CD28-independent, TRAF2-dependent Costimulation of Resting T Cells by 4-1BB Ligand

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© The Rockefeller University Press, 0022-1007/1998/6/1849/ $5.00
The Journal of Experimental Medicine, Volume 187, Number 11, June 1, 1998 1849-1862

Articles

CD28-independent, TRAF2-dependent Costimulation of Resting T Cells by 4-1BB Ligand

Katina Saoulli^*, Soo Young Lee^||, Jennifer L. Cannons^*, Wen Chen Yeh, Angela Santana, Marni D. Goldstein^*, Naveen Bangia^*, Mark A. DeBenedette^*, Tak W. Mak^*^,, Yongwon Choi^,||, and Tania H. Watts^*

From the ^* Department of Immunology, the Department of Medical Biophysics, and Amgen Institute, University of Toronto, Toronto, Ontario M5S 1A8, Canada; and the Howard Hughes Medical Institute and ^|| The Rockefeller University, New York 10021

Abstract

Top
Abstract
Materials and Methods
Results
Discussion
References

4-1BB ligand (4-1BBL) is a member of the tumor necrosis factor(TNF) family expressed on activated antigen-presenting cells.Its receptor, 4-1BB, is a member of the TNF receptor family expressed on activated CD4 and CD8 T cells. We have produceda soluble form of 4-1BBL using the baculovirus expression system.When coimmobilized on plastic with anti-CD3, soluble 4-1BBLinduces interleukin (IL)-2 production by resting CD28⁺ or CD28^–T cells, indicating that 4-1BBL can function independentlyof other cell surface molecules, including CD28, in costimulationof resting T cell activation. At low concentrations of anti-CD3,4-1BBL is inferior to anti-CD28 in T cell activation. However,when 4-1BB ligand is provided together with strong TCR signals,then 4-1BBL and anti-CD28 are equally potent in stimulationof IL-2 production by resting T cells. We find that TNF receptor–associatedfactor (TRAF)1 or TRAF2 associate with a glutathione S-transferase–4-1BBcytoplasmic domain fusion protein in vitro. In T cells, wefind that association of TRAF1 and TRAF2 with 4-1BB requires4-1BB cross-linking. In support of a functional role for TRAF2in 4-1BB signaling, we find that resting T cells isolated fromTRAF2-deficient mice or from mice expressing a dominant negativeform of TRAF2 fail to augment IL-2 production in response tosoluble 4-1BBL. Thus 4-1BB, via the TRAF2 molecule, can provideCD28-independent costimulatory signals to resting T cells.

Key Words: T cells • costimulation • 4-1BB • TRAF2 • signaling

Address correspondence to Dr. Tania H. Watts, Department ofImmunology, University of Toronto, Toronto, ON M5S 1A8, Canada.Phone: 416-978-4551; Fax: 416-978-1938; E-mail: tania.watts{at}utoronto.ca

Abbreviations used: 4-1BBL, 4-1BB ligand; AP, alkaline phosphatase; CT, cytoplasmic tail; DN, dominant negative; GST, glutathione S-transferase; HA, hemagglutinin; ICAM-1, intercellular adhesion molecule 1; JNK, c-Jun NH₂-terminal kinase; NF- ${kappa}$ B, nuclear factor– ${kappa}$ B; RT, reverse transcriptase; s4-1BBL, soluble form of 4-1BBL; TRAF, TNF receptor–associated factor.

Tcells require two signals for activation, an antigen-specificMHC-restricted signal through the TCR and a second costimulatorysignal. CD28 on T cells is widely considered as the primaryreceptor for delivering costimulatory signals to resting Tcells (1). However, CD28^– T cells are not defective inall responses, suggesting the existence of other costimulatorypathways (2–4). One such alternate costimulatory pathwayinvolves the TNFR family member 4-1BB (CDw137), a T cell activationantigen found on activated CD4 and CD8 T cells (5, 6). Theligand for 4-1BB is found on activated B cells, macrophages,and cultured dendritic cells, as well as on several B lymphomasand the thymoma, EL4 (7–11).

A number of studies have shown a role for 4-1BB in T cell activationusing either transfected ligand (7), antibodies against the4-1BB molecule (6, 12–14), or blocking studies with asoluble form of the 4-1BB receptor (10, 11, 15, 16). Anti–4-1BBantibodies are effective in the activation of T cells thathave been preactivated via their TCR to induce high levelsof 4-1BB receptor expression (12), but are poorer agonistsfor induction of IL-2 by resting T cells (6). More recently,Shuford et al. have shown that anti–4-1BB antibodiesinduce higher levels of proliferation of CD8 T cells comparedwith CD4 T cells, leading to the suggestion that 4-1BB is primarilya costimulatory molecule for CD8 T cells (14). In contrast,studies with APCs that express 4-1BB ligand (4-1BBL)¹ haveshown that 4-1BB interaction with its ligand can participatein induction of proliferation and IL-2 and IL-4 production byCD4 T cells. This role for 4-1BBL in the development of Th1and Th2 cells is most apparent in the absence of a strong B7-CD28interaction (11, 16).

Despite the accumulating body of evidence on the importanceof 4-1BB as a costimulatory receptor on activated CD4 and CD8T cells, there is controversy as to whether 4-1BBL alone canprovide a costimulatory signal for resting T cells independentlyof other molecules present on the APC. In this report we describethe production of a soluble form of 4-1BBL (s4-1BBL) usingthe baculovirus expression system. When coimmobilized on plasticwith anti-CD3 or when cross-linked in solution through its influenza hemagglutinin (HA) epitope tag, we find that s4-1BBL is a potent activator of IL-2 production by isolated high density CD28⁺ or CD28^– T cells. When TCR signals are limiting, we find that immobilized anti-CD28 is more effective than 4-1BBL in inducing IL-2 production. However, at higher anti-CD3concentrations, 4-1BBL and anti-CD28 are equally potent ininducing IL-2 production by resting T cells. Thus, isolated4-1BBL can costimulate resting T cells via a CD28-independentpathway.

The observation that 4-1BB signaling can replace CD28 signalingin costimulation of T cell activation under some circumstancesraises the question of how signals from the 4-1BB receptorsynergize with signals from the TCR to induce high level IL-2production. 4-1BB is a member of the TNFR superfamily. Othermembers of this family have been shown to signal via the TNFR-associatedfactor (TRAF) family of signaling molecules first identifiedby their ability to interact with the cytoplasmic domains of TNFR family members (17, 18). Six members of the TRAF family(TRAF1–6) have been identified to date (17–25).The TRAF proteins appear to function as adapter proteins thatlink TNFR family members to downstream signaling pathways.TRAF family members have in common a conserved TRAF-C domaininvolved in homotypic interactions or in heterotypic interactionswith other TRAF molecules and with the cytoplasmic tails ofTNFR family members. The TRAF2 molecule has been shown to interactdirectly with the cytoplasmic tails of CD40, CD30, and TNFR2and indirectly with TNFR1 (17, 18, 26–31) and has beenshown to induce both nuclear factor (NF)- ${kappa}$ B and c-Jun NH₂-terminalkinase (JNK) activation in response to TNF stimulation (26,32–34).

Transgenic mice expressing a dominant negative (DN) form ofTRAF2 (TRAF2 241-501) in their lymphoid cells (TRAF2 DN mice)have reduced JNK activity, but relatively normal NF- ${kappa}$ B activation(35). Similar results have also been obtained using mice thathave been rendered TRAF2 negative by gene targeting (36). Herewe show that T lymphocytes isolated from traf2^–/–or TRAF2 DN mice fail to augment IL-2 production in responseto s4-1BBL. Thus the 4-1BB costimulatory signal leading to IL-2 production is dependent on the TRAF2 molecule.

Materials and Methods

Top
Abstract
Materials and Methods
Results
Discussion
References

Cell Lines, Mice, Antibodies and Reagents.
The T hybrid, C8.A3, was obtained from Dr. Laurie Glimcher(Harvard Medical School, Boston, MA). CD28^– mice (2)were backcrossed on to the H-2^b background (n = 10). C57BL/6mice were obtained from Charles River Laboratories (St. Constant,Quebec, Canada). CD28^– or B6 mice were used at 8–10wk of age.

TRAF2 DN mice have been described previously (35). These micehad been backcrossed on to the BALB/c background. TRAF2 DNmice express TRAF2 (241-501) under the control of the IgH enhancerto drive the transgene expression only in B and T cells. TRAF2(241-501) lacks the RING finger domain and this form of TRAF2has been previously shown to act as a dominant negative inhibitorof TNF and CD40 signaling (26). Spleen cells and lymph nodeswere obtained from TRAF2 DN mice or their transgene-negativelittermates at 8–10 wk of age.

traf2^–/– mice were generated by gene targeting asdescribed elsewhere (36). TRAF2 expression was ablated usinga replacement vector that replaces the entire RING finger codingregion and intervening intron of traf2 with the PGK-Neo genein the reverse orientation to the endogenous traf2 gene. traf2^–/–mice were generated by breeding heterozygous mice. Lymph nodes were obtained from surviving traf2^–/– mice or theirtraf2^+/+ littermates at $~$ 3 wk of age. Hereafter, we will referto these mice as TRAF2^– and TRAF2⁺, respectively.

Mice overexpressing TRAF1 under control of the H-2^k promoterhave been described previously (38). These mice express $~$ 10-foldmore TRAF1 in their spleen and lymph nodes compared with wild-typemice, but have normal numbers of lymphocytes in their peripherallymphoid organs. The anti-CD3-producing hybridoma 145-2C11 (39)was provided by Dr. Jeff Bluestone (University of Chicago,Chicago, IL). The 12CA5 producing hybridoma (40) was obtainedfrom Dr. Bob Phillips (University of Toronto, Toronto, Canada).The hybridomas N418 (anti-CD11c), Y3-P (anti-A^b), RA3-6B2 (anti-B220), TIB-128 (anti-MAC-1), YN1/1.7.4 (anti–intercellular adhesion molecule [ICAM]-1), RG7/7.6H2 (anti–rat Ig ${kappa}$ chain), and M1/69 (anti–heat stable antigen) were obtained from theAmerican Type Culture Collection (Rockville, MD). Antibodieswere purified from hybridoma supernatants using protein G–or protein A–Sepharose (Pharmacia Biotech, Piscataway,NJ), according to the manufacturer's instructions. The anti–CD28-secretinghybridoma 37.51.1 (41) was provided by Dr. Jim Allison (University of California, Berkeley, CA). 3T3 cells secreting 4-1BB linkedto alkaline phosphatase (AP) were provided by Dr. Byoung Kwon (Indiana University, Indianapolis, IN). 4-1BB–AP waspurified on anti–AP-Sepharose as previously described(9). AP from human placenta was obtained from Sigma ChemicalCo. (St. Louis, MO). Anti–4-1BB (1AH2) was purchasedfrom Pharmacia Biotech.

Generation of s4-1BBL.
4-1BBL is a type II glycoprotein. To generate s4-1BBL in insectcells, we linked cDNA encoding the 4-1BBL extracellular COOH-terminaldomain to the signal sequence from myelin-associated glycoprotein,a signal sequence previously shown to be effective in directingthe secretion of heterologous proteins in the baculovirus expressionsystem (reference 42 and see Fig. 1 A). An HA epitope tag waslinked to the COOH terminus of the 4-1BBL molecule to facilitateisolation of the secreted molecule.

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Figure 1 Generation of a soluble form of 4-1BBL. (A) Schematic representation of the construct used to generate s4-1BBL. MAG SS, MAG signal sequence. (B) Coomassie blue–stained SDS-PAGE of s4-1BBL produced in baculovirus and isolated from insect cell supernatants using 12CA5 anti-HA affinity chromatograpy as described in Materials and Methods.

cDNA encoding the extracellular domain of 4-1BBL was obtainedby reverse transcriptase (RT) PCR amplification of RNA isolatedfrom the BALB/c B lymphoma K46J, since this cell line has beenshown to express functional 4-1BBL. RNA was extracted from K46Jcells using Promega RNAgents Total RNA Isolation System (PromegaCorp., Madison, WI). Single-stranded cDNA was synthesized from2 µg of total RNA using the First-Strand cDNA SynthesisKit (Pharmacia Biotech). PCR was performed with the primers5'-GCT TCT CGA GGG GGA CAC CGC ACC GAG CCT CGG CCA GC-3' and5'-ATT GCC GGC CCT TCC CAT GGG TTG TCG GGT T-3' (OligonucleotideSynthesis Laboratory, University of Toronto, Toronto, Canada)and 1 µg of template cDNA, using an initial 2-min denaturationat 94°C, followed by 30 cycles of each of the following:94°C for 1 min, 55°C for 1 min, and 72°C for 1 min,and a final 6-min extension at 72°C to produce a 645-bpproduct (including 4-1BBL 104-309). The PCR product was insertedinto the pCR II vector using the TA Cloning Kit (InvitrogenCorp., Carlsbad, CA) and transformed into One Shot Cells (Invitrogen Corp.) for sequencing using the T7 Sequencing Kit (Pharmacia Biotech). Four independently derived RT-PCR products, derivedfrom the K46J cell line, were sequenced. Sequencing of theseindependently derived RT-PCR products revealed a differencefrom the published sequence of C to A at NTD 476, resultingin a change from Lys to Gln at amino acid 142. Goodwin et al. originally isolated 4-1BBL from the EL4 thymoma, which originatesfrom C57Bl/6 mice, whereas the 4-1BBL cDNA isolated here wasfrom a BALB/c lymphoma (7). Therefore, this difference in sequencemay represent a polymorphism between mouse strains.

The myelin-associated glycoprotein (MAG) signal sequence wasadded 5' to the 4-1BBL 104-309 gene by subcloning into the XhoI–AvaI sites of pShoNEX 1.1 (obtained from Rob Dunn, McGill University, Montreal, Canada). The HA tag was added3' to the MAG–4-1BBL 104-309 gene by NheI insertion intothe baculovirus vector pETL-HA (obtained from C. Richardson, Amgen Institute, Toronto, Canada; reference 43). The recombinantgene was inserted by homologous recombination into the wild-typeAcMNPV baculovirus in SF9 cells by cotransfection using theLinear Transfection Module (Invitrogen Corp.). Recombinant baculovirusclones were identified by plaque assay, and their purity wasconfirmed by PCR analysis using the primers 5'-TTT ACT GTTTTC GTA ACA GTT TTG-3' and 5'-CAA CAA CGC ACA GAA TCT AG-3'.

s4-1BBL in SF9 cell supernatants was detected by capture ELISAusing antibodies to the HA tag (12CA5) for capture and s4-1BBreceptor, 4-1BB–AP, for detection. Wells were coated at 37°C for 1 h with 20 µg/ml (100 µl/well) of12CA5 in PBS. Wells were then blocked with PBS/5% skim milk/0.1%Tween 20 two times for 30 min at 37°C. After blocking,the wells were coated with various dilutions of supernatantsfrom uninfected cultures or cultures infected with recombinantor wild-type virus (100 µl). After 90 min at room temperature,wells were washed three times with PBS/0.1% Tween 20. 5 µg/mlof 4-1BB–AP (100 µl/well) diluted in PBS/5% skimmilk/0.1% Tween 20 was added to each well for 45 min at roomtemperature, and plates were washed three times with PBS/0.1%Tween 20. Finally, 1 mg/ml of p-nitrophenylphosphate (SigmaChemical Co.) in 10% diethanolamine was added to the wells,and OD₄₀₅ was measured using a Titertek Plus reader (Flow Laboratories,McLean, VA).

The recombinant virus was amplified in SF9 cells grown in Grace'sinsect media supplemented with 2% lactalbumin hydrolysate (GIBCOBRL, Gaithersburg, MD), 2% yeastolate (GIBCO BRL), plus 10%fetal bovine serum (GIBCO BRL), and titered by plaque assaybefore use for protein production.

Purification of s4-1BBL.
s4-1BBL was produced and purified as follows. A 3-liter suspensionculture of 1–2 x 10⁶ SF9 cells/ml grown in SF900II (GIBCOBRL) at room temperature was infected with recombinant virusat a multiplicity of infection of 10– 20 and harvested6 d after infection. s4-1BBL molecules were purified from thesupernatant by affinity chromatography on 12CA5 Sepharose.12CA5 Sepharose 4B was prepared using cyanogen bromide–activatedSepharose (Pharmacia Biotech) according to the manufacturer'sinstructions. To ensure that effects of s4-1BBL were not influencedby the presence of endotoxin, the level of endotoxin in thepurified s4-1BBL was measured using the Limulus amebocytes lysateQCL 1000 kit (BioWhittaker Inc., Walkersville, MD) and foundto be less than 0.1 U/ml.

Generation of 4-1BB Cytoplasmic Tail (CT)–GST Fusion and Measurement of 4-1BB CT–TRAF Association.
The entire cytoplasmic tail of 4-1BB was obtained by PCR fromthe 4-1BB full length cDNA using primers 5'-GGGAATTCAAATGGATCAGGAAAAAATTCCC-3'and 5'-GGGGATCCTCACAGCTCATAGCCTCCTCCTC-3'. Amplified PCR fragmentswere sequenced and fused in-frame to GST by cloning into EcoRIand BamHI sites of pEBG, a mammalian GST expression vector,to generate pEBG–4-1BBCT. The plasmids, pEBG, pEBG-4-1BB, and pEBG-CD30CT (28), were transfected into 293 cells. 48 h after transfection, GST and GST fusion proteins were purified with glutathione beads. For in vitro association experiments,the full-length murine TRAF1 and TRAF2 cDNA in pBluescript (Stratagene Inc., La Jolla, CA) were transcribed and translatedin vitro using the TNT coupled reticulocytes system (Promega) with ³⁵S-labeled methionine. Equal amounts of in vitro translated TRAF1 or TRAF2 were incubated in binding buffer (PBS containing0.1% NP-40, 0.5 mM DTT, 10% glycerol, 1 mM PMSF, and 2 µg/mlaprotinin) with $~$ 5 µg of fusion protein bound to glutathionebeads for 45 min at 4°C. After washing five times withbinding buffer, the proteins were eluted by boiling in SDS sample buffer for 5 min and subsequently analyzed by SDS-PAGE.

Measurement of TRAF1 and TRAF2 Association with 4-1BB in C8.A3 T Cells.
For measurement of TRAF1 and TRAF2 association in C8.A3 T hybrids,2 x 10⁷ C8.A3 cells were incubated on ice with 5 µg/mlof anti–4-1BB (1AH2) or with rat anti– ICAM-1 (YN1)control antibody for 5 min. The antibody was cross-linked with20 µg/ml of RG7 (anti–rat ${kappa}$ chain) for 15 min at37°C. After stimulation the cells were lysed with 10 mMTris, 1 mM MgCl₂, 50 mM NaCl, 0.5% NP-40, 2 µg/ml aprotinin, and 1 mM PMSF. Lysates were immunoprecipitated for 4 h at 4°C with 40 µl of protein G–Sepharose (SigmaChemical Co.). For unstimulated controls, antibody and secondstep were added on ice and the samples were carried throughthe same immunoprecipitation protocol. Precipitated proteinswere separated by SDS-PAGE and transferred to nitrocellulose.TRAF proteins were detected by polyclonal rabbit anti–murineTRAF1 (S-19) and anti–murine TRAF2 (C-20) (Santa CruzBiotechnologies, Santa Cruz, CA). Bound antibodies were detectedwith goat anti–rabbit Ig–horseradish peroxidase(Molecular Probes, Eugene, OR) and detected by chemiluminescenceaccording to the manufacturer's protocol (ECL system; AmershamLife Science, Arlington Heights, IL).

T Cell Isolation.
APCs were depleted from spleen or lymph node cell suspensionsin HBSS (GIBCO BRL)/2.5% FCS/50 µM 2-ME, with a cocktailof antibodies, anti–class II (Y3P), anti-B220, anti–heatstable antigen (M1/69), anti–MAC-1, and anti-CD11c (N418)each at a final concentration of 10 µg/ml at 4°C for 30 min. A 1:10 dilution of baby rabbit complement (CedarlaneLabs. Ltd., Hornby, Ontario, Canada) was added, and the cultureswere further incubated at 37°C for 40 min. To remove adherentcells, the cell suspensions were passaged through a SephadexG10/nylon wool column, and then centrifuged through Percollgradients consisting of 60, 70, and 80% Percoll layers. Small(high density) T cells were isolated from the 70/80% interfaceand used in all subsequent experiments.

T Cell Activation Assays.
Monoclonal anti-CD3 (145-2C11) was immobilized on the surfaceof 96-well plates (Nunc, Gaithersburg, MD) by incubating for5 h at 37°C. Where indicated, s4-1BBL or anti-CD28 antibodieswere added to the wells at the same time. 0.5–1 x 10⁵small high density T cells, from either C57BL/6, CD28^–mice, TRAF2 DN mice, TRAF2^–, or littermate controls werecocultured with either immobilized anti-CD3 antibody alone,or in the presence of immobilized s4-1BBL, immobilized anti-CD28,or control antibody as indicated in the figure legends. After2 d the culture supernatants were collected, and assayed fortheir ability to induce proliferation of the IL-2– dependentcell line CTLLs as previously described (10).

Results

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Abstract
Materials and Methods
Results
Discussion
References

Generation of s4-1BBL Using the Baculovirus Expression System.
At the time we began these studies, Hurtado et al. had shownthat antibodies to 4-1BB could activate preactivated T cellsbut were rather poor in the activation of resting T cells (12).In contrast, we had found that B lymphomas expressing 4-1BBLcould induce high levels of IL-2 and IL-4 production by restingT cells (10, 16). Therefore, it was possible either that 4-1BBLwas more potent in activating resting T cells than were availableantibodies or that other molecules on the APC contributed toT cell activation by 4-1BBL. To distinguish these possibilities,we generated a soluble form of 4-1BBL using the baculovirusexpression system.The entire extracellular domain of 4-1BBL was expressed in isolation with the addition of an influenza HA epitope tag at the COOH terminus of the protein to facilitatepurification (Fig. 1 A). Fig. 1 B shows a Coomassie blue–stainedgel of purified s4-1BBL isolated from the insect cells using12CA5 (anti-HA) affinity chromatography. It can be seen thats4-1BBL forms a disulfide-linked dimer of $~$ 63 kD, consistentwith the expected molecular weight for the glycosylated formof the extracellular domain. The band is slightly heterogeneous,possibly due to variable glycosylation or due to limited proteolysis.

Activation of CD28⁺ and CD28^– T Cells by 4-1BBL.
To assess the activity of s4-1BBL in the activation of resting T cells, high density resting T cells from the spleens of CD28⁺ or CD28^– mice were isolated by complement and SephadexG10 depletion of APCs followed by Percoll gradient fractionationas described in Materials and Methods. CD28^– T cellswere used to eliminate the possibility of any contributionfrom CD28 signaling. Fig. 2 A shows IL-2 production by purifiedT cells responding to immobilized anti-CD3 in the presenceor absence of immobilized s4-1BBL, added at 1 µg/ml. Itcan be seen that for both CD28⁺ and CD28^– T cells, noIL-2 is generated in response to immobilized anti-CD3 alone,but that coimmobilization of s4-1BBL leads to significant IL-2production. s4-1BBL added in solution did not stimulate a response, but s4-1BBL added in solution together with anti-HA antibodyto cross-link the molecule via the HA tag was also effectivein costimulation (data not shown). Fig. 2 B shows the proliferationof CD28^– T cells in response to immobilized anti-CD3 aloneor with 1 or 10 µg/ml immobilized s4-1BBL. It can beseen that at suboptimal anti-CD3 concentrations, s4-1BBL enhancesT cell proliferation. Fig. 2 C shows that the effect of s4-1BBLcan be fully blocked by coculture with a soluble form of thereceptor, 4-1BB–AP, whereas AP alone had no such effect.Thus, the enhancement of IL-2 production in response to 4-1BBLis specific to the soluble ligand.

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Figure 2 Immobilized s4-1BBL can costimulate proliferation and IL-2 production by CD28⁺ or CD28^– T cells. (A) High density resting T cells isolated from the spleens of CD28⁺ or CD28^– mice were incubated with various concentrations of anti-CD3 alone or with anti-CD3 plus immobilized s4-1BBL added to the plastic wells at 1 µg/ml as indicated in the figures. After 48 h, culture supernatants were removed and serial dilutions of supernatant were incubated with IL-2–dependent CTLL cells for 18–24 h. [³H]thymidine was added for the last 6 h of the CTLL culture. Data are shown for the first dilution of culture supernatant and are representative of four independent experiments. (B) CD28^– T cells were cultured with immobilized anti-CD3 alone or with immobilized anti-CD3 plus s4-1BBL at 1 or 10 µg/ml as indicated in the figure. After 48 h, [³H]thymidine was added to the wells and thymidine uptake was determined after a further 6 h of culture. Similar results were obtained in three separate experiments. (C) CD28^– cells were cultured with anti-CD3 (1 µg/ml) in the presence or absence of s4-1BBL (1 µg/ml) or in the presence of s4-1BBL (1 µg/ml) plus 4-1BB-AP (10 µg/ml). After 48-h incubation, culture supernatants were analyzed for induction of thymidine incorporation by CTLL. 4-1BB–AP alone had no effect on IL-2 production. Results are shown for serial dilutions of the culture supernatants and are representative of four independent experiments.

Fig. 3 compares the sensitivity of CD28⁺ and CD28^– T cells to s4-1BBL. It can be seen that the IL-2 response of CD28⁺ and CD28^– T cells saturates at a concentration of s4-1BBL of between 2 and 5 µg/ml. This titration experimentwas repeated using a different batch of purified s4-1BBL andshowed a similar saturation point (data not shown). The responseof CD28^– T cells to s4-1BBL is somewhat reduced comparedwith that of CD28⁺ T cells. Higher responses of CD28⁺ versusCD28^– T cells to s4-1BBL might be due to low level expressionof B7.2 on the T cells or due to the presence of B7 on contaminating APCs. Differences between the magnitude of the response ofCD28⁺ and CD28^– T cells to s4-1BBL were not apparent inall experiments (for example, see Fig. 2) but tended to varywith the particular T cell preparation. Similar differencesbetween CD28⁺ and CD28^– T cell responses to 4-1BBL werepreviously observed using 4-1BBL on APCs (11). Flow cytometryanalysis of CD28⁺ and CD28^– T cells after overnight treatmentwith anti-CD3 showed similar levels of induction of 4-1BB onthe surface (data not shown). Thus the difference in responseto s4-1BBL on CD28⁺ or CD28^– T cells does not appearto be due to differential expression of 4-1BB in response toanti-CD3 treatment of CD28⁺ or CD28^– T cells.

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Figure 3 Effect of 4-1BBL titration on CD28⁺ and CD28^– T cell responses. High density resting T cells isolated from the spleens of CD28⁺ or CD28^– mice were incubated with anti-CD3 alone (1 µg/ml) or with anti-CD3 plus immobilized s4-1BBL added to the plastic wells at the concentration indicated in the figures. After 2 d, serial dilutions of the culture supernatant were incubated with IL-2– dependent CTLL cells overnight. [³H]thymidine was added to the CTLL cultures for the last 6 h of culture. Similar results were obtained in three independent experiments.

Kinetics of IL-2 Production in Response to Anti-CD3 Plus s4-1BBL.
4-1BB is an activation antigen on T cells. 4-1BB mRNA appearswithin 3 h of anti-CD3 stimulation (45), but surface expressionof 4-1BB is not apparent until several hours later (6). Therefore,it was important to establish the kinetics of response to s4-1BBL.Fig. 4 shows IL-2 production by resting CD28^– T cellsat various times after exposure to immobilized anti-CD3 plusimmobilized s4-1BBL. It can be seen that IL-2 production byresting T cells responding to anti-CD3 plus immobilized s4-1BBLis detectable by 24 h with further increases in IL-2 productionby 48 h. The kinetics of response to s4-1BBL is similar tothe response of T cells to 4-1BBL expressed on B lymphomas,where we detected some IL-2 production by 12 h with increasingamounts at 24–48 h (11). Thus the kinetics of the responseto s4-1BBL appears to be rapid enough to explain the abilityof 4-1BBL to activate resting T cells and suggests that quitelow levels of 4-1BB on the T cell surface may be sufficientto provide T cell costimulation.

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Figure 4 Kinetics of IL-2 production in response to 4-1BBL. Resting T cells isolated from the spleens of CD28^– mice were incubated with anti-CD3 alone (1 µg/ml) or with anti-CD3 plus s4-1BBL immobilized at the concentrations indicated on the figure. After 12, 24, or 48 h, culture supernatants were removed and serial dilutions were analyzed for induction of proliferation of IL-2–dependent CTLL cells. Results are representative of two separate experiments.

Comparison of Costimulatory Activity of 4-1BBL with Anti-CD28 Antibodies.
To compare the efficacy of the 4-1BB versus CD28 costimulatorypathways for resting T cell activation, we compared T cell responsesto immobilized anti-CD28 and immobilized s4-1BBL in the presenceof various doses of anti-CD3 as shown in Fig. 5. Anti-CD28was titrated in a separate experiment (data not shown) and the concentration which gives maximum stimulation when immobilizedwith 1 µg/ml of anti-CD3 (10 µg/ml anti-CD28) wascompared with s4-1BBL at 5 µg/ml. It can be seen thatat low doses of anti-CD3, anti-CD28 is more effective than s4-1BBLin stimulating IL-2 production by resting CD28⁺ T cells. However,if one increases signals through the TCR, via increasing thedensity of immobilized anti-CD3, then 4-1BBL and anti-CD28 inducesimilarly high levels of IL-2 production by resting CD28⁺ T cells. As expected, only s4-1BBL but not anti-CD28 enhancedIL-2 production by CD28^– T cells. Thus, 4-1BBL can providea similar level of costimulation as anti-CD28 when providedwith a strong TCR stimulus, but is less effective when signalsthrough the TCR are limiting.

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Figure 5 Comparison of immobilized s4-1BBL with immobilized anti-CD28 for costimulation of IL-2 production by CD28⁺ and CD28^– T cells. Resting T cells isolated from CD28⁺ or CD28^– T cells were stimulated by immobilized anti-CD3 at the indicated concentrations plus or minus 4-1BBL immobilized at 5 µg/ml or anti-CD28 at 10 µg/ml or control Ig at 10 µg/ml. After 48 h, supernatants were removed and analyzed for the presence of IL-2 using CTLL cells. Results are representative of two independent experiments.

Association of 4-1BB with TRAF1 and TRAF2.
The mechanism by which 4-1BB signals T cells to costimulateIL-2 production is not known. 4-1BB is a member of the TNFRfamily of signaling molecules. As discussed above, the TRAFfamily of signaling molecules appear to function as adapterproteins in the signal transduction cascades leading to NF- ${kappa}$ Band JNK activation by members of this family. Since TRAF2 hasbeen shown to interact directly with the cytoplasmic tailsof several TNFR family molecules, we chose to focus on a possiblerole for TRAF2 in 4-1BB signaling. Therefore, the 4-1BB cytoplasmicdomain was expressed as a GST fusion protein in 293 cells. Purified4-1BB– CT-GST bound to glutathione Sepharose was usedto probe the association of the 4-1BB cytoplasmic domain within vitro translated ³⁵S-methionine labeled TRAF1 and TRAF2 proteins (Fig. 6). TRAF1 and TRAF2 were found to associatewith 4-1BB–CT-GST as well as CD30-GST (included as a positivecontrol). No association was observed between TRAF1 and TRAF2and GST alone.

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Figure 6 Association between the 4-1BB cytoplasmic tail-GST fusion protein and TRAF1 and TRAF2 proteins. As described in Materials and Methods, purified GST, GST-CD30CT, and GST–4-1BBCT proteins bound to glutathione beads were incubated with ³⁵S-labeled in vitro– translated TRAF1 or TRAF2. After washing, samples were eluted and analyzed by SDS-PAGE followed by autoradiography. In vitro–translated TRAF1 and TRAF2 were also run directly on the gel (lanes marked TRAF1 and TRAF2) for comparison.

We also attempted to detect TRAF association with the 4-1BB–CT-GSTprotein in 293 cells, but were not successful (data not shown),which suggests that in cells, aggregation of 4-1BB might berequired to induce TRAF association as has been shown for CD40/TRAFassociation (44). To test this hypothesis, we analyzed theassociation of TRAF1 and TRAF2 with full-length 4-1BB in theT cell hybridoma C8.A3. This T cell hybridoma has been shown previously to respond to 4-1BB signaling and expresses low levels of 4-1BB in the resting state, with further upregulationof 4-1BB after overnight treatment with anti-CD3 (10). C8.A3cells were incubated with anti–4-1BB and goat anti–ratIg for 15 min at 37°C or on ice, after which time the cellswere lysed and protein G–Sepharose added to immunoprecipitatethe complex. When 4-1BB was cross-linked at 0°C little orno TRAF1 or TRAF2 could be detected by Western blot analysisof the immunoprecipitated material (Fig. 7). In contrast, aggregationof 4-1BB at 37°C using anti–4-1BB followed by anti–ratIg induced the association of TRAF1 and TRAF2 with the 4-1BBprecipitates. Cross-linking of ICAM-1 on the T cells using rat anti–ICAM-1 and anti–rat Ig at 37°C did notresult in significant levels of TRAF1 or TRAF2 in the ICAM-1immunoprecipitates (Fig. 7). Thus, the presence of TRAF1 andTRAF2 in the immunoprecipitates is specific to the 4-1BB molecule.These results show that cross-linking of 4-1BB on T cells resultsin its enhanced association with TRAF1 and TRAF2 and that thereis little or no TRAF1 and TRAF2 associated with 4-1BB in theresting state.

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Figure 7 Association of TRAF1 and TRAF2 with 4-1BB in a T cell hybrid is induced by receptor aggregation at 37°C. C8.A3 T cells (2 x 10⁷ cells/ lane) were stimulated with anti– 4-1BB or with anti–ICAM-1 on ice for 5 min and then cross-linked with anti–rat Ig for 15 min on ice or at 37°C. Lysates were immunoprecipitated with protein G–Sepharose. Immunoprecipitates were separated by SDS-PAGE and analyzed by Western blotting with either anti-TRAF1 or anti-TRAF2. This experiment is representative of three separate experiments.

Role of the TRAF Family of Signaling Molecules in Costimulation of IL-2 Production by s4-1BBL.
Based on the association of the 4-1BB cytoplasmic domain withTRAF2 (Figs. 6 and 7) and the importance of TRAF2 in JNK activation in response to TNF, we explored the functional role of TRAF2using T cells isolated from TRAF2^– mice, as well as usingT cells isolated from TRAF2 DN mice.

To test the effect of the TRAF2 DN mutant on 4-1BB signalingleading to IL-2 production, we isolated high density restingT cells from TRAF2 DN mice and their transgene negative littermates.Fig. 8 compares IL-2 production by the T cells in responseto anti-CD3 alone, anti-CD3 plus immobilized s4-1BBL or anti-CD3plus immobilized anti-CD28 antibody. For the wild-type T cells,immobilized s4-1BBL clearly augments the response of resting spleen or lymph node T cells to immobilized anti-CD3. As wasobserved in Fig. 5, the effects of s4-1BBL on IL-2 productionare smaller than those of anti-CD28. The TRAF2 DN T cells showeda higher background response to anti-CD3 alone and additionof s4-1BBL actually led to a decrease in response of the TRAF2DN T cells. In contrast, anti-CD28 augmented IL-2 productionin response to anti-CD3 in both the wild-type mice and TRAF2DN mice. Although responses to anti-CD28 were retained in allinstances, with lymph node T cells we sometimes observed a lower response to anti-CD28 in transgenic T cells compared withthe nontransgenic controls (e.g., anti-CD28 at 10 µg/mlin Fig. 8). In contrast, splenic T cells sometimes showed hyperresponsivenessto anti-CD28 (e.g., anti-CD28 2 µg/ml, Fig. 8). In spiteof the variable response to anti-CD28, the observation thatthe TRAF2 DN mice largely retain responses to anti-CD28 butfail to show augmentation of IL-2 production in response toimmobilized s4-1BBL suggests that the TRAF2 signaling moleculeis required for 4-1BB signaling.

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Figure 8 Decreased response to 4-1BBL by T cells isolated from mice expressing a dominant negative form of TRAF2. Resting T cells were isolated from spleen and lymph nodes TRAF2 DN mice or their transgene-negative littermates, as described in Materials and Methods. T cells were incubated with anti-CD3 immobilized on plastic at the concentrations indicated in the figures in the presence or absence of immobilized s4-1BBL (5 µg/ml) or immobilized anti-CD28 at 2 or 10 µg/ml as indicated in the figure. At 48 h of culture, supernatants were analyzed for IL-2 production using CTLL cells. Results shown are for a single representative mouse. Similar results were obtained in three independent experiments with two control and two mutant mice analyzed separately in each experiment.

Fig. 9 shows a similar experiment carried out using T cellsisolated from the lymph nodes of TRAF2^– mice. As describedelsewhere, TRAF2^– mice have small lymphoid organs anddie on average at day 10–14 after birth (36). However,some mice survived to 3 wk and were used for these experiments.The spleens of these mice are atrophied and could not be usedfor T cell isolation, but a small number of resting T cellscould be isolated from the lymph nodes of these animals. Itcan be seen that the T cells from the TRAF2^– mice retainthe ability to respond to anti-CD28, but show no enhancementof anti-CD3 signaling by immobilized 4-1BBL. Again, the responseto anti-CD3 alone was higher in the TRAF2-deficient animalsthan the littermate controls and the addition of 4-1BBL actuallyreduces the response to anti-CD3 alone. Similarly to the resultswith lymph node T cells from the TRAF2 DN mice (Fig. 8), theresponse of lymph node T cells to anti-CD3 plus anti-CD28 wasalso somewhat reduced.

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Figure 9 Decreased response to 4-1BBL by T cells isolated from TRAF2^– mice. Resting T cells were isolated from the lymph nodes of TRAF2^– mice or their wild-type TRAF2⁺ littermates. T cells were incubated with anti-CD3 alone (immobilized at 1 µg/ml) or with anti-CD3 plus immobilized s4-1BBL (5 µg/ml) or immobilized anti-CD28 (2 µg/ml). Results are shown from one mouse and are representative of two independent experiments with two mice per experiment.

In addition to TRAF2, the 4-1BB cytoplasmic domain also interactswith TRAF1 (Figs. 6 and 7). T cells from transgenic mice thatoverexpress TRAF1 have been shown to proliferate normally inresponse to TCR engagement, but are resistant to antigen-inducedapoptosis (38). Consistent with the observations that TRAF1overexpression does not influence T cell proliferative responses(38), we find that T cells from mice overexpressing TRAF1 showed no differences in IL-2 production in response to anti-CD3 plus immobilized s4-1BBL compared with wild-type controls (datanot shown).

Discussion

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Abstract
Materials and Methods
Results
Discussion
References

The delivery of a signal through the CD28 molecule has beenshown to be critical for activation of T cells and for preventionof induction of cell death or an anergic state. For a costimulatoryreceptor to prevent the induction of anergy, it is thoughtthat the costimulatory signal must be delivered simultaneouslyor within a few hours of signaling through the TCR (46). Previousstudies using antibodies to 4-1BB to stimulate T cells havefound that unprimed T cells require 4–5 d to respondto anti–4-1BB, but that T cells that have been preactivatedfor 2–3 d to induce a high level 4-1BB expression, respondwithin 48 h (6, 12). Our data using 4-1BBL on APCs (11) orusing s4-1BBL (this report) show that T cells can produce IL-2in response to 4-1BBL within 24 h in the absence of CD28 costimulation.Other studies in which antibodies to 4-1BB have been used tocostimulate with anti-CD3 either used preactivated T cells (12)or did not separate resting from activated T cells (14). BecauseB7 family members are expressed on activated T cells, one cannotrule out that low levels of B7 were also contributing to theresponse in these studies (12, 14). Although we have previouslyshown that CD28^– T cells can respond to 4-1BBL expressedon APCs (16), in those studies it was possible that other molecules present on the cell surface contributed to this signal. Our study therefore used purified resting T cells from CD28^– mice and soluble 4-1BBL to test the role of 4-1BBL in isolation.The data presented here clearly show that 4-1BBL alone canprovide an effective costimulatory signal for resting T cellactivation, independent of other cell surface molecules includingthe CD28 molecule.

The ability of s4-1BBL to induce IL-2 in T cells more rapidlythan anti–4-1BB antibody may be due to the natural ligandfor 4-1BB providing a more potent signal than that deliveredby antibody ligation. Although surface expression of 4-1BB isnot obvious until at least 24 h after anti-CD3 treatment ofresting T cells (6), 4-1BB mRNA is readily detectable within3 h of anti-CD3 treatment (45). Our data showing that functionalresponses to isolated 4-1BBL occur within 24 h of T cell activationsuggests that it may take only a few 4-1BB molecules on theT cell surface to allow costimulatory signals to be transduced.Thus, our data show that 4-1BBL can, under appropriate conditions,function in a similar way to and independently of the CD28molecule to provide a costimulatory signal for induction ofIL-2 production by resting T cells.

A comparison of the costimulatory activity of immobilized anti-CD28and immobilized s4-1BBL (Fig. 5) showed that anti-CD28 is moreeffective than immobilized s4-1BBL in inducing IL-2 productionat low doses of anti-CD3. However, at higher concentrationsof anti-CD3, one can achieve similar levels of IL-2 productionin response to CD28 or 4-1BB engagement. CD28 is expressedon resting T cells, whereas 4-1BB is expressed only after signaling through the TCR. When anti-CD3 is bound to the plates at lowdensity, the level of 4-1BB receptor induced may be limiting,thus explaining the poorer response to s4-1BBL at low anti-CD3concentrations. Alternatively or additionally, the lower responseto s4-1BBL at low anti-CD3 doses might be due to 4-1BBL providinga weaker costimulatory signal than anti-CD28. This weaker signalfrom 4-1BBL– 4-1BB interaction may be compensated forby increasing signals through the TCR. Nevertheless, when signals through the TCR are optimized, 4-1BBL can function as wellas anti-CD28 in induction of IL-2 production by resting T cells(Fig. 5).

Shahinian et al. have shown that CD28^– T cells are unimpairedin their immune response to LCMV infection (2). Interestingly,there is evidence that it is the duration of TCR signalingthat allows CD28-independent immune responses to LCMV (47).In light of our data, one could interpret the data of Kündiget al. (47) as suggesting that antigens that induce strong signalsthrough the TCR may allow other CD28-independent costimulatorypathways, such as the 4-1BB pathway, to take over. The kineticsof the response to s4-1BBL (Fig. 4) suggest that if signal1 is strong enough, then 4-1BB can be induced and receive sufficient signals to induce IL-2 production within 24 h.

A critical question is how the various cell surface moleculesinvolved in T cell activation integrate the signals from distinctsignal transduction pathways to induce high level IL-2 geneexpression. T cell receptor signaling and CD28 signaling havebeen shown to synergize at the level of JNK (48). TRAF2 hasbeen implicated in the ability of both TNFR1 and CD40 to activateJNK (32–36). Therefore, an attractive hypothesis is that4-1BB signaling can replace CD28 signaling by synergizing withthe TCR at the level of JNK activation. As a first step towardtesting this model, we have analyzed the role of TRAF2 in Tcell activation by 4-1BB.

Using a GST fusion protein, we showed that the cytoplasmic domainof 4-1BB could associate with TRAF1 and TRAF2 in vitro (Fig.6). However, attempts to demonstrate an association betweenthe 4-1BB CT and TRAF1 and 2 in 293 cells using the same GSTfusion protein were not successful. This suggested that aggregationof 4-1BB might be required for TRAF association in cells. Insupport of this, we found that TRAF1 and TRAF2 association with 4-1BB in a T cell hybrid required cross-linking of 4-1BBat 37°C. During the revision of this manuscript, two groupshave also reported an association of TRAF1 and TRAF2 with the4-1BB cytoplasmic domain using yeast 2 hybrid analysis (49,50). Arch and Thompson (49) demonstrated TRAF1 and TRAF2 associationwith the murine 4-1BB cytoplasmic domain. In addition, usinga fusion protein between the murine 4-1BB cytoplasmic domainand the transmembrane/extracellular domains of CD28, Arch and Thompson found constitutive association of 4-1BB with TRAF2 in HEK293 cells (49). Jang et al. have reported that TRAF1and TRAF2 associate with human 4-1BB and they find that whenfull-length 4-1BB and the TRAF proteins are overexpressed in293 these associations are observed in the absence of 4-1BBreceptor cross-linking (50). The difference between those studiesand our results may reflect the higher level of proteins expressedin the 293 cells versus our use of endogenously expressed moleculesin T cells.

In this report we have also shown that resting T cells isolatedfrom mice that lack TRAF2 or express a dominant negative formof TRAF2 in their lymphoid subset fail to respond to 4-1BBsignaling. TRAF2^– mice have very small lymphoid organsand die at 2–3 wk of age, whereas mice expressing a TRAF2DN transgene in their lymphoid cells are viable and have enlargedlymphoid organs due to the presence of an abnormal number ofB cells. In spite of these marked phenotypic differences, bothtypes of TRAF2-deficient mice have demonstrated an essentialrole for TRAF2 in JNK activation in response to TNF (35, 36).Similarly, in this report we have demonstrated that the twodifferent types of TRAF-deficient mice have very similar outcomes for the T cell response to 4-1BBL. That is, responses to anti-CD28were retained, whereas responses to 4-1BBL actually went frombeing stimulatory in wild-type mice, to being inhibitory toanti-CD3–induced IL-2 production in TRAF2-deficient mice(Figs. 8 and 9). The observation that signaling via 4-1BB isactually slightly inhibitory to anti-CD3–stimulated Tcells is unexplained. It is possible that this result is dueto an inhibitory signal from 4-1BB that is normally maskedby the positive signaling effects of TRAF2.

For both TRAF2 DN mice and TRAF2^– mice, we also observedan increase in background response to anti-CD3 alone. The reasonfor this increase in background is not clear. The purity ofT cells from TRAF2 DN mice or their transgene-negative littermateswas indistinguishable and addition of CTLA-4 Ig to block effectsof B7 family molecules had no effect on the response (data notshown). Thus, the increased response of isolated resting Tcells to immobilized anti-CD3 does not appear to be due to thepresence of contaminating B7-expressing APCs. Lee et al. have shown that the response of TRAF2 DN lymph node T cells toanti-CD3 presented by accessory cells is decreased comparedwith transgene-negative littermates (35). The data in our report,showing a slight decrease in the response of lymph node TRAF2DN T cells to anti-CD3 and anti-CD28, agrees with that finding.However, the increased response to anti-CD3 alone (Figs. 8and 9) is puzzling. Yeh et al. have shown that serum levelsof TNF are increased in TRAF2-deficient animals and have suggestedthat lack of TRAF2 leads to dysregulation of TNF synthesis(36). It is possible that the dysregulation of TRAF2 preventsfeedback inhibition of the expression of other molecules producedby or expressed on the purified T cells, and that these inturn allow enhancement of the response to anti-CD3 alone.

In addition to associating with TRAF2 (Figs. 6 and 7), the4-1BB cytoplasmic tail can also associate with TRAF1 in vitro.The biological significance of this finding remains to be tested.In contrast to the results with TRAF2-negative mice or withmice expressing a dominant negative form of TRAF2, T cellsfrom mice that overexpress wild-type TRAF1 showed no perturbationof responses to anti-CD3 plus anti-CD28 or s4-1BBL (data notshown). These results are not surprising in view of the datafrom Speiser et al., which showed that T cells from the TRAF1overexpressing mice have normal proliferative responses butare resistant to antigen-induced apoptosis (38). This lackof perturbation of 4-1BB signaling by overexpression of TRAF1could be due to the dispensability of TRAF1 for 4-1BB costimulatorysignals or could be because the amount of TRAF1 recruited during4-1BB signaling in wild-type mice is not limiting. It was alsopossible that overexpression of TRAF1 would interfere withsignaling via TRAF2 by forming heterodimers that prevent otherinteractions of the TRAF2 molecule, but this did not seem to occur, as 4-1BB signaling was neither impaired nor enhancedby overexpression of TRAF1 (data not shown).

In summary, the results presented here show that 4-1BBL canfunction in isolation to costimulate T cell responses thatare independent of the CD28 molecule. When signaling throughthe TCR is strong, 4-1BB signaling is as effective as anti-CD28signaling in stimulating IL-2 production by T cells. In contrast,at low anti-CD3 doses, the CD28 costimulatory pathway seemsto be more effective than the 4-1BB costimulatory pathway.The induction of IL-2 in response to the 4-1BB costimulatorysignal is dependent on the presence of a functional TRAF2 molecule.Given the importance of TRAF2 in JNK activation in responseto CD40L or TNF, a plausible model is that synergistic activationof JNK by TCR plus 4-1BB via TRAF2 leads to high level IL-2gene transcription and in this way the 4-1BB molecule can replacethe CD28 molecule in resting T cell activation. Thus, our dataadd to the accumulating body of evidence for a pivotal rolefor the TRAF2 molecule in signaling by TNFR family members.

	Acknowledgments

We thank Chris Richardson for advice on the baculovirus expressionsystem and for providing the pETL-HA vector, Sf 9, and Hi5insect cell lines. We thank Rob Dunn for providing the MAG signalsequence-containing vector, and Pam Ohashi for helpful suggestions.

This work was funded by a grant from the Medical Research Councilof Canada (MRC) to T.H. Watts, by a grant from the NationalCancer Institute of Canada (NCIC) to T.W. Mak, and by a grantfrom the Howard Hughes Medical Institute to Y. Choi; K. Saoulliand M.D. Goldstein are funded by MRC studentships; W.-C. Yehis funded by an MRC postdoctoral fellowship; and T.H. Wattsis a Senior Scientist of the NCIC with funds from the CanadianCancer Society.

Submitted: 18 December 1997
Revised: 2 April 1998

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