Originally published In Press as doi:10.1074/jbc.M000531200 on April 11, 2000
J. Biol. Chem., Vol. 275, Issue 24, 18586-18593, June 16, 2000
TTRAP, a Novel Protein That Associates with CD40, Tumor Necrosis
Factor (TNF) Receptor-75 and TNF Receptor-associated Factors (TRAFs),
and That Inhibits Nuclear Factor-
B Activation*
Stefan
Pype
§,
Wim
Declercq¶
,
Abdelilah
Ibrahimi,
Christine
Michiels,
Johanna G. I.
Van
Rietschoten**,
Nathalie
Dewulf,
Mark
de Boer**,
Peter
Vandenabeele¶
,
Danny
Huylebroeck§§§, and
Jacques E.
Remacle¶¶
From the Department of Cell Growth, Differentiation
and Development, Flanders Interuniversity Institute for Biotechnology,
Campus Gasthuisberg, University of Leuven, Herestraat 49, B-3000
Leuven, Belgium, the § Laboratory of Molecular Biology
(Celgen), University of Leuven, B-3000 Leuven, Belgium, the
¶ Department of Molecular Biology, Flanders Interuniversity
Institute for Biotechnology, University of Gent, K. L. Ledeganckstraat
35, B-9000 Gent, Belgium, and the ** Tanox Pharma B. V., Kruislaan
318, 1098 SM Amsterdam, The Netherlands
Received for publication, January 20, 2000, and in revised form, April 7, 2000
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ABSTRACT |
CD40 belongs to the tumor necrosis factor (TNF)
receptor family. CD40 signaling involves the recruitment of TNF
receptor-associated factors (TRAFs) to its cytoplasmic domain. We have
identified a novel intracellular CD40-binding protein termed
TRAF and TNF receptor-associated protein (TTRAP)
that also interacts with TNF-R75 and CD30. The region of the CD40
cytoplasmic domain that is required for TTRAP association overlaps with
the TRAF6 recognition motif. Association of TTRAP with CD40 increases
profoundly in response to treatment of cells with CD40L. Interestingly,
TTRAP also associates with TRAFs, with the highest affinity for TRAF6.
In transfected cells, TTRAP inhibits in a dose-dependent
manner the transcriptional activation of a nuclear factor-
B
(NF-B)-dependent reporter mediated by CD40, TNF-R75 or
Phorbol 12-myristate 13-acetate (PMA) and to a lesser extent by TRAF2,
TRAF6, TNF-
, or interleukin-1
(IL-1). TTRAP does not affect
stimulation of NF-B induced by overexpression of the
NF-B-inducing kinase (NIK), the IB kinase (IKK), or the
NF-B subunit P65/RelA, suggesting it acts upstream of the latter
proteins. Our results indicate that we have isolated a novel regulatory
factor that is involved in signal transduction by distinct members of
the TNF receptor family.
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INTRODUCTION |
CD40 is a member of the tumor necrosis factor
(TNF)1 receptor family that
plays a critical role in many immunological processes (1). The receptor
is present on many cell types, and its function has been studied most
extensively in B cells, dendritic cells, monocytes, and endothelial
cells. Characterization of mice deficient for CD40 or its ligand CD40L
(also named CD154) highlights the importance of CD40-mediated signaling
in the thymus-dependent humoral immune response and in
isotype switching (2-4). CD40-mediated signal transduction induces the
transcription of a large number of genes implicated in host defense
against pathogens. This is accomplished by the activation of multiple
transcription factors, including NF-B (5), c-Jun (6), and STAT3 (7).
In the past 5 years we have come to understand in significant detail the cascade that leads from stimulation of TNF receptors to the activation of transcription factors. The signal transduction is triggered by binding of trimeric ligands of the TNF family to their
cognate receptors, which induces oligomerization of the latter at the
cell surface. This brings the intracellular domains of these receptors
in close proximity whereby they serve as a high affinity binding
platform for many cytoplasmic proteins involved in signal transduction.
Members of the TNF receptor family, such as CD30, CD40, TNF-R75, OX40,
RANK, and 4-1BB, have been implicated primarily in gene activation
rather than apoptosis and transmit their signal through the direct
recruitment of TRAFs (8). TRAFs 1-6 display similar structural
features, i.e. they have an N-terminal RING finger (which is
absent in TRAF1), followed by 5-7 zinc fingers, and a C-terminal TRAF
domain that mediates receptor binding. CD40 associates with TRAFs 2, 3, 5, and 6 (9-12). The importance of the latter for signaling by CD40
and other receptors has become clear from the characterization of
TRAF6-deficient mice. Experiments performed with cells derived from
these mice demonstrated that TRAF6 is crucial for CD40L, IL-1, and
lipopolysaccharide-dependent activation of NF-B (13).
These results confirmed earlier observations that TRAF6 is involved in
gene activation through members of the TNF receptor and IL-1 receptor
families (11, 14-16). Recently, TRAF2 was also shown to be essential
for CD40-mediated responses in mice (17). The molecular mechanisms by
which TRAFs activate downstream effector proteins remain largely
unknown. However, the current data suggest that this involves the
interaction of TRAFs with different types of kinase. Some of these are
involved in pathways leading to NF-B activation, e.g. NIK
(18), MEKK1 (19), and TAK1 (20). These kinases have the potential to
activate the IB kinases (IKK and IKK) (21-23), which
phosphorylate IB. This phosphorylation triggers ubiquitination and
subsequent degradation of IB, resulting in the release of NF-B
subunits that translocate into the nucleus, where they act as
transcription activators (reviewed in Ref. 24).
Signal transduction by members of the TNF receptor family also involves
several regulatory factors. Most of these proteins have been identified
as TRAF-binding proteins, e.g. A20 (25), I-TRAF/TANK (26,
27), and TRIP (28). Although their precise role in the signal
transduction process remains elusive, overproduction of these factors
either inhibits (in the case of A20, I-TRAF, TRIP) or synergistically
activates (in the case of TANK) TRAF-mediated activation of NF-B. As
a result of a search for novel effector proteins involved in CD40
signaling, this study describes the identification of a novel
regulatory protein that binds receptors and TRAFs and that inhibits
activation of NF-B.
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EXPERIMENTAL PROCEDURES |
Reagents and Plasmids--
Anti-FLAG M2 monoclonal antibody was
purchased from Sigma and anti-CD40 polyclonal antibody C20, that was
used for Western blot, was obtained from Santa Cruz Biotechnology
(Santa Cruz, CA). Anti-hemagglutinin (HA) tag monoclonal antibody was a
gift from Innogenetics S. A. (Zwijnaarde, Belgium), and anti-hCD40 5D12 monoclonal antibody, used for immunoprecipitation, was from Tanox
Pharma B. V. (Amsterdam, The Netherlands). The anti-hTNF-R75 mouse
monoclonal antibody utr4 was a gift of M. Brockhaus and W. Lesslauer
(Roche, Basel, Switzerland). The anti-hTNF-R75 polyclonal antibodies
were from W. Buurman (University Maastricht, The Netherlands). The
following expression vectors for production of human and murine TRAFs
were a gift from D. Goeddel (Tularik Inc., South San Francisco, CA):
FLAG-hTRAF2-pRK5, FLAG-
TRAF2-pRK5 (insert encodes amino acids
87-501 of mouse TRAF2 (10)), FLAG-hTRAF6-pRK5, and
FLAG-289TRAF6-pRK5 (insert encodes amino acids 289-511 of human
TRAF6 (16)). FLAG-317TRAF6-pcDNA3 was constructed by PCR
amplification on FLAG-hTRAF6-pRK5, engineering an EcoRI site
at the 5'-end of the partial cDNA and cloning the EcoRI-XhoI fragments into FLAG-pcDNA3.
HA-hTRAF3-pcDNA3 was a gift from V. Dixit (University of Michigan,
Ann Arbor, MI). HA-IKK-pcDNA and Xpress-NIK-pcDNA3 were a
gift from M. Karin (University of California San Diego, La Jolla, CA).
FLAG-hTRAF5-pME was provided by J. Inoue (Tokyo University, Tokyo,
Japan) and P65/RelA-pRc/cytomegalovirus by S. Plaisance (University of
Gent, Gent, Belgium).
CD40 cDNA was amplified by PCR from a human umbilical vein
endothelial cell (HUVEC) cDNA library and cloned into pcDNA3.
The cDNAs encoding the cytoplasmic part of human CD40 (amino acids 216-277 (11)), human TNF-R75 (262-437 (29)), and human CD30 (408-595
(30)), were generated by PCR and inserted into the pEG202 vector
(Gyuris et al. (32)) in-frame with the sequence encoding the
LexA DNA-binding domain. The cDNA for the C-terminal cytoplasmic
domain of LMP1 (amino acids 192-386 (31)) was obtained from M. Rowe
(University of Wales, Cardiff, United Kingdom (UK)). Our CD40
deletion and point mutants were constructed by PCR, as described by
Ishida and co-workers (11), and cloned into pEG202. Plasmid
hTNF-R75-pcDNA6 was described previously (29), and human TRADD was
cloned in frame with an N-terminal E tag, into pcDNA3.
4F2 and TRAF3 partial cDNAs that were picked in our two-hybrid
screening were excised from pJG4-5, using EcoRI, and
subcloned into the similarly digested vectors pEG202, FLAG-pcDNA3
and HA- pcDNA3. Full-length TTRAP cDNA was cloned in two
ways. First, cloning into HA-pcDNA3 was done starting directly from
the cDNA picked from the HUVEC library, via digestion with
EcoRI and ligation into HA-pcDNA3. In doing so, 34 nucleotides from the library vector and 20 from the 5'-untranslated
region of TTRAP cDNA are present between the sequence encoding the
HA tag and the translation initiation codon of TTRAP. Second, for
cloning of TTRAP cDNA in pJG4-5, a PCR-based approach was used. An
EcoRI site was engineered directly adjacent to the 5'-end of
the TTRAP cDNA by amplification of TTRAP cDNA using the primer
combination 5'-GACGAATTCAGAGGCGGCAGGAAGATGGAGTTGG and
5'-GCCTCACATCCTGAATGCAGGA. The amplified fragment was then digested with EcoRI and BglII and ligated
together with a BglII-NcoI TTRAP cDNA
fragment into pJG4-5. FLAG-TTRAP-pcDNA3 and TTRAP-pCS2 were
obtained by ligation of the EcoRI fragment from
TTRAP-pJG4-5 into FLAG-pcDNA3 and pCS2, respectively.
Two-hybrid Screening--
Two-hybrid screening in yeast was
performed by the interaction trap cloning method, which is often
referred to as the LexA two-hybrid system (32). The cytoplasmic part of
human CD40 was cloned in-frame with the LexA DNA-binding domain (the
bait plasmid). Screening was done using a HeLa cell cDNA library in
pJG4-5 (the prey plasmid), which was obtained from R. Brent (Harvard
Medical School, Boston, MA). EGY48 (MAT , his3, trp1,
ura3-52, leu2::pLEU2-LexAop) yeast cells were
transformed with the prey plasmid, the bait plasmid, and the lacZ
reporter plasmid pSH18-34 by the lithium acetate transformation
method (33).
Yeast cells containing bait plasmid and lacZ reporter
plasmid were transformed with 20 µg of library plasmid and plated on glucose medium lacking tryptophan, histidine and uracil, to select for
the presence of all three plasmids. In total, approximately 2 × 106 colonies were obtained. These transformants were
harvested and frozen at 
80 °C in a glycerol solution (65%
glycerol (v/v), 100 mM MgSO4, 25 mM
Tris/HCl pH 7.4). To screen for protein-protein interaction, 20 × 106 colony-forming units of an amplified stock of original
transformants were tested for a positive interaction phenotype, as
described (32). When using yeast two-hybrid as test for interaction, we performed mating assays (34). Bait and prey constructs were transformed
in yeast strain EGY48 (mating type ) and EGY42 (mating type a), respectively.
Northern Blotting, in Situ Hybridization and Isolation of
Full-length TTRAP cDNA--
Northern analysis of human and murine
mRNA blots (CLONTECH, Palo Alto, CA) was
carried out with human 4F2 and the entire cDNA of mouse TTRAP (EST
clone 876634) as probes, respectively. Blots were hybridized at
65 °C in QUICKHYB hybridization solution (Stratagene, La Jolla, CA).
The 2-kb-long probe used for in situ hybridization was the
same as used for Northern analysis of mouse TTRAP. In vitro
transcription with T3 RNA Polymerase yielded [35S]-uracil
(NEN Life Science Products) labeled single-stranded riboprobe. In
situ hybridization in sections of mouse embryos was done as
described previously (35).
Full-length human TTRAP cDNA was obtained by screening a HUVEC
cDNA plasmid library with human 4F2 as probe; colony lifting and
hybridization was as described previously (36). The mouse TTRAP
homologue was obtained by screening with BLAST (37) the EST data base
for sequences homologous to human TTRAP. EST clone 1262914 (GenBankTM accession number AI465781) was requested from
the IMAGE consortium (Cambridge, UK) and sequenced completely to obtain
the mouse TTRAP cDNA sequence. The coiled coil prediction was
obtained by running the program COILS (38).
Transient Transfections and Reporter Assays--
293T human
embryonic kidney cells were grown in Dulbecco's modified Eagle's
medium supplemented with glucose (4.5 g/liter) and 10% (v/v) fetal
bovine serum. Transient transfection of plasmids for luciferase
reporter assay or co-immunoprecipitation analysis was done with Fugene
6 (Roche Molecular Biochemicals), using 2 µl of Fugene per µg of
plasmid DNA. For luciferase reporter assays, transfections were done in
duplicate using 3 × 105 293T cells per well of a
24-well plate. Each well was transfected with 15 ng of reporter plasmid
NFconluc, encoding the luciferase reporter gene driven by a minimal
NF-B-responsive promoter (gift of A. Israel, Institut Pasteur,
Paris, France) or 50 ng of AP-1-luc (Stratagene, La Jolla, CA). To
normalize the transfection efficiency, we co-transfected 75 ng of a
lacZ reporter construct that contains the Rous sarcoma virus
promoter inserted upstream of Escherichia coli
lacZ. If the amount of TTRAP plasmid used in transfections was varied, we kept the total amount of DNA constant by adding a
Myc-TTRAPmutant-pCS3 construct that does not produce TTRAP protein, because the TTRAP cDNA was cloned out-of-frame of the sequence encoding the N-terminal Myc tag. Cell extracts were prepared and assayed for luciferase activity and -galactosidase activity
according to the manufacturers' protocols (Promega (Madison, WI) and
CLONTECH (Palo Alto, CA), respectively). Data were
normalized by calculating the ratio of luciferase and -galactosidase
activities. The average normalized luciferase activity is presented
relative to the activity in nonstimulated samples as x-fold activation.
For co-immunoprecipitation, 1-2 × 106 293T cells
were transfected with 2 µg of each expression vector. In the
TRAF-TTRAP co-immunoprecipitation experiments, we noticed that
overexpression of TRAFs 2, 3, 5, and 6 resulted in different synthesis
levels of TTRAP from the co-transfected TTRAP-pcDNA3 construct.
This was probably because of the fact that the cytomegalovirus promoter
in the pcDNA3 vector (Invitrogen BV, Groningen, The Netherlands) is
sensitive to the different levels of NF-B induced by overexpressing
these TRAFs. To circumvent this problem, we co-transfected 0.1 µg of
hNIK-pcDNA3, which potently stimulates NF-B.
Stimulation of cells with CD40L was done by overlaying transfected
cells with mouse 3T6 fibroblasts stably transformed with an expression
vector encoding hCD40L (39). As a negative control we used
nontransfected 3T6 cells. Transiently transfected 293T cells at
subconfluence were overlaid with approximately twice the number of 3T6 cells.
Co-immunoprecipitation and Western Blotting--
Cells were
harvested 24-48 h after transfection in 300 µl of lysis buffer (50 mM Tris/HCl, pH 7.4, 200 mM NaCl, 10%
glycerol, 0.2% Nonidet P-40, 50 mM NaF, 1 mM
Na4P2O7, 5 mM
NA3VO4, 1 mM phenylmethylsulfonyl
fluoride, 3 µg aprotinin/ml). Cells were then lyzed by incubation for
20 min on ice or by passing five times through a 22-gauge needle.
Cellular debris and nuclei were eliminated by centrifugation (Eppendorf
4517R, 14,000 rpm, 4 °C, 10 min). Five µg of antibody was added to
the lysate and incubated for 3 h at 4 °C. Subsequently, 20 µl
of a 50% slurry of protein G-Sepharose (Amersham Pharmacia Biotech,
Gent, Belgium) was added to the samples, and the incubation was
continued for 1 h. Next, the-Sepharose was washed four times in
750 µl of lysis buffer for 10 min at 4 °C. Finally, the beads were
mixed with 20 µl of sample buffer, and the samples were analyzed by
SDS-polyacrylamide gel electrophoresis. To verify the expression levels
of the different proteins, 0.1% of the cytoplasmic extract was
analyzed on Western blot.
Proteins were separated on 12.5% Tris-Tricine gels and transferred
onto polyvinylidene difluoride membrane (NEN Life Science Products)
using a semi-dry blotting apparatus (Sigma). For Western analysis, the
membrane was blocked in 3% skimmed milk in TBS-T (10 mM
Tris/HCl, pH 7.4, 150 mM NaCl, 0.2% Tween 20). After
sequential incubation with primary and horseradish
peroxidase-conjugated secondary antibody (Jackson Laboratories, West
Grove, PA) for 1 h at 24 °C, proteins were visualized with the
ECL chemiluminescent detection system (NEN Life Science Products).
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RESULTS |
Cloning of a Novel CD40-binding Polypeptide--
A two-hybrid
screen in yeast was set up to identify novel CD40-interacting proteins.
The cDNA encoding the cytoplasmic region of CD40 was cloned into
the bait vector, which was transformed in yeast together with a HeLa
cDNA library cloned in the prey vector. After screening
approximately 2 × 106 transformants, eight different
cDNAs were isolated from yeast colonies with a positive interaction
phenotype. The corresponding eight polypeptides were tested for
interaction with the cytoplasmic domain of other members of the TNF
receptor family, i.e. human TNF-R75 and CD30. In addition,
we also used as bait the C-terminal 192 amino acids of LMP1 from
Epstein-Barr virus. Similar to CD30, CD40, and TNF-R75, LMP1 can signal
through direct interaction with TRAFs (40, 41). One of the prey
plasmids that was isolated in our screen contained a cDNA sequence
encoding part of TRAF3 (amino acids 381-568, comprising part of the
TRAF-N domain and the complete TRAF-C domain (9)). This hybrid prey
protein associated with the cytoplasmic region of CD40, CD30, and LMP1,
but not TNF-R75 (Table I), which is in
accordance with published results for TRAF3 (10, 30, 41). Another
positive prey, coded 4F2, bound to CD40, CD30, and TNF-R75 baits but
not the LMP1 bait (Table I). The interaction phenotype of 4F2 with
TNF-R75 was somewhat weaker than with CD40 and CD30. Also, the
interaction phenotype of the latter two receptors with 4F2 was
apparently not as strong as with the N-terminally truncated TRAF3 prey.
The 1.8-kb-long partial cDNA for 4F2 encoded a novel polypeptide
with no homology to TRAFs or other factors known to be involved in TNF
receptor signaling.
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Table I
Interaction test of TRAF3 (amino acids 381-566), 4F2, and TTRAP with
the cytoplasmic domain of different receptors, using the yeast
two-hybrid assay
The interaction phenotype was estimated by blue/white staining of yeast
colonies. Staining was scored as blue, i.e. relatively
strong and visible within 12 hours (++), strong and visible within 24 hours (+), or as white ().
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To obtain a full-length cDNA of this protein, we screened a HUVEC
cDNA library using 4F2 cDNA as a probe and isolated a 2-kb-long cDNA. This yielded a complete open reading frame encoding a protein of 362 amino acids, that has been named TTRAP (TRAF and
TNF Receptor-associated protein). Recently the complete genomic sequence of human
TTRAP became available in the data base as a cosmid clone that maps to
chromosome 6p22.1-22.3 (EBI accession number AL031775). The sequence of
mouse TTRAP was obtained by sequencing EST clone 1262914, and the
candidate Caenorhabditis elegans homologue of TTRAP was
retrieved from the data base as putative protein predicted from the
genomic sequence. Further comparison of TTRAP with the public data
bases revealed that it is related to the C-terminal 380 amino acids of
the yeast transcription factor CCR4 (42) and to a CCR4-like protein
named nocturnin, which has been isolated from Xenopus (43)
and recently also from human and mouse (44). CCR4 is distinct from
TTRAP and nocturnin because it is approximately twice as big. The
alignment of the TTRAP-related protein sequences shows that, although
the overall amino similarities are rather low, there are stretches of
identical amino acids scattered throughout the C-terminal 250 residues
in the alignment (Fig. 1). The data in
Table II furthermore indicate that
nocturnin is more related to CCR4 than to TTRAP, whereas the C. elegans protein is more similar to TTRAP than to nocturnin. Taken
together, our results indicate that TTRAP, nocturnin, and CCR4 belong
to an emerging gene family. Neither nocturnin nor the C-terminal part
of CCR4 has been characterized functionally.
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Fig. 1.
Alignment of the amino acid sequences of
human TTRAP (hTTRAP), mouse TTRAP
(mTTRAP), C. elegans TTRAP
(celTTRAP), Xenopus nocturnin
(xnoctur), and the C-terminal part of yeast CCR4
(yCCR4-C). Residue 1 of yCCR4-C shown here
corresponds to amino acid 385 of the full-length protein (57). The
start of the partial human TTRAP polypeptide, 4F2, is indicated with a
thick arrow. Upright arrowheads show the
hydrophobic residues that could potentially be involved in the
formation of a coiled coil region. Boxed amino acids are
identical or physicochemically similar in 3 (light gray), 4 (dark gray), or all (black) of the aligned
sequences.
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Table II
Amino acid identity (percentage) for pair wise aligned protein
sequences
The aligned sequences and their GenBankTM/EBI accession numbers
are: hTTRAP (human, AJ269473); mTTRAP (mouse, AJ251328); celTTRAP
(C. elegans, CAA21707); hnocturnin (human, AAD56548.1);
xnocturnin (Xenopus laevis, P79942); yCCR4-C (S. cerevisiae, amino acids 385-837, P31384).
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The only known structural feature that could be deduced from the
primary structure of TTRAP is a potential short coiled coil motif
between amino acids 236 and 250 (Fig. 1), but this motif is poorly
conserved in the C. elegans candidate TTRAP. Like 4F2, TTRAP
also interacted with CD30, CD40, and TNF-R75 in the yeast two-hybrid
assay (Table I). Interestingly, in the latter assay TTRAP also
interacted with itself.
Distribution of Human and Mouse TTRAP mRNA in Adult Tissues and
Embryos--
We examined the expression of TTRAP mRNA using
multiple tissue Northern blots, with 4F2 cDNA as a probe. In human
tissues, a 2.2-kb transcript was observed in all tissues tested. In
testis, an additional transcript of approximately 1.8 kb could be seen (Fig. 2A). The mouse TTRAP
cDNA was used as a probe to screen murine blots. This revealed two
transcripts of 3.4 and 2.2 kb, respectively (Fig. 2B), the
larger of which is the more prominent. Like human TTRAP, mouse TTRAP
mRNA was expressed in all of the adult tissues tested, but in heart
and skeletal muscle the signal was very weak. In addition to adult
expression, mouse TTRAP mRNAs are present in embryos throughout
post-implantation, with somewhat a different ratio between the 2.2-and
3.4-kb bands (Fig. 2C). In situ hybridization in
sections of E12.5 mouse embryos showed that TTRAP mRNA was
expressed ubiquitously (data not shown). At E15.5, widespread
expression was weak, but stronger signals were observed in the kidneys,
the small intestine, the seminiferous tubules of the testis, the lungs,
the liver, brown fat, and the submandibular gland. The most striking
expression was observed in the thymus lobes and in discrete regions of
the brain (Fig. 2D).
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Fig. 2.
Analysis of TTRAP mRNA expression in
adult human and murine tissues and in the murine embryo. Northern
blots from human (A) and mouse (B, C)
tissues are shown. The blots were also hybridized with a rat probe for
glyceraldehyde 3-phosphate dehydrogenase (GAPDH).
D, in situ hybridization of TTRAP on a
section of an E15.5 mouse embryo. Darkfield and brightfield images are
shown in the right and left panel, respectively.
Abbreviations: b.f., brown fat; ki, kidney;
li, liver; lu, lung; th, thymus;
s.g., submandibular gland, and s.i., small
intestine.
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TTRAP Interaction with CD40 Is Increased by Stimulation of Cells
with CD40L--
To confirm the interactions observed in yeast, we
first tested co-immunoprecipitation of 4F2 with CD40 or TNF-R75 in
cultured human cells. 293T cells were transfected with expression
plasmids for FLAG-tagged 4F2 and either CD40, TNF-R75, or empty plasmid (as negative control). Extracts from transfected cells were then incubated with antibodies specific for CD40 or TNF-R75, followed by
immunoprecipitation of these receptors. Subsequent Western blotting
with anti-FLAG antibody revealed that 4F2 co-precipitated both with
CD40 and TNF-R75 (Fig. 3A,
lanes 1 and 2 and 3 and 4, respectively). We further examined whether cell stimulation with CD40L
would affect the TTRAP-CD40 interaction. Expression vectors for CD40
and FLAG-TTRAP were co-transfected in 293T cells, and cells were
stimulated with CD40L for a period of 2, 8, or 24 h. We repeatedly
observed that treatment of the cells with CD40L for up to 24 h
resulted in strongly increased TTRAP binding to CD40. In the experiment
displayed in Fig. 3B, the amount of TTRAP co-immunoprecipitated with CD40 was densitometrically estimated to
increase at least 10-fold after 24 h of stimulation. This could neither be explained by increasing levels of cellular production of
TTRAP, which varied no more than 2-fold, nor was it because of
increased precipitation of CD40 (Fig. 3B). In separate
experiments (data not shown), this increase at 24 h even amounted
to approximately 50-fold compared with the level of interaction at
8 h of stimulation.
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Fig. 3.
Co-immunoprecipitation of 4F2 and TTRAP with
CD40 and TNF-R75. A, FLAG-4F2-pcDNA3 (2 µg) was
transiently transfected in 293T cells together with 2 µg of
CD40-pcDNA3 (lane 1) or TNF-R75-pcDNA6 (lane
3) (both indicated as +) or empty vector (lanes 2 and
4; indicated as ). Immunoprecipitation was performed as
described under "Experimental Procedures." Top panels,
Western blot of 4F2-FLAG co-immunoprecipitated with CD40 (lanes
1 and 2) or TNF-R75 (lanes 3 and
4). The 5D12 or utr4 antibodies visible in the
immunoprecipitates are marked IgG. Lower panels, synthesis
level of 4F2-FLAG in lysates from transfected 293T cells. B,
CD40-pcDNA3 (2 µg) was transiently transfected in 293T cells
together with 2 µg of FLAG-TTRAP-pcDNA3. All cells were harvested
at the same time point, i.e. 48 h after transfection,
so the CD40L-expressing 3T6 fibroblasts were added to the 293T cells
24, 8, or 2 h prior to harvesting. The nonstimulated cells (0 h)
were treated with 3T6 control cells for 2 h prior to harvesting.
Co-immunoprecipitations were carried out as described under
"Experimental Procedures." Co-precipitation of TTRAP-FLAG with CD40
is depicted in the top panel. Middle panel,
immunoprecipitation of CD40. Lower panel, synthesis of
TTRAP-FLAG in lysates from transfected 293T cells. In the
top and bottom panels, proteins were detected
with anti-FLAG antibody, and in the middel panel, anti-CD40
was used.
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The TTRAP Binding Site on CD40 Differs from That of TRAF3--
The
binding sites for TRAF2 and TRAF3 in the cytoplasmic domain of CD40
have been mapped to the PVQET motif (residues 250-254), whereas TRAF6
has been shown to bind to a distinct motif, KQEPQEINF (residues
230-238) (11, 45). In addition to binding TRAFs, CD40 interacts with
JAK3 by a motif located N-terminal to the TRAF6 binding site (residues
222-229) (7). To map the region that binds TTRAP, a panel of CD40 tail
mutants was tested as bait in a yeast two-hybrid assay. As a control
prey, we used the partial TRAF3 that was picked in our original
two-hybrid screening.
Shortening of the CD40 cytoplasmic tail from 62 residues (amino acids
216-277) to 30 amino acids (mutant 216-245) had no effect on TTRAP
binding, whereas the same CD40 mutant no longer interacted with TRAF3
(Fig. 4). The latter result is in
accordance with previous observations (11, 45). Further truncation of
the cytoplasmic tail to 14 amino acids (mutant 216-229) abrogated
TTRAP binding. Removing only these 14 amino acids of the cytoplasmic
domain of CD40 (mutant 230-277) did not affect the binding of TTRAP.
These results indicate that residues 230-245 of CD40 are required for its association with TTRAP. We also tested the Thr to Ala mutation at
position 254, which is known to affect CD40 association with TRAFs 2, 3, and 5, as well as JAK3 (7, 45). TTRAP bound to this T254A mutant,
whereas the partial TRAF3 did not (Fig. 4). In summary, these
observations clearly show that the region of CD40 required for binding
TTRAP differs from the one defined previously for TRAF2 and TRAF3, but
may overlap with the interaction site mapped for TRAF6.
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Fig. 4.
Interaction of TTRAP with CD40 requires the
region between residues 230 and 245 in the receptor. TTRAP binding
to mutants of the cytoplasmic domain of CD40 was tested using the yeast
two-hybrid mating assay as described under "Experimental
Procedures." Different fragments of the human CD40 cytoplasmic
domain, and the Thr-254 mutation to Ala (T254A), were used as bait
constructs. Prey constructs were full-length TTRAP or N-truncated TRAF3
(amino acids 381-568). + indicates blue colonies after 24 h
growth on 5-bromo-4-chloro-3-indolyl
-D-galactopyranoside plates; indicates lack of color
development after 48 h. Amino acids printed in bold
represent known binding sites for JAK3, TRAF6, or TRAF2/3.
|
|
TTRAP Inhibits Activation of NF-B Mediated by CD40 and
TNF-R75--
Overexpression of CD40 or TNF-R75 leads to activation of
NF-B (5, 10). To examine whether TTRAP may be involved in these signaling pathways, we investigated the effect of TTRAP overexpression on the activation of a reporter construct specific for NF-B. Co-expression of TTRAP with these receptors inhibited NF-B
activation in a dose-dependent manner (Fig.
5). Typically, we observed that TTRAP
overexpression decreased stimulation mediated by CD40 to a level of
20-30% of that in the absence of TTRAP. When using the CD40 T254A
mutant, which signals through TRAF6 but not TRAF2 or TRAF5 (46), the
inhibition by TTRAP was similar. In the case of TNF-R75, the effect of
TTRAP ranged in the order of 40% residual NF-B activity at the
highest amount of TTRAP tested. To check whether overexpression of
TTRAP influences the receptor expression levels, Western blots were
carried out on the same lysates as used for the luciferase assays (Fig.
5, insets). Synthesis of CD40 or TNF-R75 did not decrease,
indicating that TTRAP down-regulates their signal transduction normally
leading to activation of NF-B.
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Fig. 5.
Inhibition of receptor-mediated activation of
NF-B by TTRAP. 293T cells were
transfected with an NF-B-responsive luciferase reporter plasmid
together with increasing amounts of TTRAP-pCS2 (0, 250, or 500 ng) and
one of the following: 50 ng of CD40-pcDNA3, CD40(T254A)-pcDNA3,
or TNF-R75-pcDNA6 and harvested after 48 h. Western blots in
insets show CD40, TNF-R75, and TTRAP present in 5% of the
cell lysates. Shown are the average values and S.D. of assays performed
in duplicate, which are representative of at least three independent
experiments.
|
|
Interaction of TTRAP with TRAFs--
CD40 has been shown to bind
TRAFs 2, 3, 5, and 6 (9-12). The TRAFs are key players in the signal
transduction cascade, and they interact not only with receptors but
also with other effector proteins (8). We therefore investigated
whether TRAFs could also interact with TTRAP. This was done by
co-immunoprecipitation using protein extracts prepared from cells
transfected with expression vectors for TTRAP-HA and FLAG-tagged human
TRAFs 2, 3, 5, or 6. Immunoprecipitation from cell lysates was
performed with anti-FLAG antibody. Subsequent Western blotting with
anti-HA antibody revealed that TTRAP co-precipitated with all TRAFs
tested, albeit with different efficiency (Fig.
6A). We repeatedly observed
that TTRAP interacted more strongly with TRAF6 than with the other
TRAFs, and this was not because of variation in efficiency of TRAF
precipitation or TTRAP synthesis (Fig. 6A, middle
and bottom panel, respectively). This suggests that TTRAP
has a higher affinity for TRAF6 than for other TRAFs. In contrast to
the ligand-dependent increase of TTRAP association with
CD40 (Fig. 3B), its binding to TRAF6 was not affected by
stimulation of the cells with CD40L for 2 or 24 h (data not
shown). Because TTRAP interacted with TRAFs, we also tested whether the
protein would associate with TRADD, an adaptor protein that links TRAFs
to TNF-R55 (8). However, TTRAP could not be co-immunoprecipitated with
transfected TRADD (data not shown).
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Fig. 6.
TTRAP co-immunoprecipitates with different
TRAFs. HA-TTRAP-pcDNA3 (2 µg) was transiently transfected in
293T cells together with 2 µg of FLAG-tagged wild-type or mutant TRAF
constructs or empty FLAG vector. See "Results" for description of
TRAF6 mutants. A and B, top panels:
co-immunoprecipitation of TTRAP-HA with FLAG-tagged TRAF (mutants). The
anti-FLAG antibody visible in the immunoprecipitates is marked IgG.
Middle panels, immunoprecipitation of FLAG-tagged TRAFs.
Bottom panels, synthesis of TTRAP-HA in lysates from
transfected cells. Proteins were detected with anti-HA antibody
(top and bottom panels) or anti-FLAG antibody
(middle panels).
|
|
To analyze which region in TRAF6 is required for binding TTRAP, we used
TRAF6 deletion mutants. First, we tested the 289TRAF6 mutant that
has no RING or zinc finger domains and therefore consists only of the
TRAF domain (composed of TRAF-N and TRAF-C). TTRAP co-immunoprecipitated equally well with 289TRAF6 as with full-length TRAF6 (Fig. 6B, upper panel, lanes 2 and 1, respectively). By deleting 27 amino acids more,
leaving only half of the TRAF-N domain and the complete TRAF-C domain
(mutant 317TRAF6), the TRAF-TTRAP interaction was abrogated (Fig.
6B, upper panel, lane 3). Thus, in
mammalian cells TTRAP can associate with TRAFs 2, 3, 5, and 6, with
preference for the latter, and our data also show that the N-terminal
half of the TRAF-N domain is required for TTRAP binding.
TTRAP Inhibits Activation of NF-B Mediated by TRAF2, TRAF6, and
PMA, but not by NIK, IKK, or P65/RelA--
It is known that
overexpression of TRAFs 2, 5, and 6 leads to activation of NF-B
(10-12). To examine the effect of TTRAP co-expression on TRAF-mediated
signaling, 293T cells were transfected with TRAF2 or TRAF6 and
increasing amounts of TTRAP. TTRAP inhibited in a dose-dependent manner the TRAF-mediated activation of the
NF-B-dependent luciferase reporter (Fig.
7A), but the effect was not as
profound as on receptor-mediated signaling (Fig. 5). Similar to TRAFs, overexpression of NIK, IKK, and the NF-B subunit P65/RelA induces transcription of the NF-B reporter (18, 21). In contrast to our
observations with CD40, TNF-R75, TRAF2, or TRAF6, TTRAP did not
significantly affect NIK or IKK-induced activation of NF-B (Fig.
7A). Similarly, TTRAP overexpression had no effect on
P65/RelA-mediated transactivation in the nucleus (Fig. 7A). These results suggest either that TTRAP exerts its inhibitory effect
upstream of NIK or IKK- mediated activation of NF-B or that the
pathway(s) involving these kinases are not affected by TTRAP.
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Fig. 7.
Effect of TTRAP overexpression on activation
of NF-B by different stimuli. 293T cells
were transfected with an NF-B (A)-or AP-1
(B)-responsive luciferase construct, together with
increasing amounts of TTRAP-pCS2 (0, 250, or 500 ng) and one of the
following: 50 ng of FLAG-TRAF2-pRK5, 10 ng of FLAG-TRAF6-pRK5, 50 ng of
HA-IKK-pcDNA, 20 ng of Xpress-NIK-pcDNA3, 20 ng of
P65/RelA-pRc, or 0.5 ng of CD40-pCDNA3. Alternatively, cells were
stimulated with TNF- (100 units/ml), IL-1 (100 units/ml), PMA
(250 ng/ml), or CD40L for 24 h. In all cases, activation-fold was
measured relative to cells not transfected with any stimulatory
factor.
|
|
TRAFs have also been implicated in signaling by TNF-R55 and the IL-1
receptor, therefore we tested the effect of TTRAP overexpression on
NF-B activation by these receptors by treating the cells with TNF- and IL-1. Because human embryonic kidney 293 cells do not express detectable levels of TNF-R75, TNF- signals through TNF-R55 only (10). To compare the effect of TTRAP on stimulation by these
ligands with its effect on CD40-mediated activation of NF-B, cells
were also stimulated with CD40L. Because 293T cells do not express the
CD40 gene (45), we transfected relatively low quantities of receptor
expression plasmid, so that ligand independent signaling contributed
less than 5% to the CD40L-induced activation of NF-B. TNF- and
IL-1-induced activation of NF-B was only modestly affected by
TTRAP, whereas stimulation by CD40L was inhibited more profoundly (Fig.
7A) and to a similar extent as observed when overexpressing
CD40 (Fig. 5). In addition to using specific ligands, we also treated
the cells with the protein kinase C activator PMA. Luciferase reporter
levels after stimulation with PMA were reduced to 20-30% at the
highest TTRAP concentration tested (Fig. 7A). Because PMA
also activates transcription of an AP-1-dependent reporter
construct in 293T cells, it was analyzed whether TTRAP could also
inhibit AP-1 induced gene expression. Unlike its effect on PMA-mediated
activation of NF-B, TTRAP did not down-regulate AP-1-dependent gene activation by the phorbol ester (Fig.
7B), suggesting the inhibition by TTRAP may be restricted.
Moreover, the fact that gene activation induced by P65/RelA or AP-1 was not sensitive to TTRAP indicates that the protein does not affect transcription in general. Taken together, these results demonstrate that TTRAP affects NF-B induction in a dose-and
stimulus-dependent fashion.
| |
DISCUSSION |
We report here on the isolation and characterization of the novel
factor TTRAP that interacts with CD30, CD40, and TNF-R75, as well as
with TRAFs 2, 3, 5, and 6. The binding properties of TTRAP resemble
some of those described previously for the TRAFs and are indicative for
a role of TTRAP in the signaling cascade induced by ligands of the TNF
family. Structurally, TTRAP is unrelated to TRAFs or other
intracellular proteins implicated in TNF signaling. The complete genome
sequence for Saccharomyces cerevisiae and C. elegans is now available, and we found a candidate TTRAP homologue in the nematode but not in the yeast. Vertebrates express TTRAP and a
related protein, named nocturnin, the precise function of which is
unknown (43, 44). Another protein distantly related to TTRAP is the
yeast factor CCR4, which is approximately twice as big as TTRAP and
nocturnin (42). The domain homologous to the latter proteins spans the
C-terminal 300 amino acids of CCR4, which has so far not been
functionally characterized. Interestingly, this transcription cofactor
has been shown by genetic analysis to be a potential downstream
mediator of the protein kinase C1-MAPK signaling cascade in yeast (47).
Therefore, our data suggest that TTRAP, nocturnin, and CCR4 are
structurally related proteins with a potential role in signal transduction.
Judging from the quasi ubiquitous mRNA expression of TTRAP in adult
mammals, its function may exceed an involvement in signaling by CD40 or
TNF-R75. TRAFs 2, 3, and 6 mRNAs are also widely expressed in adult
tissues (9, 11, 48), and mice deficient for each TRAF display severe
problems during embryogenesis, clearly extending the importance of the
latter signal transducers beyond the inflammatory response (8). The
expression level and pattern of TTRAP mRNA during murine
embryogenesis also suggests a role in development. For example, the
strong mRNA signal in the embryonic thymus points toward a
potential role for TTRAP in this organ.
Like the TRAFs, TTRAP binds to receptors of the TNF receptor family,
i.e. CD30, CD40, and TNF-R75. However, unlike TRAF3, it does
not associate with the Epstein-Barr virus protein LMP1. This
demonstrates that TTRAP does not bind aspecifically to any receptor
known to signal via TRAFs. To map the TTRAP binding site on CD40, we
tested several deletion mutants of the cytoplasmic domain of the
receptor and found the region between residues 230 and 245 to be
required for TTRAP interaction. This stretch of 16 amino acids contains
the TRAF6 binding motif, but is distinct from the site required for
association of CD40 with TRAFs 2 and 3 (11, 45). This suggests that
TTRAP and TRAF6 bind in close proximity or may even compete for the
same region of CD40.
The interaction of CD40 with TTRAP apparently involves a mechanism that
is different from what is known for the association of CD40 with TRAFs.
Indeed, TRAFs 2 and 3 bind to the receptor within minutes after cell
stimulation (49), whereas the recruitment of TTRAP to CD40 appears to
be slower, with a continuous increase in time up to at least 24 h.
Because in our experiments the TTRAP and CD40 protein levels do not
change significantly upon CD40L stimulation, the increase in CD40-TTRAP
interaction cannot result from an aspecific aggregation caused by the
overexpression of TTRAP and/or CD40. This suggests that there is a
CD40L-induced recruitment of TTRAP to CD40, which might involve
activation or synthesis of one or more cofactors that assist or
modulate the interaction. Alternatively, regulated proteolysis or
decreased binding affinity of other receptor-interacting proteins may
clear the way for TTRAP to form a complex with CD40.
TTRAP was isolated as a receptor-interacting protein, and therefore we
were surprised to find that it also interacted with several TRAFs. We
observed that TTRAP interacted more avidly with TRAF6 than with the
other TRAFs. It is therefore possible that TTRAP is linked more
specifically, but not exclusively, to TRAF6-mediated signaling events.
Given the fact that TRAF6 is involved in signal transduction mediated
by multiple receptors, i.e. CD40 (11), RANK (50, 51), Toll
(14, 15), and the IL-1 receptor (16), the scope of TTRAP action could
potentially be broader than shown by the results with CD40 and TNF-R75
reported here. Our observation that TTRAP partially inhibited NF-B
activation induced by IL-1 corroborates this possibility.
We have shown that TTRAP interacts with TRAF6 via the TRAF domain,
which consists of a TRAF-N and-C subdomain. The former is a
structurally conserved region that folds into an amphipathic helix that
is required for the trimerization of TRAFs by forming a coiled coil
with two other TRAF-N domains (52, 53). The TRAF-C domain is the most
conserved region in this family of proteins and was shown to be
involved in the direct interaction with different receptors, in
trimerization of TRAFs, and in the association with other TRAF-binding
proteins (8, 52, 53). Our experiments have shown that an intact TRAF-N
domain is needed for binding TTRAP. Other proteins have previously been
shown to require the TRAF-N domain for interaction with TRAFs,
including the regulatory factors A20 (25), TRIP (28), and the cIAPs
(54). Interestingly, TRAF2 can still bind to TNF-R75 when associated
with TRIP or cIAPs, yielding a triple complex. Whether this is also the
case with TTRAP remains to be investigated.
Recruitment of TTRAP to CD40 could either assist TRAFs and other
proteins in triggering the signaling cascade or could counteract signal
transduction to control cell stimulation with respect to duration and
strength. The fact that overexpression of TTRAP inhibits activation of
NF-B mediated by CD40, TNF-R75, TRAF2, and TRAF6 supports the latter
possibility. The inhibition by TTRAP may be the result of its
interaction with receptors and/or TRAFs, whereby it (sterically)
affects signal transduction. However, at this moment we cannot rule out
the possibility that TTRAP acts (also) downstream of receptors and
TRAFs. On the other hand, IKK and P65/RelA-mediated activation of
NF-B was not down-regulated in our assays, suggesting that TTRAP
inhibits processes upstream of IB-phosphorylation by IKK. NF-B
induction by NIK was also not significantly affected by TTRAP. In this
respect, the action of TTRAP resembles that of another inhibitor of
NF-B activation, A20 (55). Our results imply either that NIK is
downstream of TTRAP or that the pathway that is affected by TTRAP does
not involve NIK. Evidence for the existence of such alternative but
NIK-independent pathway stimulated by CD40 and involving TRAF6 was
presented recently (46). It remains to be established whether TTRAP
inhibits this particular signaling cascade.
Surprisingly, overexpression of TTRAP down-regulated NF-B activation
by the phorbol ester PMA. It is unclear how this activator of protein
kinase C stimulates a plethora of cascades in the cell, but the fact
that TTRAP did not prevent PMA-induced activation of the AP-1 reporter
indicates that TTRAP affects processes downstream of the bifurcation of
stimulatory pathways for NF-B and AP-1. This is again similar to
what was shown for A20 (55). On the other hand, TTRAP and A20 differ by
the fact that the effect of TTRAP depends on the receptor that is
triggered, whereas this is not the case for A20. Indeed, the latter
potently inhibits NF-B activation by CD40, TNF, or IL-1 (55),
whereas TTRAP had a more pronounced effect on stimulation by CD40L as
compared with TNF or IL-1. Therefore, TTRAP does not seem to regulate
all pathways involving TRAFs to the same extent. Signaling by TNF
(through TNF-R55) is mediated by direct binding of TRAFs to the adaptor protein TRADD rather than to this 55 kDa receptor. TRAFs do, however, contact the receptors CD40 and TNF-R75 directly, and maybe
overexpression of TTRAP affects this interaction more strongly than
TRAF-TRADD interaction. This could be related to the fact that TTRAP
does not bind to TRADD, whereas it does associate with CD40 and
TNF-R75. Taken together, our current data demonstrate that
overexpression of TTRAP results in a dose-dependent and
stimulus-dependent inhibition of NF-B.
Combining the observed inhibition of signal transduction with the
increased recruitment of TTRAP to CD40 after ligand stimulation, we
propose that TTRAP contributes to a negative feedback loop. Thus, by
association with receptors and signaling factors, the protein would
function to interfere progressively with gene activation, similar to
inhibitory Smads in the transforming growth factor- signaling
pathway (56). However, at this point we cannot exclude that TTRAP could
be a scaffold protein that tethers TRAFs, receptors, and maybe other
signaling factors in the cell. In that case, TTRAP overexpression could
also lead to decreased NF-B activation, because instead of bringing
the signal transducers together, it would separate them. Further
research will be required to discriminate whether TTRAP functions as
feedback inhibitor or scaffold protein in signaling by proteins of the
TNF receptor and TRAF family.
| |
ACKNOWLEDGEMENTS |
We thank V. Dixit, D. Goeddel, J. Inoue,
A. Israel, M. Karin, S. Plaisance, and M. Rowe for providing expression
plasmids. We are grateful to R. Brent for sending us yeast
strains, plasmids, and a cDNA library, which were used for
two-hybrid screening. We also thank W. Buurman for providing antibodies
and K. Thielemans for 3T6 (CD40L) cells.
| |
FOOTNOTES |
*
This work was supported by a postdoctoral fellowship of the
"Vlaams Instituut voor de Bevordering van het
Wetenschappelijk-Technologisch Onderzoek in de Industrie" (IWT) (to
S. P.) and by funds from Innogenetics S. A., and the Flanders
Interuniversitary Institute for Biotechnology, within the framework of
a collaboration agreement (1998-2000).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) AJ269473 and AJ251328.
Supported by the "Interuniversitaire Attractiepolen" (IUAP 9005097N).
Research associate with the "Fonds voor Wetenschappelijk
Onderzoek" (FWO).
§§
Supported by the Flanders Interuniversitary Institute for
Biotechnology. To whom correspondence should be addressed. Tel.: 32-16-345916; Fax: 32-16-345933, E-mail:
dhu@sgi.celgen.kuleuven.ac.be.
¶¶
Supported by the Flanders Interuniversitary Institute
for Biotechnology.
Published, JBC Papers in Press, April 11, 2000, DOI 10.1074/jbc.M000531200
| |
ABBREVIATIONS |
The abbreviations used are:
TNF, tumor necrosis
factor;
CCR4, carbon catabolite repressor protein;
HA, hemagglutinin (tag);
HUVEC, human umbilical vein endothelial cell;
IKK, IB-kinase;
IL, interleukin;
TRAF, TNF receptor-associated factor;
I-TRAF, TRAF-interacting protein;
JAK, Janus kinase;
LMP1, latent membrane
protein 1;
MAPK, mitogen-activated kinase;
MEKK1, MAPK/extracellular
response kinase;
NF-B, nuclear factor B;
NIK, NF-B-inducing
kinase;
PMA, phorbol 12-myristate 13-acetate;
RANK, receptor activator
of NF-B;
STAT, signal transducer and activator of transcription;
TAK1, transforming growth factor--activated kinase;
TANK, TRAF-associated NF-B activator;
TNF-R, TNF receptor;
TRADD, TNF-R1-associated death domain protein;
TRIP, TRAF-interacting protein;
TTRAP, TRAF and TNF receptor-associated protein;
EST, expressed
sequence tag;
Tricine, N-[2-hydroxy-1,1-bis(hydroxymethyl)ethyl]glycine.
| |
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TOP
ABSTRACT
INTRODUCTION
