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NEOPLASIA
From Georgetown University Medical Center, Washington,
DC.
The malignant Reed-Sternberg cell of Hodgkin disease is an aberrant
B cell that persists in an immunolgically mediated inflammatory infiltrate. Despite its nonproductive immunoglobulin genes, the Reed-Sternberg cell avoids the usual apoptotic fate of defective immune
cells through an unknown mechanism. A likely candidate is the surface
receptor, CD40, consistently expressed by Reed-Sternberg cells, and the
first link in the pathway to NF- The Reed-Sternberg (RS) cell of Hodgkin disease is
a malignant germinal center B cell1,2 with rearranged but
nonproductive immunoglobulin genes.1 However, through as
yet unknown mechanisms, RS cells resist the apoptotic fate normally
suffered by defective B cells with crippled immunoglobulin genes.
Intervention in this antiapoptotic mechanism might be an approach for
the development of targeted, pharmacologic management of
Hodgkin disease.
The RS cells survive and thrive in a milieu of an intense cellular
inflammatory infiltrate. A complex array of secreted factors and
surface receptors are elaborated by the RS cell to recruit and nurture
this infiltrate. The transcription factor, NF- In B cells, CD40 regulates the progression from immunoglobulin isotype
switch to cytokine secretion and, ultimately, terminates in
Fas-mediated apoptosis to shut down the immune
response.6-9 CD40 signal transduction pathways result in
transcriptional events: CD40 activates both NF- Proximal events in CD40-mediated transcription factor activation depend
on the family of TNFR-associated factors (TRAFs), especially TRAFs 2, 3, and 5.12-14 We have shown these genes to be expressed
in single RS cells from patient samples.15 These proteins
do not have enzymatic activity themselves but serve as adapters to
downstream kinases. Recently, more links in the pathway were
discovered: TRAF3 interaction with CD40 increases during CD40 ligation,
whereas TRAF2 binding decreases,16,17 the TRAFs bind to
TRAF-associated activator of NF- In an RS cell-derived line,23 we show that, following CD40
ligation, TRAF3 is degraded by a protease, thus removing the block in
NF- Cell culture
Isolation of membrane, cytosolic, and nuclear fractions
Electrophoretic mobility shift assay (EMSA) The nuclear pellet, isolated as described above, was resuspended in an equal volume of buffer C (20 mmol/L HEPES, pH 7.5, 20% glycerol, 0.42 mol/L NaCl, 1.5 mmol/L MgCl2, 0.2 mmol/L EDTA, 0.25 mmol/L DTT) supplemented with PMSF (0.5 mmol/L), pepstatin A (1 mg/mL), aprotinin (1 mg/mL), leupeptin (1 mg/mL), Na3VO4 (2 mmol/L), and NaF (10 mmol/L). Nuclei were lysed by vortexing for 30 minutes at 4°C followed by centrifugation at 10 000g for 45 minutes at 4°C. The supernatant containing nuclear protein was harvested and stored at 70°C. Ten nanograms of an oligonucleotide containing the NF- B
consensus sequence (Santa Cruz Biotechnologies, Santa Cruz, CA) was
end-labeled with 50 µCi  -32P-adenosine triphosphate
(NEN Life Science Products, Boston, MA), using T4 polynucleotide kinase
(Life Technologies) according to the manufacturer's instructions. The
radiolabeled probe was separated from unincorporated nucleotides by
passing it through a G-25 Sephadex spin column (Boehringer Mannheim,
Indianapolis, IN). One microgram of nuclear extract, in 2 µL of
buffer C, was combined with 0.1 ng of 32P-end-labeled
double-stranded DNA containing the NF-B consensus sequence in the
presence of 1.5 µg poly dI:dC (Sigma), 10 ng of an irrelevant
25-nucleotide single-stranded oligonucleotide, 12 mmol/L HEPES, pH 7.5, 1 mmol/L EDTA, 1 mmol/L 2-mercaptoethanol, 6% glycerol, 10 mmol/L KCl,
0.05 mmol/L DTT, 0.05 mmol/L PMSF, 0.1% NP-40 in a final volume of 10 µL. In competition experiments, an unlabeled oligonucleotide
containing either the wild-type or a mutant NF-B binding site (Santa
Cruz Biotechnologies) was added at 30-fold excess (3 ng). The mixture
was incubated at 25°C for 30 minutes, after which 1 mL of 1%
bromophenol blue dye was added. The sample was immediately loaded onto
a 4% polyacrylamide gel and separated by electrophoresis at 150 V for
1 hour. The gel was transferred to 3M Whatman paper and dried under
vacuum at 80°C, followed by autoradiography. Autoradiographs were
scanned using densitometry and evaluated with Quantity One software
(PDI, Huntington Station, NY) to quantitate fold-activation of
NF-B.
Western blotting TRAF3 was detected by immunoblotting with the H122 rabbit polyclonal antibody (Santa Cruz Biotechnologies) and goat antirabbit-horseradish peroxidase (HRP) conjugate. The Renaissance HRP substrate was applied (NEN Life Science Products) and the membrane was exposed to film (Eastman Kodak, Rochester, NY). The membrane was stripped by incubating in stripping buffer (60 mmol/L Tris, pH 6.8, 2% sodium dodecyl sulfate [SDS], 50 mmol/L 2-mercaptoethanol) for 30 minutes at 70°C with constant agitation. The stripped membrane was washed 5 times DPBS (Life Technologies) and 0.1% Tween-20. Membranes were then re-probed with either anti-CD40 antibody (Santa Cruz Biotechnologies), anti-CD30 antibody (BerH2; Dako Corporation, Carpentiera, CA), or antihuman glyceraldehyde-3-phosphate dehydrogenase (GAPDH) antibody (Trevigen, Inc, Gaithersburg, MD).Expression vectors and transfections The N-terminal deletion mutant of TRAF3 was constructed from the plasmid expression vector pSG5FLAGLAP1 (generous donation from Dr G. Mosialos, reference 25) containing the full-length human TRAF3 (F-TRAF3) complementary DNA (cDNA) by cleaving within the gene with BssH2 (Life Technologies) and Sfu1 (Boehringer Mannheim), which removed nucleotides 39 to 927. The 3'-recessed ends were filled in using the large (Klenow) fragment of DNA polymerase I (Life Technologies), according to the manufacturer's instructions. The plasmid DNA was recircularized with T4 DNA ligase (Life Technologies). This expression construct containing a TRAF3 deletion mutant, pSG5FLAGTRAF3 300 (here
called 300TRAF3) was replicated in Escherichia coli
strain DH5 (Life Technologies), and the plasmid DNA was isolated by
alkaline lysis and column purification procedure (Qiagen, Chatsworth,
CA). For stable transfection, F-TRAF3 or 300TRAF3 and the selectable
marker pSV2neo (Stratagene, La Jolla, CA) (4:1) were co-precipitated,
and resuspended at a concentration of 0.5 mg/mL. Ten micrograms of the
plasmid mix was added to 107 cells in 80 mL DPBS (Life
Technologies) and the mixture was placed into a Gene Pulser cuvette
(BioRad, Hercules, CA). The cells were electroporated at 200 mV, and
placed directly into 10-mL nonselective medium for 3 days, followed by
selection medium containing 250 µg/mL Geneticin (Life Technologies).
The medium was changed every 4 days until log-phase growth was
attained. The cells were then placed into culture medium containing 500 µg/mL Geneticin and split into 4 pools. Following additional
log-phase growth, expression of the transfected TRAF3 cDNA was
confirmed by Western blotting.
Radiolabeling and immunoprecipitation Cellular proteins were metabolically labeled by the addition of 40 µCi/mL 35S-EasyTag Labeling Mix (NEN Life Science Products) to KMH2 cells in culture without cysteine and methionine. The cells were cultured in the presence of the radiolabeled amino acids for 5 hours. CD40L (Immunex) was added during the last hour of incubation. So that labeling time did not vary between samples, the different time points of CD40L stimulation were separated into different flasks and stimulated such that all time points were harvested at the same time (ie, labeling began at time [0 hour:00 minute], stimulation of flask 1 began at 4:00, flask 2 at 4:30, flask 3 at 4:55, flask 4 left untreated, and all were harvested at 5:00). The cells were harvested in 1 mL lysis buffer (50 mmol/L HEPES, pH 7.5,10% glycerol,0.5% NP-40). Protein content was normalized to 2 mg. The protein and antibody were mixed with protein A Sepharose beads in 1 ml lysis buffer (50 mmol/L HEPES, pH 7.5,10% glycerol, 0.5% NP-40) under constant agitation at 4°C overnight. For untransfected KMH2 cells, the antihuman TRAF3 antibody H20 (Santa Cruz Biotechnologies) was used. For transfected KMH2 cell lines, the anti-FLAG monoclonal antibody M2 (Eastman Kodak) was used. The protein A Sepharose beads were washed 3 times with 1 mL lysis buffer and resuspended in 200 µL SOL buffer (50 mmol/L TEA-HCl, pH 7.4, 100 mmol/L NaCl, 2 mmol/L EDTA, 0.4% SDS, 2 mmol/L -mercaptoethanol). Samples were boiled for 2 minutes and
allowed to cool to 25°C, after which 4 µL of 0.5 mol/L
iodoacetamide was added. The beads were then pelleted and the
supernatant was added to 700 µL of lysis buffer with clean beads and
antihuman TANK antibody C20 (Santa Cruz Biotechnologies). Samples were
incubated at 4°C for 2 hours with constant agitation. Immune
complexes were separated on 10% SDS-ppolyacrylamide gel
electrophoresis (PAGE). The gel was dried onto Whatman 3M paper and
exposed to film (Eastman Kodak) using the BioMax TranScreen LE
intensifying screen (Eastman Kodak).
Quantitative reverse transcriptase-polymerase chain reaction (RT-PCR) Cells were lysed in Trizol reagent (Life Technologies) and RNA was isolated according to the manufacturer's instructions. cDNA was generated from the RNA by reverse transcription. Briefly, 1 µg of total RNA was denatured in the presence of random hexamer primers by heating at 70°C. A mixture of 10 mmol/L dNTPs was added to the denatured RNA and primers. The reverse transcription was performed with Superscript II RT enzyme (Life Technologies) in a final reaction volume of 20 µL according to the manufacturer's recommendations. The interleukin (IL)-6 gene expression was quantitated using the IL-6 PCR-MIMIC kit (Clontech, Palo Alto, CA) with the IL-6 amplimer set according to the manufacturer's protocol. Briefly, the PCR mixture contained 0.2 pmol/µL of each IL-6 primer, 1 mmol/L dNTPs, 20 mmol/L Tris-HCl (pH 8.4), 50 mmol/L KCl, 1.5 mmol/L MgCl2, 1 µL of the MIMIC dilution, 1 µL of the above RT reaction mixture, and 2.5 U Taq DNA polymerase in a final volume of 50 µL. Thermal cycling was carried out as follows: 1 cycle of 94°C for 3 minutes, 60°C for 1 minute, 72°C for 1 minute, followed by 34 cycles of 94°C for 30 seconds, 60°C for 45 seconds, 72°C for 30 seconds, and an additional extension period at 72°C for 5 minutes. For actin PCR, the following primer pair used: 5'-GAACGGTGAAGG TGACAG CAG T-3', 5'-TGGGGGACAAAAAGG GGGAAG G-3'.
TRAF 3 depletion precedes NF- B is a known consequence of CD40 ligation,
resulting in the nuclear translocation of the p50/p65 dimer and c-Rel
proteins.26 CD40 ligation in KMH2 cells causes increased cell survival and secretion of NF-B-dependent cytokines such as
IL-8.27,28 We determined the time-course of activation of NF-B in stimulated KMH2 cells. As shown in Figure
1A, no change in DNA binding activity of
NF-B activity was noted within 5 minutes, but activity increased at
30 minutes and reached a maximum level (~2.2-fold unstimulated) by 1 hour after CD40 ligation.
In looking at TRAF3 levels within this time period, there was a notable
decline in the total level of endogenous TRAF3 protein in KMH2 cells
within 5 minutes of stimulation of CD40 by its ligand (Figure 1B).
Depletion of TRAF3 continued for the duration of the study (1 hour). We
asked whether TRAF3 is in the membrane and if changes in the protein
level could be detected in the membrane and/or cytosolic component(s)
of TRAF3 following CD40 ligation. By Western blotting, TRAF3 was
observed in the membrane fraction of unstimulated cells and there was
no significant change in the level of membrane-associated TRAF 3 on
activation of CD40 within 1 hour (Figure 1C). In contrast, a decrease
in the cytoplasmic pool of TRAF 3 occurred within 5 minutes and
cytosolic TRAF3 levels continued to decline for at least up to 1 hour
of CD40 stimulation (Figure 1D). Because membrane content of TRAF3 did
not change at these time points (5 minutes to 1 hour), depletion of the
cytosolic pool of TRAF3 did not correlate with its otherwise
anticipated translocation to the membrane. In Figure 1B-C, the level of
the "housekeeping" enzyme GAPDH is detected to demonstrate equal
protein content in each lane. In Figure 1D, the membrane-bound CD30 is used for this purpose. These results suggested that CD40 ligation resulted in rapid elimination of the cytosolic TRAF3 in KMH2 cells. These data indicate that CD40 ligation results in depletion of TRAF3,
followed by NF- CD40-generated signals are blocked by a protease inhibitor We hypothesized that depletion of TRAF3 following CD40 ligation may be due to activation of a protease(s) in KMH2 cells, and protease inhibition may then restore the level of TRAF3 in stimulated cells. Several different classes of protease inhibitors (serine-aprotinin, leupeptin, PMSF; thiol-leupeptin, PMSF; lysosomal-ALLN; and acid/aspartate-pepstatin A, ritonavir, indinavir) were tested for their ability to protect TRAF3 in stimulated KMH2 cells. Treatment with the aspartate protease inhibitor, pepstatin A, resulted in the partial restoration of TRAF3 level in CD40L-treated cells (Figure 2A). Under the conditions of the experiment, none of other inhibitors had any effect on CD40-induced depletion of TRAF3 in these cells (data not shown), including the 2 other aspartate protease inhibitors, ritonavir and indinavir (Figure 2B). This indicates that partial recovery of TRAF3 observed in the presence of pepstatin A was not due to nonspecific effects of a protease inhibitor on CD40L binding or CD40 stimulation. Pepstatin A treatment also caused the marked inhibition of NF-B activity in
CD40-stimulated KMH2 cells (Figure 3A,B).
Taken together, these data suggest a role of a protease(s) in CD40
signaling leading to NF-B activation.
A TRAF3 amino-terminus deletion mutant is resistant to
CD40-mediated degradation and blocks NF- B activation. An expression vector (pSG5) containing FLAG-tagged
F-TRAF3 cDNA25 was used to construct the amino-terminus
deletion mutant of TRAF3 cDNA (300TRAF 3) similar to the previously
reported dominant negative TRAF3 mutant14 as explained in
"Materials and methods." KMH2 cells were stably cotransfected with
F-TRAF3, 300TRAF3, and a selectable marker pSV2neo plasmid DNA, or
control vector pSV2neo alone. Expression of the epitope-tagged TRAF3
protein was examined at various times following CD40 stimulation
(Figure 4). In the first experiment, the
FLAG-tagged F-TRAF3 construct was selectively immunoprecipitated with
anti-FLAG antibody to distinguish it from endogenous TRAF3. The
immunoprecipitate was then immunoblotted with anti-TRAF3 antibody. Although F-TRAF3 was degraded after CD40 ligation (Figure 4A,B), the
deletion mutant (300TRAF3, aa13-aa310) appeared to be resistant to
degradation (Figure 4C,D). The presence of 300TRAF3, however, did
not prevent degradation of the endogenous TRAF3 protein in 300TRAF3
transfectants (Figure 4C,D). In these experiments, TRAF3 was detected
by immunoblotting total protein samples because its molecular size
distinguishes it from endogenous TRAF3. These data imply that the
amino-terminus of TRAF3 is a potential target site for proteolytic
degradation following CD40 stimulation.
To address the possibility of a negative regulatory effect of the
nondegradable TRAF3 deletion mutant on CD40 signaling, DNA binding
activity of NF-
We next sought to determine a molecular mechanism for the inhibitory
properties of TRAF 3 in the CD40 pathway. Figure 4 demonstrates that a
deletion mutant of TRAF3 ( Sustained interaction between TANK and a nondegradable TRAF 3 deletion mutant ( B activation. Thus, lack of detection of TANK in TRAF3
immunoprecipitates can be attributed to the unavailability of TRAF3 in
CD40-stimulated cells. To rule out the possibility that the TANK level
may have decreased in response to CD40 stimulation, we measured the
expression of TANK in KMH2 cells at various times after ligation. The
total level of TANK remained constant for at least up to 60 minutes
after CD40 stimulation of KMH2 cells (data not shown). 300TRAF3 was found to associate with TANK, as demonstrated by immunoprecipitation of
the N-terminal FLAG epitope tag on 300TRAF3, followed by
immunoprecipitation of TANK (Figure 6A). The association between
300TRAF3 and TANK decreased to a much lesser extent than occurred
with the endogenous TRAF3 throughout 1 hour of CD40 ligation. Seventy
percent of TANK bound in the unstimulated state remained bound to
300TRAF3 after 1 hour of CD40 ligation (Figure 6B). As a control,
interaction between TANK and F-TRAF3 was found to parallel that with
endogenous TRAF3. That is, TANK interaction with F-TRAF3 declined with
CD40 stimulation so that only one tenth of the original amount of TANK remained bound to F-TRAF3 by 1 hour of CD40 ligation (data not shown).
Taken together, these data imply that physical sequestration of TANK by
TRAF3 serves as a regulatory mechanism in resting cells and degradation
of TRAF3 following CD40 stimulation may be critical to the role of TANK
as a key mediator of NF-B activity.
Nondegradable deletion mutant ( 300TRAF3 transfectants. An NF-B binding
site exists in the promotor of the IL-6 gene29
and IL-6 is known to be up-regulated in response to CD40 ligation in
KMH2 cells.28 We quantified the magnitude of CD40-mediated
regulation of this gene in the F-TRAF3 and 300TRAF3 transfectants by
RT-PCR. The quantitative RT-PCR method uses a known titration of a
size-modified IL-6 competitor DNA to measure the amount of IL-6 cDNA in
a sample. By this method, it was evident that the IL-6 gene
transcription was up-regulated by approximately 5-fold in vector and
F-TRAF3 transfectants after 3 hours of CD40 ligation (Figure
7A,C and data not shown), whereas IL-6 RNA levels remained unchanged in 300TRAF3 transfectants in the same time period (Figure 7B,C). Therefore, the nondegradable 300TRAF3 mutant inhibited CD40-mediated up-regulation of the IL-6 gene, while maintaining
interaction with the TANK protein.
The CD40-NF- Initial studies suggest that the mutation in I- One prior study failed to demonstrate an increase in NF- Significantly, we found that NF- We have found a novel role of TRAF3 in Hodgkin cells: the cytoplasmic
pool of TRAF3 was eliminated prior to NF-
This action of TRAF3 in the cytoplasm is distinct from its role when
associated with the membrane-bound CD40 cytoplasmic tail. CD40 is able
to stimulate NF- Abrogation of both CD40-mediated TRAF3 degradation and NF- We have demonstrated that transfection of the F-TRAF3 does not inhibit
NF- The next link in the pathway toward NF- CD40-mediated NF-
We thank Dr Hiroshi Kamesaki for the KMH2 cell line, Dr G. Mosialos for the expression vector containing epitope-tagged full-length TRAF3 cDNA (pSG5FLAGLAP1) and Immunex Corporation for the purified human CD40 ligand.
Submitted January 11, 2000; accepted May 29, 2000.
Supported by the American Cancer Society (grant no. DHP112 to J.C.) and the O. Benwood Hunter Endowment.
Correspondence: Jeffrey Cossman, Georgetown University Medical Center, NW 103 Medical-Dental Bldg, 3900 Reservoir Rd, NW, Washington, DC 20007; e-mail: cossmanj{at}gunet.georgetown.edu.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
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S. Fujioka, C. Schmidt, G. M. Sclabas, Z. Li, H. Pelicano, B. Peng, A. Yao, J. Niu, W. Zhang, D. B. Evans, et al. Stabilization of p53 Is a Novel Mechanism for Proapoptotic Function of NF-{kappa}B J. Biol. Chem., June 25, 2004; 279(26): 27549 - 27559. [Abstract] [Full Text] [PDF]
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B. Zheng, P. Fiumara, Y. V. Li, G. Georgakis, V. Snell, M. Younes, J. N. Vauthey, A. Carbone, and A. Younes MEK/ERK pathway is aberrantly active in Hodgkin disease: a signaling pathway shared by CD30, CD40, and RANK that regulates cell proliferation and survival Blood, August 1, 2003; 102(3): 1019 - 1027. [Abstract] [Full Text] [PDF]
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B. F. Skinnider and T. W. Mak The role of cytokines in classical Hodgkin lymphoma Blood, May 29, 2002; 99(12): 4283 - 4297. [Abstract] [Full Text] [PDF]
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A. Gruber, J. C. Wheat, K. L. Kuhen, D. J. Looney, and F. Wong-Staal Differential Effects of HIV-1 Protease Inhibitors on Dendritic Cell Immunophenotype and Function J. Biol. Chem., December 14, 2001; 276(51): 47840 - 47843. [Abstract] [Full Text] [PDF]
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B
pathway by a protease inhibitor
Top
Abstract
Introduction
represents the level
of the transfected F-TRAF3 protein. (C) Stable KMH2 transfectants
expressing the deletion mutant of TRAF3 (
represents the
endogenous, full-length TRAF3. Unstim indicates unstimulated; IP,
immunoprecipitated; IB, immunoblotted.
