Activation of Lymphocyte Signaling by the R1 Protein of Rhesus Monkey Rhadinovirus

doi:10.1128/JVI.74.6.2721-2730.2000

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Journal of Virology, March 2000, p. 2721-2730, Vol. 74, No. 6
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Activation of Lymphocyte Signaling by the R1 Protein of Rhesus Monkey Rhadinovirus

Blossom Damania, Maryann DeMaria, Jae U. Jung, and Ronald C. Desrosiers^*

New England Regional Primate Research Center, Harvard Medical School, Southborough, Massachusetts 01772-9102

Received 11 November 1999/Accepted 17 December 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Rhesus monkey rhadinovirus (RRV) is a gamma-2 herpesvirus that exhibits a considerable degree of similarity to the human Kaposi'ssarcoma-associated herpesvirus (KSHV). The R1 protein of RRV isdistantly related to the K1 protein of KSHV, and R1, like K1,can contribute to cell growth transformation. In this study weanalyzed the ability of the cytoplasmic tail of R1 to functionas a signal transducer. The cytoplasmic domain of the R1 proteincontains several tyrosine residues whose phosphorylation is inducedin cells expressing Syk kinase. Expression of a CD8 chimera proteincontaining the extracellular and transmembrane domains of CD8fused to the cytoplasmic domain of R1 mobilized intracellularcalcium and induced cellular tyrosine phosphorylation in B cellsupon stimulation with anti-CD8 antibody. None of the CD8-R1 cytoplasmicdeletion mutants tested were able to mobilize intracellular calciumor to induce tyrosine phosphorylation to a significant extentupon addition of anti-CD8 antibody. Expression of wild-type R1protein activated nuclear factor of activated T lymphocytes (NFAT)eightfold in B cells in the absence of antibody stimulation; expressionof the CD8-R1C chimera strongly induced NFAT activity (60-fold)but only upon the addition of anti-CD8 antibody. We conclude thatthe cytoplasmic domain of R1 is capable of transducing signalsthat elicit B-lymphocyte activation events. The signal-inducingproperties of R1 appear to be similar to those of K1 but differin that the required sequences are distributed over a much longerstretch of the cytoplasmic domain (>150 amino acids). In addition,the induction of calcium mobilization was considerably longerin duration and stronger with R1 than withK1.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Src homology-2 (SH2) domains are present in a number of signal-transducing proteins including protein kinases, phosphatases,and phospholipases (6, 23, 24). Sequences that bind toSH2 domains are characterized by phosphorylated tyrosine residuespresent in a variety of cellular signaling proteins such as lymphocytereceptors, adapter proteins, protein kinases, and transcriptionfactors. The sequences containing these phosphorylated tyrosineresidues are referred to as SH2 binding motifs and serve to recruitcellular proteins containing SH2 domains into lymphocyte receptor-mediatedsignaling complexes. SH2 binding motifs consist of a tyrosineresidue followed by three amino acids, YXX(L/I/V), whose sequenceis specific for binding a particular SH2 domain (23, 28).These motifs can occur in either a singular or tandem fashion.Hematopoietic lymphocyte receptors including immunoglobulin- $alpha$ (Ig $alpha$ ), Ig $beta$ , T-cell receptor- $varepsilon$ , IgE- $beta$ , and IgE- $gamma$ contain two suchSH2 binding motifs in tandem, and this motif has been termed theimmunoreceptor tyrosine-based activation motif (ITAM) (3, 4,13, 16, 32, 33). The archetypal ITAM consists of a stretchof negatively charged amino acids preceding the two tyrosine-containingsequences: (D/E)X₇(D/E)X₂YX₂LX_7-10YX₂L/I, where X is anyamino acid. In B cells, T cells, and mast cells, the ITAMs havebeen shown to be critical for interactions with Src family (Src,Lyn, Blk, Lck, and Fyn) and Syk family (Syk and Zap70) kinases(16, 19, 29). The antigen binding site of the B-cell receptor(BCR) is a membrane-bound Ig that is noncovalently attached toa disulfide-linked Ig $alpha$ -Ig $beta$ heterodimer that serves as the majorsignaling component of the BCR complex. In the resting state ofB cells, the Src family of protein tyrosine kinases is associatedwith the Ig $alpha$ subunit of the Ig $alpha$ -Ig $beta$ heterodimer. Binding of antigento the membrane Ig results in a higher affinity of the Src kinasefamily members for the BCR, leading to the phosphorylation ofthe tyrosine residues present in the ITAMs of the Ig $alpha$ and Ig $beta$ subunits. This in turn recruits the Syk family of protein kinasesto the BCR complex in a manner that is SH2 domain dependent. Theimmediate effect is an activated receptor complex that providesbinding sites for signal adapter and transducer proteins thatinitiate a signal cascade leading to proliferation and differentiationof the Bcell.

Kaposi's sarcoma-associated herpesvirus (KSHV), also called Human herpesvirus 8, has been consistently identified in Kaposi'ssarcomas, body cavity-based lymphomas, and some forms of multicentricCastleman's disease (7, 14, 25, 26, 30). Recently anew herpesvirus called Rhesus monkey rhadinovirus (RRV), whichis closely related to but distinct from KSHV, has been isolatedfrom rhesus monkeys (10). RRV is the closest known relativeof KSHV on the basis of sequence similarities and structural organizationof the genomes (1, 27). Similar to KSHV, RRV has been shownto be present predominantly in B lymphocytes (22). At a genomiclocation equivalent to that of the saimiri transforming protein(STP) of herpesvirus saimiri (HVS) and K1 of KSHV, we have identifieda novel open reading frame called the R1 open reading frame atthe left end of the RRV genome (9). The R1 protein is a glycosylatedtransmembrane protein of approximately 70 kDa. Expression of R1in rodent fibroblasts induces transformation, resulting in morphologicalchanges and focus formation (9). Injection of R1-expressingcells into nude mice induced the formation of multifocal, disseminatedtumors (9). A recombinant herpesvirus in which the STP oncogeneof HVS was replaced with the R1 gene was capable of immortalizingT lymphocytes to interleukin-2-independent growth, further indicatingthe transforming potential of the R1 protein (9).

R1, like K1, has features of a receptor protein. While the predicted extracellular domain of R1 of RRV exhibits considerablehomology and is similar in length to the extracellular domainof K1 of KSHV, the cytoplasmic domain of R1 is markedly differentfrom that of K1. The K1 protein has a short cytoplasmic tail containingonly 38 amino acids (20). This short cytoplasmic tail has beenshown to contain an ITAM that is capable of eliciting cellularsignal transduction, evidenced by the induction of cellular tyrosinephosphorylation and calcium mobilization in B cells (17, 19).In contrast, the R1 protein has a 171-amino-acid cytoplasmic tail.Unlike K1, which contains 2 tyrosine residues in a single ITAMsequence in its cytoplasmic tail, R1 contains a total of 13 tyrosineresidues in its cytoplasmic domain. Five of these 13 tyrosinesare present in contiguous YXXL ITAM-like sequences and are localizedto a defined stretch proximal to the carboxylterminus.

To investigate the potential signal-transducing activity of the cytoplasmic region of R1, we constructed a chimeric proteinin which the cytoplasmic tail of the human CD8 $alpha$ polypeptide wasreplaced with that of R1. We demonstrate that expression of thischimera in B cells induced cellular tyrosine phosphorylation,intracellular calcium mobilization, and nuclear factor of activatedT lymphocytes (NFAT) activity upon stimulation with an anti-CD8antibody. Our results demonstrate that the cytoplasmic domainof the RRV transforming protein R1 is an efficient transducerof signals to elicit lymphocyte activationevents.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmids. The pFJ-R1 expression plasmid has been described previously (9). For the CD8-R1 chimera proteins, the coding sequencesfor the cytoplasmic deletion mutants of R1 were cloned in-framewith those for the CD8 extracellular and transmembrane domainsinto the EcoRI-XbaI site of the pcDNA3-CD8 $Delta$ vector, which containedthe coding sequences for the CD8 extracellular and transmembranedomains inserted in the BglII and EcoRI sites. The R1 cytoplasmicdeletions were obtained by PCR using EcoRI and XbaI containingprimers. To facilitate detection, the CD8-R1 chimeras were taggedwith the AU1 epitope (BAbCO) at the C-terminal end. PFJ-K1 hasbeen described previously (19). The NFAT-luciferase constructwas obtained from Don Ganem. The Syk expression plasmid was providedby A. Veillette, and the Src expression plasmid was provided byT. M.Roberts.

Cell culture and transfection. Cos-1 cells and Rat-1 fibroblasts were grown in Dulbecco modified Eagle medium supplemented with 10% fetal calf serum (FCS).Calcium phosphate was used for transient transfection of Cos-1cells. For Rat-1 fibroblasts stably expressing the R1 constructs,cells were transfected using Lipofectamine (Gibco-BRL) and stabletransfectants were selected using 2 mg of geneticin per ml. BJABcells were cultured in RPMI media containing 10% FCS. Ten microgramsof each CD8-R1 chimera plasmid was electroporated into BJAB cellsat 200 V and 960 µF in Optimem (Gibco-BRL) media. Forty-eighthours postelectroporation, cells were pelleted and transferredinto RPMI media supplemented with geneticin (2 mg per ml) andcultured for 5 weeks. Cells were sorted by fluorescence-activatedcell sorting(FACS).

FACS analysis. For FACS, 2 × 10⁷ B cells expressing chimera proteins were washed with Optimem and stained with phycoerythrin-conjugated CD8antibody (Pharmingen) for 30 min at 4°C. Excess antibody was washedaway, and cells were sorted based on CD8 expression using a FACSVantage(Becton Dickinson). After being sorted, cells were washed andcultured in complete RPMImedia.

Calcium mobilization assay. Cells (10⁶) were resuspended in 2 ml of complete RPMI medium and incubated with 1 µM indo-1 for 20 min at 37°C. The cells weresubsequently placed on ice till ready to be used. Five minutesprior to use, cells were warmed at 37°C and baseline calcium levelswere read for 1 min. Cells were then stimulated with 10 µg ofanti-CD8 antibody, OKT8 (American Type Culture Collection), oranti-human IgM antibody (Upstate Biotechnology), and data werecollected for 4 min for the IgM stimulation and 8 min for theOKT8 stimulation. A FACSVantage (Becton Dickinson) was used fordata collection andanalysis.

Antibody stimulation. Cells (10⁶) were stimulated with 10 µg of OKT8 antibody or anti-human IgM antibody, after which cells were flash frozen inliquid nitrogen and subsequently thawed and lysed in cold lysisbuffer containing 1 mM Na₂VO₃ and protease inhibitors. Cell lysateswere used for immunoprecipitation and Westernanalysis.

Immunoprecipitation and immunoblotting. After transfection and antibody stimulation, cells were harvested and lysed in NP-40 lysis buffer (0.15 M NaCl, 50 mM Tris[pH 8], 1% NP-40) containing 1 mM Na₂VO₃, and protease inhibitors.Cellular debris was pelleted at 10,000 rpm for 10 min, and thesupernatants were used for immunoprecipitation with the appropriateantibody and protein A/G-Sepharose beads (Santa Cruz Biotechnology).Immune complexes were pelleted and washed at least five timeswith lysis buffer. Complexes were resolved by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) and transferred to nitrocellulose.Immunoblot detection was performed using the enhanced chemiluminescenceECL kit(Amersham).

For immunoprecipitations and immunoblotting, anti-AU1 antibody was obtained from BAbCO. Anti-Src and anti-Syk antibodies wereobtained from Upstate Biotechnology. Anti-pTyr (4G10) primaryantibody and horseradish peroxidase-conjugated antiphosphotyrosine(anti-pTyr) antibody was obtained from UpstateBiotechnology.

In vitro kinase assay. Coimmunoprecipitations were performed as described above. After being washed, the complexes were incubated with 5 µCi of [ $gamma$ -³²P]ATP in kinase buffer (50 mM Tris, 10 mM MgCl₂, 10 mM CaCl₂)for 30 min at room temperature. At the end of the incubation,complexes were subjected to SDS-PAGE, and the gel was subsequentlyexposed to X-rayfilm.

Luciferase assays. Luciferase assays were performed by a method similar to the previously described protocol with a few modifications (18).BJAB cells (10⁶) were electroporated with 20 µg of NFAT luciferase plasmid, 40µg of pFJ-R1 or pFJ-K1 plasmids, and 5 µg of $beta$ -galactosidase expressionplasmid. Cells were harvested 24 h posttransfection, and luciferaseassays were performed using the luciferase assay kit from Promega.For the experiments involving antibody stimulation, BJAB cellswere electroporated with the indicated plasmids and 24 h postelectroporationcells were pelleted and washed in serum-free media. Cells wereincubated with anti-CD8 antibody for 5 min at 37°C and subsequentlyresuspended in 10 ml of medium and placed in the incubator. Aliquotsof cells were removed at various time points, and luciferase assayswere performed as describedabove.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

R1 contains multiple YXXL motifs in its cytoplasmic domain. The cytoplasmic domain of R1 contains several potential SH2 binding motifs (Fig. 1). Analysis of the tyrosine residues andtheir surrounding sequences revealed similarities to sequencesthat are capable of binding the SH2 domains of signal transducerproteins. YXXA, YXXP, YXXT, and YXXV motifs have been shown tobind SH2 domains within proteins such as the Src family of kinases,Shc, Abl, Nck, and phosphatidylinositol 3-kinase (6, 29).Five of the 13 tyrosines in the cytoplasmic domain of R1 havesuch a sequence (Fig. 1). The five C-terminal tyrosines in R1are present within YXXL sequences. Similar YXXL sequence elementshave been previously shown to be important for the binding ofB-cell-specific Syk kinase (16, 19, 29). The third and fourthand fourth and fifth YXXL motifs resemble ITAMs in that they andthe surrounding sequences are spaced in a fashion consistent withthat of the ITAM consensus sequence, (D/E)X₇(D/E)X₂YX₂LX_7-10YX₂L/I(Fig. 1).

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FIG. 1. Amino acid sequences of the R1 cytoplasmic tail. The 170 amino acids of the C-terminal cytoplasmic domain of R1 are shown. The cytoplasmic domain of R1 contains several potential SH2 binding motifs (boldface). Dotted underlining, SH2 binding motifs YXXA, YXXV, YXXT, and YXXP; solid underlining, last five YXXL motifs. The third and fourth and fourth and fifth YXXL motifs resemble ITAMs in that they and the surrounding sequences are spaced in a fashion consistent with the consensus sequence, (D/E)X₇(D/E)X₂YX₂LX_7-10YX₂L/I. These motifs are boxed.

Construction of CD8 $Delta$ -R1 chimeras. The full-length R1 cytoplasmic domain (R1C) and deletion mutants derived from it were fused to the extracellular and transmembranedomains of CD8 in order to analyze the contributions of the varioustyrosine-containing elements to B-cell signaling. Six CD8 $Delta$ -R1chimera constructs were made (Fig. 2). The cytoplasmic deletionmutations were selected based on the types of SH2 binding motifspresent in the R1 cytoplasmic domain. The last five tyrosine residuesin R1 are all present in YXXL motifs, and some or all could potentiallyfunction as ITAMs. Hence, this region was separated from the remainingportion which contains a more diverse set of tyrosine-containingmotifs. CD8 $Delta$ -R1C represents the full-length R1 cytoplasmic tailextending from amino acids 253 to 423 fused to the CD8 extracellulardomain and transmembrane region. CD8 $Delta$ -D1 contains the first 121amino acids of the R1 cytoplasmic tail which includes 7 tyrosineresidues, 2 of which are in YXXP sequences, 1 of which is in aYXXA sequence, and another of which is in a YXXT sequence. Suchsequences have been previously shown to function as SH2 bindingmotifs and protein tyrosine kinase docking sites in T-cell receptors,BCRs, Epstein-Barr virus (EBV) LMP2A, and KSHV K1 (2, 3,5, 8, 16, 18, 20, 23, 32, 33). The CD8 $Delta$ -D4 constructhas a stretch of 106 amino acids extending from the first tyrosineresidue (amino acid 265) in the R1 cytoplasmic tail to amino acid373, which is the amino acid preceding the start of the putativeITAMs in the R1 cytoplasmic domain. Hence, CD8 $Delta$ -D4 differs fromCD8 $Delta$ -D1 in that it is missing amino acids 253 to 264, a regionthat is immediately adjacent to the R1 transmembrane domain. CD8 $Delta$ -D2contains a short stretch of 13 amino acids in the R1 cytoplasmictail and is devoid of any tyrosine residues. CD8 $Delta$ -D3 containsthe five YXXL motifs present at the C-terminal end of R1. CD8 $Delta$ -D5contains the same stretch of amino acids as CD8 $Delta$ -D2 in additionto the residues extending from amino acid 345 to amino acid 423.All chimera proteins, including CD8 $Delta$ -R1C, were tagged with theAU1 epitope at the C-terminal end.

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FIG. 2. Construction of CD8-R1 chimeras. The cytoplasmic domain (Cyt) of R1 was fused to the extracellular (Ext) and transmembrane (T.M.) domains of CD8. The CD8 chimera containing the full-length cytoplasmic domain of R1 (CD8 $Delta$ -R1C) and cytoplasmic domains with various deletions (CD8 $Delta$ -D1, CD8 $Delta$ -D2, CD8 $Delta$ -D3, CD8 $Delta$ -D4, CD8 $Delta$ -D5) are depicted. YXXX, tyrosine residues and their surrounding sequences.

In order to construct stable cell lines expressing the six CD8 $Delta$ -R1 chimera proteins, BJAB (EBV KSHV) cells were electroporated with plasmids encoding the individualchimeras. pCDNA3 constructs containing CD8 $Delta$ , CD8 $Delta$ -R1C, CD8 $Delta$ -D1,CD8 $Delta$ -D2, CD8 $Delta$ -D3, CD8 $Delta$ -D4 and CD8 $Delta$ -D5 coding sequences were electroporatedinto BJAB cells, and neomycin-resistant cells were selected for6 weeks. To further enrich for CD8 chimera-expressing cell lines,an anti-CD8 antibody was used to sort these cell lines by flowcytometry to obtain a population of cells, greater than 95% ofwhich expressed the CD8 $Delta$ -R1 chimeric proteins. The CD8 $Delta$ -R1C cellline was sequentially sorted four times in order to obtain a >95%pure population of cells (data notshown).

The cytoplasmic tail of R1 can elicit a calcium response in B cells. Many B- and T-lymphocyte receptors, when activated by extracellular stimulation, are capable of transducing signals that causethe release of calcium from intracellular stores. Since R1 hasseveral SH2 binding motifs, we tested the ability of the CD8 $Delta$ -R1chimeras to induce intracellular calcium mobilization in B cells.BJAB cells expressing the chimeric proteins were individuallystimulated with either anti-IgM antibody or anti-CD8 antibody,and levels of free intracellular calcium were monitored by flowcytometry (Fig. 3A). All seven cell lines, CD8 $Delta$ , CD8 $Delta$ -R1C, CD8 $Delta$ -D1,CD8 $Delta$ -D2, CD8 $Delta$ -D3, CD8 $Delta$ -D4, and CD8 $Delta$ -D5 cells, were capable ofinducing calcium when stimulated with an anti-IgM antibody, suggestingthat these cells were similarly capable of eliciting intracellularcalcium mobilization through the B-cell antigen receptor (Fig.3A). In order to test whether the cytoplasmic domain of R1 andthe various deletion mutants could elicit calcium mobilization,we stimulated the BJAB cell lines expressing CD8-R1 chimeras withan anti-CD8 antibody. The CD8 $Delta$ , CD8 $Delta$ -D1, CD8 $Delta$ -D2, CD8 $Delta$ -D3, andCD8 $Delta$ -D4 cell lines exhibited little or no calcium mobilizationupon stimulation with an anti-CD8 antibody as monitored by flowcytometry (Fig. 3A). However, BJAB cells expressing the CD8 $Delta$ -R1Cchimera did mobilize intracellular calcium, and there was a prolongedperiod of calcium release from intracellular stores that lastedmore than 5 min (Fig. 3A). This is in sharp contrast to the calciumresponse seen with the anti-IgM antibody, which peaked rapidlyand returned to the basal level within a short period of time(Fig. 3A). The calcium response of a CD8 $Delta$ -K1_cytoplasmic BJAB cellline (20) was also tested using the anti-CD8 antibody (Fig.3A), and the response was found to be similar in nature to thatinduced by anti-IgM antibody. The prolonged release of calciumobserved in the CD8 $Delta$ -R1C cell line in response to anti-CD8 antibodysuggests that the full-length cytoplasmic tail of R1 can transducesignals to elicit calcium mobilization. None of the other CD8 $Delta$ -R1deletion mutants could mobilize calcium to a significant extent,including CD8 $Delta$ -D3 and CD8 $Delta$ -D5, which contain the putative ITAM-likesequences. However, all of the tyrosine-containing chimeras didshow a very small increase in intracellular calcium levels, whichwere only slightly above baseline (Fig. 3A). In order to determinethe levels of CD8 $Delta$ and CD8 $Delta$ -R1 chimeric tagged proteins expressedin the B-cell lines, protein extracts from B cells were separatedby SDS-PAGE and Western blotting was performed using an anti-AU1antibody. The data in Fig. 3B indicate that equivalent levelsof CD8 $Delta$ and CD8 $Delta$ -R1 chimera proteins were expressed in the stablecell lines. In addition, the failure of the deletion mutants tosignal could not be explained by differences in the levels ofsurface expression of these proteins as measured by flow cytometry(data not shown).

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FIG. 3. Mobilization of intracellular free calcium upon antibody stimulation. (A) Intracellular calcium release from the chimera cell lines was monitored by flow cytometry. Either an anti-IgM antibody (left) or an anti-CD8 antibody (right) was used to stimulate cells. Data are presented as histograms of the numbers of cells expressing blue fluorescence (y axis) versus time. The intensities of the responses are depicted as different shades of gray, with the darkest shade representing the highest levels of free calcium in the cell. (B) Western blot analysis of CD8-R1 chimera cell extracts using an anti-AU1 antibody to detect expression levels of the AU1-tagged chimera proteins.

R1 induces NFAT activity in B cells. The release of calcium from intracellular stores induces further signaling events that eventually result in the activationof transcription factors in the nucleus. Recently Lagunoff etal. (18) demonstrated that the cytoplasmic domain of the K1protein, specifically the ITAM, is responsible for the activationof NFAT in BJAB (EBV) and Raji (EBV⁺) cells. NFAT is a transcription factor that is present in bothT and B lymphocytes (31). We tested the ability of R1 to activateNFAT in BJAB cells using an NFAT-luciferase reporter construct(18). BJAB cells were electroporated with the NFAT-luciferasereporter construct along with pFJ vector alone, pFJ-R1, or pFJ-K1(Fig. 4A), and cells were harvested 24 h posttransfection. A $beta$ -galactosidaseexpression plasmid was also included as a control for transfectionefficiency. Figure 4A graphs the result of these experiments.We observed that R1 could activate NFAT eightfold with respectto the vector control and that K1 could activate NFAT sevenfold.

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FIG. 4. Activation of NFAT activity in BJAB cells by the R1 protein. (A) BJAB cells were transfected with an NFAT luciferase and $beta$ -galactosidase reporter plasmid along with either a pFJ vector control plasmid, a pFJ-R1-expressing plasmid, or a pFJ-K1-expressing plasmid. At 48 h posttransfection cells were harvested and tested for luciferase activity. Luciferase counts for each sample were normalized with respect to $beta$ -galactosidase activity. Luciferase assays were repeated three times, and the average of these values was graphed as the fold activation of NFAT by the R1 and K1 proteins versus that of control vector alone. (B) Transfections similar to those in panel A except that the CD8 $Delta$ -R1 chimera-expressing plasmids indicated in the graph were electroporated into BJAB cells. (C) BJAB cells were transfected with NFAT luciferase and $beta$ -galactosidase reporter plasmids along with a CD8 $Delta$ -R1C-expressing plasmid. At 24 h posttransfection cells were harvested and incubated with anti-CD8 antibody for 12, 24, 36, and 48 h. Ab, antibody.

We subsequently tested the ability of the CD8 $Delta$ -R1 chimeras to induce NFAT activity in BJAB cells. We performed an experimentsimilar to that described above except that this time each CD8 $Delta$ -R1chimera construct was electroporated into the B cells in lieuof the pFJ-R1 plasmid. Figure 4B demonstrates that none of theCD8 $Delta$ -R1 chimeras were able to induce a significant level of NFATactivity in these cells, including the CD8 $Delta$ -R1C chimera. We conductedan additional experiment in which each CD8 $Delta$ -R1 chimera plasmidwas electroporated into BJAB cells and 24 h posttransfection thesecells were incubated with an anti-CD8 antibody for different periodsof time (for 12, 24, 36, and 48 h following addition of anti-CD8antibody). The results are graphed in Fig. 4C. We observed thatthe CD8 $Delta$ -R1C chimera, upon stimulation with anti-CD8 antibody,could strongly induce NFAT activity in B cells. The effect ofthis activation peaked 24 h after the addition of the anti-CD8antibody, inducing a 60-fold increase in the level of NFAT activitycompared to that induced by the CD8 $Delta$ chimera alone. Similar experimentsconducted with the other CD8 $Delta$ -R1 deletion mutants showed themincapable of inducing NFAT activity even when incubated with theanti-CD8 antibody (data not shown). These results demonstratethat the CD8 $Delta$ -R1C chimera requires antibody stimulation to induceNFATactivity.

The cytoplasmic tail of R1 induces cellular phosphorylation. Calcium mobilization and NFAT activation are indicators of lymphocyte activation. The ability of the cytoplasmic tail of R1to induce calcium mobilization prompted us to determine whetherthis event involved cellular tyrosine phosphorylation as is thecase with BCRactivation.

We stimulated the CD8 $Delta$ -R1C-expressing cell line with an anti-IgM or an anti-CD8 antibody and performed Western blot analysiswith cellular extract using an anti-pTyr antibody. As shown inFig. 5A, both the anti-IgM and anti-CD8 antibodies were capableof inducing tyrosine phosphorylation in the B-cell line comparedto unstimulated cells. Cross-linking with the anti-CD8 antibodyinduced the phosphorylation of an additional 48-kDa protein, whosemolecular mass correlates with that of the CD8 $Delta$ -R1C protein (Fig.5A).

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FIG. 5. Induction of cellular tyrosine phosphorylation upon antibody stimulation. (A) Comparison of anti-IgM- and anti-CD8-stimulated CD8 $Delta$ -R1C cells. Cross-linking of the CD8 $Delta$ -R1C cell line with an anti-IgM or anti-CD8 (OKT8) antibody (Ab) induced tyrosine phosphorylation of cellular proteins as determined by Western analysis using an anti-pTyr antibody. Asterisk, 50-kDa phosphorylated protein seen in the CD8 antibody-stimulated, but not IgM antibody-stimulated, B cells. (B) Mutational analysis of CD8 $Delta$ -R1 chimeras for the induction of tyrosine phosphorylation upon antibody stimulation. Cells were incubated in the absence ( $-$ ) or presence (+) of anti-CD8 antibody for 1 min at 37°C and immediately lysed. Cell extracts were subjected to gel electrophoresis, transferred to nitrocellulose, and reacted with an anti-pTyr antibody (top). Cell extracts were probed with an anti-AU1 antibody (bottom) to show comparative levels of chimeric proteins in these cells. Asterisks, heavy and light chains of the CD8 antibody used for stimulation. I.B., immunoblotting.

We next tested the abilities of the different R1 cytoplasmic deletion mutants to induce cellular tyrosine phosphorylation(Fig. 5B, top). In contrast to what was seen for cells expressingCD8 $Delta$ -R1C, which showed a marked degree of cellular tyrosine phosphorylationupon stimulation with the anti-CD8 antibody, a very slight increasein tyrosine phosphorylation was seen with the CD8 $Delta$ -D1 and CD8 $Delta$ -D4deletion mutants (Fig. 5B, top). In order to control for the levelof CD8 $Delta$ -R1 chimera expression, we reacted extracts from stimulatedand unstimulated cells with an anti-AU1 antibody and observedthat similar levels of chimeric proteins were expressed in thesecells (Fig. 5B, bottom). These results indicate that an intactcytoplasmic tail of the R1 protein is required not only for thecalcium mobilization described above but also for the inductionof tyrosine phosphorylation in cells, although the deletion mutantsmay exhibit partialfunction.

The wild-type CD8 $Delta$ -R1C cell line showed the presence of an ~70 kDa protein whose phosphorylation was increased upon antibodystimulation. The molecular mass of this protein corresponds withthat of Syk kinase. In order to determine whether the hyperphosphorylatedband represented phosphorylated Syk kinase, we performed immunoprecipitationsusing an anti-Syk antibody with the same extracts from anti-CD8-stimulatedand unstimulated cells. The immunoprecipitated complexes weresubjected to Western blot analysis using anti-pTyr antibody. Extractsfrom stimulated CD8 $Delta$ -R1C cells showed the presence of Syk kinaseas a 70-kDa protein which was phosphorylated to a greater extentthan Syk in unstimulated CD8 $Delta$ -R1C cells (Fig. 6). In addition,the stimulated CD8 $Delta$ -R1C cells showed a phosphorylated proteinof ~50 kDa coimmunoprecipitating with Syk kinase. This proteincorresponds in size to the CD8 $Delta$ -R1C chimera protein itself, suggestingthat the phosphorylated full-length R1 cytoplasmic domain is complexedwith phosphorylated Syk kinase when activated. The CD8 $Delta$ -D3 andCD8 $Delta$ -D4 immunoprecipitation complexes (Fig. 6) revealed a slightincrease in the levels of phosphorylated Syk kinase compared tothat of unstimulated cells.

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FIG. 6. Tyrosine phosphorylation of Syk kinase and CD8 chimeras. Shown is the induction of tyrosine phosphorylation by Syk kinase. The CD8-R1 chimera cell lines were incubated with (+) or without ( $-$ ) anti-CD8 antibody. Extracts were subjected to immunoprecipitation (I.P.) with an anti-Syk antibody (Ab), and immune complexes were resolved by gel electrophoresis and subjected to a Western blot analysis using an anti-pTyr antibody.

Syk kinase can induce phosphorylation of R1. The above results indicated that the cytoplasmic domain of R1 is phosphorylated and raised the possibility that R1 may potentiallybe phosphorylated by a B-cell kinase. Since Syk is a major B-cellkinase, we conducted additional experiments to determine whetherSyk kinase can induce phosphorylation of the R1 protein. Cos-1cells were cotransfected with a Syk expression plasmid in thepresence or absence of a vector expressing a C-terminal, AU1 epitope-taggedR1 protein (Fig. 7). Forty-eight hours after transfection, lysatesfrom transfected cells were reacted with anti-AU1 antibody andimmune complexes were analyzed by SDS-PAGE, transferred to nitrocellulose,and reacted with a pTyr antibody. Tyrosine phosphorylation ofa 70-kDa protein was detected only in cells transfected with Sykand R1 expression plasmids (Fig. 7A). Since both Syk and R1 havean apparent molecular mass of 70 kDa, it is possible that bothof these proteins were represented in the 70-kDa phosphorylatedband. We also performed coimmunoprecipitations using an anti-pTyrantibody and a Western analysis with an anti-AU1 antibody to detectthe presence of phosphorylated R1 protein. We observed that theR1 protein was tyrosine phosphorylated when Cos-1 cells were cotransfectedwith Syk expression and R1 expression plasmids (Fig. 7B).

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FIG. 7. Syk kinase induces the phosphorylation of full-length R1. (A) Cotransfection of R1 and Syk expression plasmids in Cos-1 cells. A full-length, C-terminal AU1 epitope-tagged R1-expressing plasmid was transfected into Cos-1 cells either alone or in the presence of Syk kinase. Cells were harvested 48 h posttransfection, and extracts were subjected to immunoprecipitation (I.P.) with an anti-AU1 antibody followed by a Western blot analysis (I.B.) using an anti-pTyr antibody. (B) The same extracts were coimmunoprecipitated with an anti-pTyr antibody followed by Western blotting with an anti-AU1 antibody.

An in vitro kinase assay was performed using extracts from cells cotransfected with an R1 expression plasmid in the absenceor presence of Syk kinase- or Src kinase-expressing plasmids (Fig.8A). Anti-AU1 immune complexes from these cells were washed extensivelyand incubated with [ $gamma$ -³²P]ATP. The in vitro kinase assay showed that a 70-kDa phosphorylatedprotein was specifically immunoprecipitated with the AU1 antibody(Fig. 8A). In order to confirm that R1 was indeed phosphorylatedin Syk kinase-expressing cells, we cotransfected Cos-1 cells witha Syk kinase expression vector and individual CD8 $Delta$ -R1 chimeraexpression plasmids. Figure 8B shows that Syk kinase induced phosphorylationof the CD8 $Delta$ -R1C protein as well as of the three other tyrosine-containingmutants, CD8 $Delta$ -D1, CD8 $Delta$ -D3, and CD8 $Delta$ -D4. Syk kinase could not inducephosphorylation of the CD8 $Delta$ -D2 mutant, which does not containany tyrosine residues. These results show that the cytoplasmicdomain of the R1 protein contains several phosphorylation siteswhose phosphorylation is induced in cells expressing Syk kinase.

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FIG. 8. Syk-induced phosphorylation of R1 and CD8 $Delta$ -R1 chimeras. (A) Phosphorylation of R1 in vitro. An in vitro kinase assay was performed using extracts from Cos-1 cells transfected with R1 alone or in combination with Syk and Src kinase. Immune complexes were washed extensively and subsequently incubated with [ $gamma$ -³²P]ATP. Complexes were then separated by gel electrophoresis and exposed to autoradiography. Arrow, presence of a 70 kDa phosphorylated protein that corresponds to the molecular sizes of both Syk and R1. (B) Tyrosine phosphorylation of CD8 $Delta$ -R1 chimeras induced by Syk kinase. Cos-1 cells were cotransfected with a Syk expression plasmid along with the CD8 $Delta$ -R1 chimera-expressing plasmids. The chimeras were tagged with an anti-AU1 antibody. Immunoprecipitations (I.P.) were performed using an anti-AU1 antibody and an anti-pTyr antibody was used for a Western blot analysis (I.B.). Dots, positions of mutant proteins.

Syk kinase can interact with R1. To investigate whether the interaction between Syk and R1 is sufficiently stable to be detected by coimmunoprecipitation,Cos-1 cells were transfected with vectors expressing Src kinaseor Syk kinase together with the AU1-tagged R1 gene, and immunoprecipitationswere performed using an anti-Src or anti-Syk antibody. Immunecomplexes were resolved by SDS-PAGE, transferred to nitrocellulose,and reacted with the anti-AU1 epitope antibody. As shown in Fig.9, R1 was specifically coimmunoprecipitated with Syk kinase butnot with Src kinase. The lower panel indicates that there wasequal expression of Syk kinase and Src kinase in these cells.Thus, these data indicate that Syk kinase can interact with andinduce phosphorylation of R1.

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FIG. 9. R1 can specifically interact with Syk kinase. Coimmunoprecipitations (I.P.) were performed using an anti-Src or anti-Syk kinase antibody on cells transfected with an AU1-tagged R1-expressing plasmid alone or together with Src or Syk kinase-expressing plasmids. Immune complexes were subjected to gel electrophoresis. The gel was transferred to nitrocellulose and subsequently probed with an anti-AU1 antibody. Bottom, levels of Syk and Src kinase in transfected cells. I.B., immunoblotting.

We compared the abilities of both Syk and Src kinases to phosphorylate RRV R1 and KSHV K1 proteins. Cos-1 cells were cotransfectedwith plasmids expressing R1 or K1 in the presence or absence ofSrc kinase or Syk kinase expression plasmids (Fig. 10). The toppanel represents an immunoblot of the corresponding cell extractsreacted with an anti-pTyr antibody and shows that Syk kinase canphosphorylate R1 to a greater extent than K1, whereas the levelsof R1 and K1 phosphorylation induced by Src kinase are similar.The bottom panel represents the same reaction mixtures probedwith an AU1 antibody and demonstrates that equivalent levels ofK1 and R1 were expressed in these cells.

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FIG. 10. Tyrosine phosphorylation of the R1 and K1 proteins. Comparison of the phosphorylation of R1 and K1 proteins by Src and Syk kinase. Both R1- and K1-expressing plasmids were transfected into Cos-1 cells in the absence or presence of Src and Syk kinases. The immunoblot (I.B.) was reacted with a pTyr antibody (Top). Arrows, R1 and K1 proteins. (Bottom) Western blot analysis of cell extracts used for the immunoprecipitations in the upper panel. The extracts were probed with an AU1 antibody to detect expression levels of R1 and K1 proteins expressed in transfected cells.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The R1 open reading frame, the first open reading frame of RRV, encodes a transmembrane protein predicted to contain an extracellularamino-terminal domain and a cytoplasmic carboxy-terminal domain.The extracellular domain of R1 is similar in length and sequenceto that of KSHV K1 and shows homology to the Ig receptor superfamily.These properties suggest that R1, like other receptor proteins,may be capable of binding a stimulating ligand, which can resultin the transduction of signals inside thecell.

Our results demonstrate that upon cross-linking with an anti-CD8 antibody, B cells expressing a CD8 $Delta$ -R1C chimera protein containingthe full-length cytoplasmic domain of R1 become fully activated,as indicated by the release of free calcium from intracellularstores. This event differs from that induced by BCR cross-linkingby an anti-IgM antibody in that the release of free calcium isprolonged, lasting significantly longer than the BCR-induced response.Importantly, none of the R1 deletion mutants could elicit calciummobilization to a significant degree. Mutants CD8 $Delta$ -D1 and CD8 $Delta$ -D4,which contain putative SH2 binding domains, as well as CD8 $Delta$ -D3,which contains putative ITAM-like sequences, showed only a marginalincrease in calcium mobilization, suggesting that the releaseof calcium from intracellular stores is dependent on the full-lengthcytoplasmic tail. The fact that the CD8 $Delta$ -D3 mutant could not significantlymobilize calcium was surprising since it contains sequences thatmatch well with the ITAM consensus. One possibility that we consideredwas that the CD8 $Delta$ -D3 mutant requires a linker sequence betweenthe CD8 extracellular and transmembrane domains and the carboxy-terminalSH2 binding motifs in R1 in order to induce calcium mobilization.However, CD8 $Delta$ -D5, which contains such a linker sequence, was alsoincapable of eliciting a significant calcium response. Thus thesedata are supportive of the need for the full-length R1 cytoplasmicdomain for calcium mobilization. The differences in the lengthsof the R1 versus K1 cytoplasmic domains required to achieve calciummobilization could possibly result from additional functions forR1 that remain to be determined or could reflect the fact thatthe K1 protein is more highly evolved. It seems likely that theamino acids that are required for calcium mobilization residein two or more distinct domains in the R1 cytoplasmic tail andthat proper folding of the cytoplasmic tail is needed to bringtogether disparate parts of themolecule.

In agreement with our calcium mobilization data, we have also observed that the R1 protein is capable of inducing NFAT activityeightfold in B lymphocytes. Both these events are indicative ofB-cell activation. We determined that none of the CD8 $Delta$ -R1 chimeraproteins could activate NFAT activity to a significant level inB cells by themselves, but upon addition of anti-CD8 antibodywe observed a dramatic increase in the activation of NFAT by theCD8 $Delta$ -R1C chimera protein. This is suggestive of a role for theextracellular and transmembrane regions of the R1 protein forlymphocyte activation, in addition to that for a full-length cytoplasmictail. The extracellular domain of the R1 protein may be bindinga ligand present at least to some extent in the media or on thesurfaces of B cells. Another possibility is that the extracellularand transmembrane domains of R1 may undergo self-oligomerizationleading to the phosphorylation of the R1 cytoplasmic domain followedby B-cell activationevents.

In agreement with the calcium mobilization assays, we observed that only the chimera with the full-length R1 cytoplasmic domain(CD8 $Delta$ -R1C) could induce a state of cellular phosphorylation inB cells. Cross-linking of the CD8 $Delta$ -R1C chimeric protein by ananti-CD8 antibody induced a pattern of tyrosine phosphorylationsimilar to that seen withBCR.

We detected complex formation between R1 and the major B-cell kinase, Syk. Although both Src and Syk kinase were capable ofphosphorylating R1, only Syk kinase specifically interacted detectablywith R1. The ability of Src kinase to phosphorylate R1 may beindirect. Syk induced the phosphorylation of the CD8 $Delta$ -R1C chimera.Syk also induced the phosphorylation of the deletion mutants CD8 $Delta$ -D1,CD8 $Delta$ -D3, and CD8 $Delta$ -D4, and these same mutants showed marginal responsesin the calcium mobilization assay. Taken together, these datasuggest that these mutants may exhibit partial function to a slightextent. In addition, stimulation of the CD8 $Delta$ -R1C cell line withan anti-CD8 antibody resulted in increased phosphorylation ofSyk kinase indicative of the need for a full-length R1 cytoplasmicprotein to elicit tyrosine phosphorylation in Bcells.

The cytoplasmic tail of R1 is 170 amino acids in length and contains 13 tyrosine residues, 5 of which are part of YXXL motifsat the carboxyl-terminal end of the protein and match consensussequences for ITAMs. Five of the other eight tyrosine residuescould also potentially function as SH2 binding motifs since theassociated sequences, YXXA, YXXP, YXXT, and YXXV, match sequencespreviously shown to bind SH2 domains. YXXA can bind Src, Lyn,Fyn, Shc, phosphatidylinositol 3 kinase, and phospholipase C $gamma$ (28, 29). YXXP has been shown to interact with Abl, Crk, andNck SH2 binding domains (29). Thus the R1 protein has rich potentialfor interacting with a number of different signal-transducingmolecules. Nonetheless, our data have shown that one contiguousstretch containing seven tyrosines and a separate overlappingstretch containing seven different contiguous tyrosines are insufficientfor a significant mobilization of calcium, induction of tyrosinephosphorylation, and NFATactivity.

Both RRV R1 and KSHV K1 have been shown to transform rodent fibroblasts, to substitute for STP in HVS-induced immortalizationof T cells to interleukin-2-independent growth, and to inducecellular phosphorylation and signal transduction (20, 21).Although these proteins have sequence and structural homologyin their external domains, the length of the R1 cytoplasmic domainand the number of potential SH2 binding motifs contained in thisdomain differ markedly from those of K1, which has a short 38-amino-acidcytoplasmic tail and only two SH2 binding motifs, which constitutea single ITAM (18, 20). One striking difference in the activitiesof these proteins is the sustained calcium mobilization inducedin B cells by R1 versus K1. This prolonged activation event maybe a result of the phosphorylation of multiple tyrosine residuesin the R1 cytoplasmic tail as these residues are part of SH2 bindingmotifs that could possibly interact with a variety of cellularkinases.

Cellular receptors, upon ligand stimulation, are capable of undergoing oligomerization and of inducing cellular proliferation.LMP1 protein of EBV mimics an activated CD40 receptor by undergoingmultimerization of its transmembrane domains in a ligand-independentmanner, which results in the activation of the NF- $kappa$ B pathway leadingto cellular proliferation (11, 12, 15, 24). It remainsto be determined whether signal induction via R1 and K1 resultsfrom stimulation by an exogenous ligand or self-multimerization.If there is no self-multimerization, a ligand appears to be present,at least to some extent, on the surfaces of BJAB cells, in theculture supernatant, or in the serum. Regardless of the mechanism,both R1 and K1 appear to be able to activate B cells independentof the traditional BCRengagement.

	ACKNOWLEDGMENTS

We thank Don Ganem and Mike Lagunoff for the NFAT-luciferaseplasmid.

This work was supported by U.S. Public Health Service grants RR00168, CA82057, and AI38131. B. Damania is a fellow of theCancer ResearchInstitute.

	FOOTNOTES

^* Corresponding author. Mailing address: New England Regional Primate Research Center, Harvard Medical School, One Pine HillDr., Box 9102, Southborough, MA 01772-9102. Phone: (508) 624-8041.Fax: (508) 624-8190. E-mail: ronald_desrosiers{at}hms.harvard.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Alexander, L., L. Denenkamp, A. Knapp, M. Auerbach, S. Czajak, B. Damania, and R. C. Desrosiers. 1999. The primary sequence of rhesus rhadinovirus isolate 26-95: sequence similarities to Kaposi's sarcoma herpesvirus and rhesus rhadinovirus isolate 17577. J. Virol.
2.	Beaufils, P., D. Choquet, R. Z. Mamoun, and B. Malissen. 1993. The (YXXL/I)2 signaling motif found in the cytoplasmic segments of the bovine leukaemia virus envelope protein and Epstein-Barr virus latent membrane protein 2A can elicit early and late lymphocyte activation events. EMBO J. 12:5105-5112[Medline].
3.	Cambier, J. C. 1995. Antigen and Fc receptor signaling. The awesome power of the immunoreceptor tyrosine-based activation motif (ITAM). J. Immunol. 155:3281-3285[Medline].
4.	Cambier, J. C., and W. A. Jensen. 1994. The hetero-oligomeric antigen receptor complex and its coupling to cytoplasmic effectors. Curr. Opin. Genet. Dev. 4:55-63[CrossRef][Medline].
5.	Cambier, J. C., C. M. Pleiman, and M. R. Clark. 1994. Signal transduction by the B cell antigen receptor and its coreceptors. Annu. Rev. Immunol. 12:457-486[CrossRef][Medline].
6.	Cantley, L. C., and Z. Songyang. 1994. Specificity in recognition of phosphopeptides by src-homology 2 domains. J. Cell Sci. 18(Suppl.):121-126.
7.	Cesarman, E., Y. Chang, P. S. Moore, J. W. Said, and D. M. Knowles. 1995. Kaposi's sarcoma-associated herpesvirus-like DNA sequences in AIDS-related body-cavity-based lymphomas. N. Engl. J. Med. 332:1186-1191[Abstract/Free Full Text].
8.	Clark, M. R., S. A. Johnson, and J. C. Cambier. 1994. Analysis of Ig-alpha-tyrosine kinase interaction reveals two levels of binding specificity and tyrosine phosphorylated Ig-alpha stimulation of Fyn activity. EMBO J. 13:1911-1919[Medline].
9.	Damania, B., M. Li, J. K. Choi, L. Alexander, J. U. Jung, and R. C. Desrosiers. 1999. Identification of the R1 oncogene and its protein product from the rhadinovirus of rhesus monkeys. J. Virol. 73:5123-5131[Abstract/Free Full Text].
10.	Desrosiers, R. C., V. G. Sasseville, S. Czajak, X. Zhang, K. G. Mansfield, A. Kaur, R. P. Johnson, A. A. Lackner, and J. U. Jung. 1997. A herpesvirus of rhesus monkeys related to the human Kaposi's sarcoma-associated herpesvirus. J. Virol. 71:9764-9769[Abstract].
11.	Devergne, O., E. Hatzivassiliou, K. M. Izumi, K. M. Kaye, M. F. Kleijnen, E. Kieff, and G. Mosialos. 1996. Association of TRAF1, TRAF2, and TRAF3 with an Epstein-Barr virus LMP1 domain important for B-lymphocyte transformation: role in NF- $kappa$ B activation. Mol. Cell. Biol. 16:7098-7108[Abstract].
12.	Devergne, O., E. C. McFarland, G. Mosialos, K. M. Izumi, C. F. Ware, and E. Kieff. 1998. Role of the TRAF binding site and NF- $kappa$ B activation in Epstein-Barr virus latent membrane protein 1-induced cell gene expression. J. Virol. 72:7900-7908[Abstract/Free Full Text].
13.	Flaswinkel, H., and M. Reth. 1994. Dual role of the tyrosine activation motif of the Ig-alpha protein during signal transduction via the B cell antigen receptor. EMBO J. 13:83-89[Medline].
14.	Gessain, A., A. Sudaka, J. Briere, N. Fouchard, M. A. Nicola, B. Rio, M. Arborio, X. Troussard, J. Audouin, and J. Diebold. 1996. Kaposi sarcoma-associated herpes-like virus (human herpesvirus type 8) DNA sequences in multicentric Castleman's disease: is there any relevant association in non-human immunodeficiency virus-infected patients? Blood 87:414-416[Free Full Text].
15.	Izumi, K. M., and E. D. Kieff. 1997. The Epstein-Barr virus oncogene product latent membrane protein 1 engages the tumor necrosis factor receptor-associated death domain protein to mediate B lymphocyte growth transformation and activate NF- $kappa$ B. Proc. Natl. Acad. Sci. USA 94:12592-12597[Abstract/Free Full Text].
16.	Johnson, S. A., C. M. Pleiman, L. Pao, J. Schneringer, K. Hippen, and J. C. Cambier. 1995. Phosphorylated immunoreceptor signaling motifs (ITAMs) exhibit unique abilities to bind and activate Lyn and Syk tyrosine kinases. J. Immunol. 155:4596-4603[Abstract].
17.	Jung, J. U., J. J. Trimble, N. W. King, B. Biesinger, B. W. Fleckenstein, and R. C. Desrosiers. 1991. Identification of transforming genes of subgroup A and C strains of Herpesvirus saimiri. Proc. Natl. Acad. Sci. USA 88:7051-7055[Abstract/Free Full Text].
18.	Lagunoff, M., R. Majeti, A. Weiss, and D. Ganem. 1999. Deregulated signal transduction by the K1 gene product of Kaposi's sarcoma-associated herpesvirus. Proc. Natl. Acad. Sci. USA 96:5704-5709[Abstract/Free Full Text].
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