheral B-cell pool as resting memory cells. Inthis scenario, expression of the growth program in a naive B cellin a lymph node would be transient and not a pathogenic threateven to the immunosuppressed host. If true, then the CTL existnot to kill infected naive cells in the mantle zone, but to killcells that express the growth program in inappropriate locationswhere they cannot differentiate into a resting memory cell. Thiswould include all nonnaive B cells in lymph nodes and all extranodalB cells that would not have access to follicles to allow differentiation.These ideas are especially interesting in light of recent studiesfrom acute infectious mononucleosis patients (15a). These authorsmicrodissected single cells from the tonsils of infectious mononucleosispatients. They observed that the proliferating EBNA2⁺ clones in the tonsils are memory cells. Since we have never detectedmemory lymphoblastoid cells in the tonsils of healthy carriers,we assume that the situation in infectious mononucleosis is aderegulated one. Here the virus has escaped the usual anatomicalconfines that allow only infection of naive B cells and has infectedmemory cells. These cells grow out of control because they cannotdifferentiate. Eventually these clones of memory cells are destroyedwhen the CTL response arises. The situation in infectious mononucleosisis so atypical that proliferating, infected lymphoblastoid cellsexpressing the growth program are even present in the peripheralblood (36). Such cells have never been found in the blood ofhealthy carriers of the virus (5, 26, 36) even when immunosuppressed(3). It is our presumption that it is the role of the CTL toclear these types of aberrant and uncontrolled infections of Bcells in the lymph nodes and in the blood. The infection of naiveB cells in the tonsils is, by comparison, regulated by differentiationand may not require surveillance byCTL.

One caveat to our experiments is that we do not know what fraction of the infected IgD⁺ naive cells are actually expressing the growth program. In previousstudies, we have shown that all of the EBV-positive naive cellsare latently infected (7), but it is conceivable that a largefraction of the infected cells are resting and expressing noneof the growth-promoting latent genes. However, it is difficultto conceive how this could occur. When EBV infects B cells, theyautomatically go to the growth program and start to proliferate;there is no evidence that other forms of latency are adopted.Such infected, naive B cells in vivo would then have to leavethe cell cycle and be maintained as resting naive B cells thatstay in the tonsil, because there are no infected naive B cellsin the peripheral blood. Such behavior has never been documentedfor a normal naive B cell. Activated naive B cells can only exitthe cell cycle through differentiation ordeath.

In conclusion, cells in the tonsil expressing the growth program, characteristic of direct infection, are restricted to thenaive subset. It will be important now to characterize the typeand location of cells that replicate the virus in the tonsilsof healthy carriers and identify the signals that are requiredin vivo to initiate viralreplication.

	ACKNOWLEDGMENTS

We thank Allen Parmalee for excellent flow cytometry and Cheryl Greene for providing thetonsils.

The authors' work is supported by Public Health Service grants AI 18757 and CA65883.

	FOOTNOTES

^* Corresponding author. Mailing address: Dept. of Pathology, Tufts University School of Medicine, 136 Harrison Ave., Boston,MA 02111. Phone: (617) 636-2726. Fax: (617) 636-2990. E-mail:dlawson{at}opal.tufts.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. 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].

2. Anagnostopoulos, I., M. Hummel, C. Kreschel, and H. Stein. 1995. Morphology, immunophenotype, and distribution of latently and/or productively Epstein-Barr virus-infected cells in acute infectious mononucleosis: implications for the interindividual infection route of Epstein-Barr virus. Blood 85:744-750[Abstract/Free Full Text].

3. Babcock, G. J., L. L. Decker, R. B. Freeman, and D. A. Thorley-Lawson. 1999. Epstein-Barr virus-infected resting memory B cells, not proliferating lymphoblasts, accumulate in the peripheral blood of immunosuppressed patients. J. Exp. Med. 190:567-576[Abstract/Free Full Text].

4. Babcock, G. J., L. L. Decker, M. Volk, and D. A. Thorley-Lawson. 1998. EBV persistence in memory B cells in vivo. Immunity 9:395-404[CrossRef][Medline].

5. Chen, F., J. Z. Zou, R. L. DiRenzo, 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. Deacon, E. M., G. Pallesen, G. Niedobitek, J. Crocker, L. Brooks, A. B. Rickinson, and L. S. Young. 1993. Epstein-Barr virus and Hodgkin's disease: transcriptional analysis of virus latency in the malignant cells. J. Exp. Med. 177:339-349[Abstract/Free Full Text].

7. 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].

8. Fahraeus, R., H. L. Fu, I. Ernberg, J. Finke, M. Rowe, G. Klein, K. Falk, E. Nilsson, M. Yadav, P. Busson, et al. 1988. Expression of Epstein-Barr virus-encoded proteins in nasopharyngeal carcinoma. Int. J. Cancer 42:329-338[Medline].

9. Freedman, A. S., G. Freeman, J. C. Horowitz, J. Daley, and L. M. Nadler. 1987. B7, a B-cell-restricted antigen that identifies preactivated B cells. J. Immunol. 139:3260-3267[Abstract].

10. Herbst, H., F. Dallenbach, M. Hummel, G. Niedobitek, S. Pileri, L. N. Muller, and H. Stein. 1991. Epstein-Barr virus latent membrane protein expression in Hodgkin and Reed-Sternberg cells. Proc. Natl. Acad. Sci. USA 88:4766-4770[Abstract/Free Full Text].

11. Kaplan, M. A., J. A. Ferry, N. L. Harris, and J. O. Jacobson. 1994. Clonal analysis of posttransplant lymphoproliferative disorders, using both episomal Epstein-Barr virus and immunoglobulin genes as markers. Am. J. Clin. Pathol. 101:590-596[Medline].

12. Khan, G., E. M. Miyashita, B. Yang, G. J. Babcock, and D. A. Thorley-Lawson. 1996. Is EBV persistence in vivo a model for B cell homeostasis? Immunity 5:173-179[CrossRef][Medline].

13. Khanna, R., S. R. Burrows, and D. J. Moss. 1995. Immune regulation in Epstein-Barr virus-associated diseases. Microbiol. Rev. 59:387-405[Abstract/Free Full Text].

14. Kieff, E. 1996. Epstein-Barr virus and its replication, p. 2343-2396. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Fields virology, 2nd ed., vol. 2. Raven Press, New York, N.Y.

15. Klein, G. 1994. Epstein-Barr virus strategy in normal and neoplastic B-cells. Cell 77:791-793[CrossRef][Medline].

15a. Kurth, J., T. Spieker, J. Wustrow, J. G. Strickler, M. L. Hansmann, K. Rajewsky, and R. Küppers. Tracing EBV-infected B cells in infectious mononucleosis: viral strategies for spreading in the B cell compartment and establishment of latent infection. Immunity, in press.

16. Liu, Y. J., and C. Arpin. 1997. Germinal center development. Immunol. Rev. 156:111-126[CrossRef][Medline].

17. MacLennan, I. C. 1994. Germinal centers. Annu. Rev. Immunol. 12:117-139[CrossRef][Medline].

18. Masucci, M. G., and I. Ernberg. 1994. Epstein-Barr virus: adaptation to a life within the immune system. Trends Microbiol. 2:125-130[CrossRef][Medline].

19. 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].

20. 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[CrossRef][Medline].

21. Niedobitek, G., E. Kremmer, H. Herbst, L. Whitehead, C. W. Dawson, E. Niedobitek, C. von Ostau, N. Rooney, F. A. Grasser, and L. S. Young. 1997. Immunohistochemical detection of the Epstein-Barr virus-encoded latent membrane protein 2A in Hodgkin's disease and infectious mononucleosis. Blood 90:1664-1672[Abstract/Free Full Text].

22. Nonkwelo, C., J. Skinner, A. Bell, A. Rickinson, and J. Sample. 1996. Transcription start sites downstream of the Epstein-Barr virus (EBV) Fp promoter in early-passage Burkitt lymphoma cells define a fourth promoter for expression of the EBV EBNA-1 protein. J. Virol. 70:623-627[Abstract].

23. Oudejans, J. J., D. F. Dukers, N. M. Jiwa, A. J. van den Brule, F. A. Grasser, P. C. de Bruin, A. Horstman, W. Vos, J. van Gorp, J. M. Middeldorp, and C. J. Meijer. 1996. Expression of Epstein-Barr virus encoded nuclear antigen 1 in benign and malignant tissues harbouring EBV. J. Clin. Pathol. 49:897-902[Abstract/Free Full Text].

24. Pallesen, G., S. J. Hamilton-Dutoit, M. Rowe, and L. S. Young. 1991. Expression of Epstein-Barr virus latent gene products in tumour cells of Hodgkin's disease. Lancet 337:320-322[CrossRef][Medline].

25. Perry, M., and A. Whyte. 1998. Immunology of the tonsils. Immunol. Today 19:414-421[CrossRef][Medline].

26. 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].

27. 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.), Fields virology, 3rd ed., vol. 2. Raven Press, New York, N.Y.

28. Rickinson, A. B., Q. Y. Yao, and L. E. Wallace. 1985. The Epstein-Barr virus as a model of virus-host interactions. Br. Med. Bull. 41:75-79[Abstract/Free Full Text].

29. Robertson, E., and E. Kieff. 1995. Reducing the complexity of the transforming Epstein-Barr virus genome to 64 kilobase pairs. J. Virol. 69:983-993[Abstract].

30. Schaefer, B. C., J. L. Strominger, and S. H. Speck. 1995. Redefining the Epstein-Barr virus-encoded nuclear antigen EBNA-1 gene promoter and transcription initiation site in group I Burkitt lymphoma cell lines. Proc. Natl. Acad. Sci. USA 92:10565-10569[Abstract/Free Full Text].

31. Thomas, J. A., N. A. Hotchin, M. J. Allday, P. Amlot, M. Rose, M. Yacoub, and D. H. Crawford. 1990. Immunohistology of Epstein-Barr virus-associated antigens in B cell disorders from immunocompromised individuals. Transplantation 49:944-953[Medline].

32. Thorley-Lawson, D. A. 1999. EBV $---$ schizophrenic but not dysfunctional. Epstein-Barr Virus Rep. 6:158-163.

33. Thorley-Lawson, D. A., and G. J. Babcock. 1999. A model for persistent infection with Epstein-Barr virus: the stealth virus of human B cells. Life Sci. 65:1433-1453[CrossRef][Medline].

34. Thorley-Lawson, D. A., and K. P. Mann. 1985. Early events in Epstein-Barr virus infection provide a model for B cell activation. J. Exp. Med. 162:45-59[Abstract/Free Full Text].

35. Thorley-Lawson, D. A., and E. M. Miyashita. 1996. Epstein-Barr virus and the B cell: that's all it takes. Trends Microbiol. 4:204-208[CrossRef][Medline].

36. 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].

37. Tsai, C. N., S. T. Liu, and Y. S. Chang. 1995. Identification of a novel promoter located within the Bam HI Q region of the Epstein-Barr virus genome for the EBNA 1 gene. DNA Cell Biol. 14:767-776[Medline].

38. Wang, F., S. F. Tsang, M. G. Kurilla, J. I. Cohen, and E. Kieff. 1990. Epstein-Barr virus nuclear antigen 2 transactivates latent membrane protein LMP1. J. Virol. 64:3407-3416[Abstract/Free Full Text].

39. 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].

40. Young, L., C. Alfieri, K. Hennessy, H. Evans, C. O'Hara, K. C. Anderson, J. Ritz, R. S. Shapiro, A. Rickinson, E. Kieff, et al. 1989. Expression of Epstein-Barr virus transformation-associated genes in tissues of patients with EBV lymphoproliferative disease. N. Engl. J. Med. 321:1080-1085[Abstract].

41. Young, L. S., C. W. Dawson, D. Clark, H. Rupani, P. Busson, T. Tursz, A. Johnson, and A. B. Rickinson. 1988. Epstein-Barr virus gene expression in nasopharyngeal carcinoma. J. Gen. Virol. 69:1051-1065[Abstract/Free Full Text].

42. 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].

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Clambey, E. T., Virgin, H. W. IV, Speck, S. H. (2002). Characterization of a Spontaneous 9.5-Kilobase-Deletion Mutant of Murine Gammaherpesvirus 68 Reveals Tissue-Specific Genetic Requirements for Latency. J. Virol. 76: 6532-6544 [Abstract] [Full Text]
Tune, C. E., Pilon, M., Saiki, Y., Dosch, H.-M. (2002). Sustained Expression of the Novel EBV-Induced Zinc Finger Gene, ZNFEB, Is Critical for the Transition of B Lymphocyte Activation to Oncogenic Growth Transformation. J. Immunol. 168: 680-688 [Abstract] [Full Text]
Harris, R. S., Croom-Carter, D. S. G., Rickinson, A. B., Neuberger, M. S. (2001). Epstein-Barr Virus and the Somatic Hypermutation of Immunoglobulin Genes in Burkitt's Lymphoma Cells. J. Virol. 75: 10488-10492 [Abstract] [Full Text]

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	Abstract

1.	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].
2.	Anagnostopoulos, I., M. Hummel, C. Kreschel, and H. Stein. 1995. Morphology, immunophenotype, and distribution of latently and/or productively Epstein-Barr virus-infected cells in acute infectious mononucleosis: implications for the interindividual infection route of Epstein-Barr virus. Blood 85:744-750[Abstract/Free Full Text].
3.	Babcock, G. J., L. L. Decker, R. B. Freeman, and D. A. Thorley-Lawson. 1999. Epstein-Barr virus-infected resting memory B cells, not proliferating lymphoblasts, accumulate in the peripheral blood of immunosuppressed patients. J. Exp. Med. 190:567-576[Abstract/Free Full Text].
4.	Babcock, G. J., L. L. Decker, M. Volk, and D. A. Thorley-Lawson. 1998. EBV persistence in memory B cells in vivo. Immunity 9:395-404[CrossRef][Medline].
5.	Chen, F., J. Z. Zou, R. L. DiRenzo, 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.	Deacon, E. M., G. Pallesen, G. Niedobitek, J. Crocker, L. Brooks, A. B. Rickinson, and L. S. Young. 1993. Epstein-Barr virus and Hodgkin's disease: transcriptional analysis of virus latency in the malignant cells. J. Exp. Med. 177:339-349[Abstract/Free Full Text].
7.	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].
8.	Fahraeus, R., H. L. Fu, I. Ernberg, J. Finke, M. Rowe, G. Klein, K. Falk, E. Nilsson, M. Yadav, P. Busson, et al. 1988. Expression of Epstein-Barr virus-encoded proteins in nasopharyngeal carcinoma. Int. J. Cancer 42:329-338[Medline].
9.	Freedman, A. S., G. Freeman, J. C. Horowitz, J. Daley, and L. M. Nadler. 1987. B7, a B-cell-restricted antigen that identifies preactivated B cells. J. Immunol. 139:3260-3267[Abstract].
10.	Herbst, H., F. Dallenbach, M. Hummel, G. Niedobitek, S. Pileri, L. N. Muller, and H. Stein. 1991. Epstein-Barr virus latent membrane protein expression in Hodgkin and Reed-Sternberg cells. Proc. Natl. Acad. Sci. USA 88:4766-4770[Abstract/Free Full Text].
11.	Kaplan, M. A., J. A. Ferry, N. L. Harris, and J. O. Jacobson. 1994. Clonal analysis of posttransplant lymphoproliferative disorders, using both episomal Epstein-Barr virus and immunoglobulin genes as markers. Am. J. Clin. Pathol. 101:590-596[Medline].
12.	Khan, G., E. M. Miyashita, B. Yang, G. J. Babcock, and D. A. Thorley-Lawson. 1996. Is EBV persistence in vivo a model for B cell homeostasis? Immunity 5:173-179[CrossRef][Medline].
13.	Khanna, R., S. R. Burrows, and D. J. Moss. 1995. Immune regulation in Epstein-Barr virus-associated diseases. Microbiol. Rev. 59:387-405[Abstract/Free Full Text].
14.	Kieff, E. 1996. Epstein-Barr virus and its replication, p. 2343-2396. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Fields virology, 2nd ed., vol. 2. Raven Press, New York, N.Y.
15.	Klein, G. 1994. Epstein-Barr virus strategy in normal and neoplastic B-cells. Cell 77:791-793[CrossRef][Medline].
15a.	Kurth, J., T. Spieker, J. Wustrow, J. G. Strickler, M. L. Hansmann, K. Rajewsky, and R. Küppers. Tracing EBV-infected B cells in infectious mononucleosis: viral strategies for spreading in the B cell compartment and establishment of latent infection. Immunity, in press.
16.	Liu, Y. J., and C. Arpin. 1997. Germinal center development. Immunol. Rev. 156:111-126[CrossRef][Medline].
17.	MacLennan, I. C. 1994. Germinal centers. Annu. Rev. Immunol. 12:117-139[CrossRef][Medline].
18.	Masucci, M. G., and I. Ernberg. 1994. Epstein-Barr virus: adaptation to a life within the immune system. Trends Microbiol. 2:125-130[CrossRef][Medline].
19.	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].
20.	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[CrossRef][Medline].
21.	Niedobitek, G., E. Kremmer, H. Herbst, L. Whitehead, C. W. Dawson, E. Niedobitek, C. von Ostau, N. Rooney, F. A. Grasser, and L. S. Young. 1997. Immunohistochemical detection of the Epstein-Barr virus-encoded latent membrane protein 2A in Hodgkin's disease and infectious mononucleosis. Blood 90:1664-1672[Abstract/Free Full Text].
22.	Nonkwelo, C., J. Skinner, A. Bell, A. Rickinson, and J. Sample. 1996. Transcription start sites downstream of the Epstein-Barr virus (EBV) Fp promoter in early-passage Burkitt lymphoma cells define a fourth promoter for expression of the EBV EBNA-1 protein. J. Virol. 70:623-627[Abstract].
23.	Oudejans, J. J., D. F. Dukers, N. M. Jiwa, A. J. van den Brule, F. A. Grasser, P. C. de Bruin, A. Horstman, W. Vos, J. van Gorp, J. M. Middeldorp, and C. J. Meijer. 1996. Expression of Epstein-Barr virus encoded nuclear antigen 1 in benign and malignant tissues harbouring EBV. J. Clin. Pathol. 49:897-902[Abstract/Free Full Text].
24.	Pallesen, G., S. J. Hamilton-Dutoit, M. Rowe, and L. S. Young. 1991. Expression of Epstein-Barr virus latent gene products in tumour cells of Hodgkin's disease. Lancet 337:320-322[CrossRef][Medline].
25.	Perry, M., and A. Whyte. 1998. Immunology of the tonsils. Immunol. Today 19:414-421[CrossRef][Medline].
26.	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].
27.	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.), Fields virology, 3rd ed., vol. 2. Raven Press, New York, N.Y.
28.	Rickinson, A. B., Q. Y. Yao, and L. E. Wallace. 1985. The Epstein-Barr virus as a model of virus-host interactions. Br. Med. Bull. 41:75-79[Abstract/Free Full Text].
29.	Robertson, E., and E. Kieff. 1995. Reducing the complexity of the transforming Epstein-Barr virus genome to 64 kilobase pairs. J. Virol. 69:983-993[Abstract].
30.	Schaefer, B. C., J. L. Strominger, and S. H. Speck. 1995. Redefining the Epstein-Barr virus-encoded nuclear antigen EBNA-1 gene promoter and transcription initiation site in group I Burkitt lymphoma cell lines. Proc. Natl. Acad. Sci. USA 92:10565-10569[Abstract/Free Full Text].
31.	Thomas, J. A., N. A. Hotchin, M. J. Allday, P. Amlot, M. Rose, M. Yacoub, and D. H. Crawford. 1990. Immunohistology of Epstein-Barr virus-associated antigens in B cell disorders from immunocompromised individuals. Transplantation 49:944-953[Medline].
32.	Thorley-Lawson, D. A. 1999. EBV $---$ schizophrenic but not dysfunctional. Epstein-Barr Virus Rep. 6:158-163.
33.	Thorley-Lawson, D. A., and G. J. Babcock. 1999. A model for persistent infection with Epstein-Barr virus: the stealth virus of human B cells. Life Sci. 65:1433-1453[CrossRef][Medline].
34.	Thorley-Lawson, D. A., and K. P. Mann. 1985. Early events in Epstein-Barr virus infection provide a model for B cell activation. J. Exp. Med. 162:45-59[Abstract/Free Full Text].
35.	Thorley-Lawson, D. A., and E. M. Miyashita. 1996. Epstein-Barr virus and the B cell: that's all it takes. Trends Microbiol. 4:204-208[CrossRef][Medline].
36.	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].
37.	Tsai, C. N., S. T. Liu, and Y. S. Chang. 1995. Identification of a novel promoter located within the Bam HI Q region of the Epstein-Barr virus genome for the EBNA 1 gene. DNA Cell Biol. 14:767-776[Medline].
38.	Wang, F., S. F. Tsang, M. G. Kurilla, J. I. Cohen, and E. Kieff. 1990. Epstein-Barr virus nuclear antigen 2 transactivates latent membrane protein LMP1. J. Virol. 64:3407-3416[Abstract/Free Full Text].
39.	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].
40.	Young, L., C. Alfieri, K. Hennessy, H. Evans, C. O'Hara, K. C. Anderson, J. Ritz, R. S. Shapiro, A. Rickinson, E. Kieff, et al. 1989. Expression of Epstein-Barr virus transformation-associated genes in tissues of patients with EBV lymphoproliferative disease. N. Engl. J. Med. 321:1080-1085[Abstract].
41.	Young, L. S., C. W. Dawson, D. Clark, H. Rupani, P. Busson, T. Tursz, A. Johnson, and A. B. Rickinson. 1988. Epstein-Barr virus gene expression in nasopharyngeal carcinoma. J. Gen. Virol. 69:1051-1065[Abstract/Free Full Text].
42.	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].