Originally published In Press as doi:10.1074/jbc.M202485200 on April 25, 2002
J. Biol. Chem., Vol. 277, Issue 26, 23420-23426, June 28, 2002
Convergence of Signaling Pathways on the Activation of ERK in
B Cells*
Anand
Jacob
,
Damon
Cooney,
Madhura
Pradhan§¶, and
K. Mark
Coggeshall
From the Oklahoma Medical Research Foundation,
Immunobiology and Cancer Program, Oklahoma City, Oklahoma 73104 and
§ Department of Microbiology, Ohio State University,
Columbus, Ohio 43210
Received for publication, March 14, 2002
 |
ABSTRACT |
The B cell receptor (BCR) initiates
three major signaling pathways: the Ras pathway, which leads to
extracellular signal-regulated kinase (ERK) activation; the
phospholipase C-
pathway, which causes calcium mobilization; and the
phosphoinositide 3-kinase (PI 3-kinase) pathway. These combine to
induce different biological responses depending on the context of the
BCR signal. Both the Ras and PI 3-kinase pathways are important for B
cell development and activation. Several model systems show evidence of
cross-regulation between these pathways. Here we demonstrate through
the use of PI 3-kinase inhibitors and a dominant-negative PI 3-kinase
construct that the BCR-induced phosphorylation and activation of ERK is dependent on PI 3-kinase. PI 3-kinase feeds into the Ras signaling cascade at multiple points, both upstream and downstream of Ras. We
also show that ERK activation is dependent on phospholipase C-, in
keeping with its dependence on calcium mobilization. Last, the
activation of PI 3-kinase itself is completely dependent on Ras. We
conclude that the PI 3-kinase and Ras signaling cascades are intimately
connected in B cells and that the activation of ERK is a signal
integration point, since it requires simultaneous input from all three
major signaling pathways.
| |
INTRODUCTION |
Triggering the B cell antigen receptor
(BCR)1 by antigen or
polyclonal activators initiates signaling cascades that lead to various
cellular responses (1). Receptor ligation is followed by the
phosphorylation of the immunoreceptor tyrosine-based activation motifs
(2-4), which recruit cytosolic proteins and enzymes. Receptor recruitment brings enzymes into proximity of their substrates or
kinases, which permits the sequential reactions that form the basis of
signaling cascades. Three such cascades stimulated by immunoreceptors
involve Ras, phosphoinositide 3-kinase (PI 3-kinase), and phospholipase
C- (PLC-) (reviewed in Ref. 1).
The activation of PI 3-kinases results in the rapid accumulation of
D-3 phosphorylated inositol phospholipids in the cell membrane
(5). PI 3-kinase products bind with high specificity to pleckstrin
homology domains of signaling proteins, to recruit pleckstrin homology
domain-containing enzymes to the plasma membrane and promote their
subsequent activation (6, 7). Class IA PI 3-kinases, the major class
induced by tyrosine kinase-dependent receptors (6) consist
of an SH2 domain-containing adapter p85 subunit that is constitutively
bound to a catalytic p110 subunit. Animals lacking the p85 isoform
p85
show a defect in B cell development, and mature B cells from
these animals are impaired in their response to anti-IgM (8, 9).
The activation of Ras requires the membrane localization of a guanine
nucleotide exchange factor (GEF) such as Sos (10). In growth
factor-stimulated cells, Sos translocation is mediated by the adapter
proteins, Grb2 and Shc (11). BCR triggering causes the association of
Sos with the adaptors Shc and Grb2 (12-14). The ternary complex of
Shc, Grb2, and Sos is associated with the plasma membrane after BCR
triggering, consistent with an essential role for the adapter proteins.
GTP-bound Ras causes membrane recruitment of the protein kinase Raf,
which is followed by its phosphorylation by the kinase PAK (15) and by
Src family tyrosine kinases (16). Activated Raf binds to and activates
MEK1 and MEK2, which in turn activate the MAP kinases ERK1 and ERK2.
The duration of ERK activation induced by receptors can affect signal
outcome (17). Thus, growth factor-stimulated fibroblasts require a
sustained low level of ERK activation for progression through the
G1 phase. Conversely, transient ERK activity of high
amplitude causes G1 arrest (17). The activation of MEK and
ERK in B cells is also dependent on calcium flux (18), but the
mechanism(s) involved are unexplored.
Despite the importance of Ras and ERK activation for B cell development
and activation (19, 20), the pathways that lead to the induction of Ras
by BCR have not been closely investigated. For example, the requirement
for Shc and Grb2 has not been directly tested.
Although signaling cascades involving Ras, PI 3-kinase, and PLC- are
generally thought to be independent of each other, some reports
indicate cross-talk between these pathways. For example, full
activation of PI 3-kinase in growth factor-stimulated fibroblasts showed a requirement for an interaction between active GTP-bound Ras
and p110 (21-23). Likewise, assembly of a membrane-associated signaling complex containing PLC-, the adapter BLNK, and the tyrosine kinases Btk (Bruton's tyrosine
kinase) and Syk allows activation of PLC- and the
subsequent rise in intracellular calcium and the activation of protein
kinase C (24). PI 3-kinase products are required for the recruitment
and activation of Btk and may also contribute to the recruitment and/or
allosteric regulation of PLC- itself (25, 26). Consequently,
intracellular calcium flux is partially dependent on PI 3-kinase
activity (27, 28).
PI 3-kinase might also contribute to the activation of ERK. In
fibroblasts, the induction of ERK by low doses of growth factor is
dependent on PI 3-kinase (29, 30). In Jurkat T cells, ERK activation by
T cell receptor is dependent on PI 3-kinase (31). Class IB PI 3-kinase
p110 has been shown to be necessary for ERK activation by
G-protein-coupled receptors (32). A mutant of p110 that lacks lipid
kinase activity but retains protein kinase activity (33, 34) was shown
to activate ERK but not Akt (33).
Given the central importance of Ras and ERK in B cell antigen
receptor-induced proliferation and development, we examined in greater
detail the events that lead to ERK activation. Our broader aim was also
to determine whether there is cross-talk between the PI 3-kinase and
the Ras pathway in BCR signal transduction. Our results indicate that
this is indeed the case. We used different methods to inhibit PI
3-kinase signaling and observed that ERK activation is correspondingly
blocked. This influence of PI 3-kinase on ERK is independent of
intracellular calcium mobilization. Additional experiments show that PI
3-kinase influences the Ras cascade both upstream and downstream of Ras
itself. Finally, we show that Ras is required for the activation of PI
3-kinase, as it is in fibroblasts (21-23). Taken together, our results
demonstrate that the PI 3-kinase and Ras pathways in B cells are
intimately connected at several levels.
| |
EXPERIMENTAL PROCEDURES |
Cells and Cell Lines--
Splenic B cells were prepared from the
spleens of 5-8-week-old male BALB/cByJ mice (Jackson Laboratories) as
described earlier (35). In brief, erythrocytes were removed by osmotic
lysis, and T cells were removed by incubation with anti-Thy 1.2 followed by guinea pig complement serum. The resulting population is
85-95% sIg+ FcRII+. The murine B cell
lymphoma A20 and its FcRII-deficient derivative IIA1.6 were
maintained at 37 °C in RPMI 1640 (ICN) containing 10% fetal bovine
serum (Invitrogen), 50 µM 2-mercaptoethanol, and antibiotics.
Antibodies and Reagents--
Anti-ERK2(C-14), anti-Grb2, and
anti-MEK1 were purchased from Santa Cruz Biotechnology, Inc. (Santa
Cruz, CA); anti-HA (high affinity) was from Roche Molecular
Biochemicals; F(ab')2 rabbit anti-mouse IgG (H + L) was
from Pierce; anti-Shc was from Upstate Biotechnology, Inc. (Lake
Placid, NY); anti-Sos was a rabbit antiserum described previously (36);
and anti-phospho-ERK (E10 mouse monoclonal antibody), anti-phospho-MEK
(S217/221), anti-phospho-Akt (Ser473), and
anti-phospho-Akt (Thr308) were from Cell Signaling.
Anti-Ras was the anti-pan-Ras (Ab-3) monoclonal antibody from Oncogene
Research Products. Anti-rabbit horseradish peroxidase was purchased
from Amersham Biosciences, and all other horseradish peroxidase-linked
secondary reagents were from Kirkegaard and Perry Laboratories. For the
anti-Ras immunoblot, an anti-mouse IgG () secondary antibody was
used to avoid detection of the endogenous light chain in the whole lysate. Ionomycin (free acid), U73122, PD98059, and PMA were purchased
from Calbiochem; LY294002 and wortmannin were from Sigma, and Fluo-4/AM
was from Molecular Probes, Inc. (Eugene, OR).
[-32P]ATP (3000 µCi/mmol) was purchased from
PerkinElmer Life Sciences. GST-Grb2 has been described elsewhere (35).
His-tagged kinase-inactive ERK2 DNA was obtained from Dr. Walter Kolch
(University of Glasgow, Glasgow, UK), and the His-ERK2 fusion protein
was prepared as described earlier (37). GST-Raf-RBD in pGEX was
obtained from Dr. David Shalloway (Cornell University, New York, NY),
and the fusion protein was prepared as described elsewhere (38).
DNA Constructs--
V12Ras (oncogenic Ras) in pEF was obtained
from Dr. Andrew Thorburn (Huntsman Cancer Institute, Salt Lake City,
UT) and is described elsewhere (39); N17Ras in pEFneo was obtained from Dr. Erich Gulbins (Department of Immunology, St. Jude Children's Research Hospital, Memphis, TN); HA-Akt in pSG5 was obtained from Dr.
David Stokoe, University of California at San Francisco (40) and
subcloned into pEFneo with EcoRI and XbaI; Shc
Y239F/Y240F/Y317F was obtained from Dr. Ben Margolis (University
of Michigan Medical School, Ann Arbor, MI) (41); GST-ERK2 in pEBG and
Grb2R86K in pEBB were from Dr. Bruce Mayer (Howard Hughes Medical
Institute, Children's Hospital, Boston, MA) (42); and
p85
inter-SH2N in pSG5 was obtained from Dr. Julian Downward
(Imperial Cancer Research Fund, London, UK) and subcloned into
pEF1/myc-HisA(Invitrogen) with EcoRI and orientation of the
insert confirmed by sequencing. All the constructs in these plasmids
are driven by the EF-1 promoter with the exception of Shc
Y239F/Y240F/Y317F, which is in the retroviral expression vector
pBabe-Myc (41).
Stimulations--
For immunoprecipitations, 10 × 106 cells were washed and resuspended in 100 µl of
Hanks' balanced salt solution and stimulated at 37 °C with
15-20 µg/ml F(ab')2 rabbit anti-mouse IgG (H + L) and
lysed in ice-cold TN-1 buffer (125 mM NaCl, 50 mM Tris, pH 8, 10 mM EDTA, 10 mM
Na4P2O7, 10 mM NaF, and
1% Triton X-100) containing 3 mM activated
Na3VO4, 10 µg/ml aprotinin, 25 µg/ml leupeptin, 100 µg/ml phenylmethylsulfonyl fluoride, and, for
anti-HA-Akt immunoprecipitations, 1 µg/ml microcystin-LR. For
spectrofluorometric measurements, 1-2 × 106
loaded cells were resuspended in 1 ml of Hanks' balanced salt solution. Stimulating reagents were added directly to the
cuvette. PMA was added to 20 ng/ml for 10 min at 37 °C. wortmannin
and LY294002 were added to equilibrated cells for 10 min at 37 °C; U73122 was added for 30-40 s prior to stimulation.
Immunoprecipitations, Affinity Precipitations, and
Immunoblotting--
Cleared lysate was incubated overnight on a rocker
at 4 °C with 2-3 µg of immunoprecipitating antibody/ml. Protein
A/G-Sepharose was added for 1 h, and immune complexes were washed
five times in lysis buffer and eluted with SDS sample buffer. For whole
lysate preparation, 107 splenic B cells were resuspended in
100 µl, stimulated, and lysed with an equal volume of 2× lysis
buffer, and the cleared lysates were boiled with 5× SDS sample buffer
(1× SDS sample buffer: 65 mM Tris-HCl, 10% glycerol, and
2.3% SDS). Affinity precipitation of Shc with GST-Grb2 was carried out
as described earlier (35). Boiled samples were analyzed by SDS-PAGE and
transferred to nitrocellulose, and the membranes were blocked for
1 h at room temperature in 5% nonfat milk or 1% gelatin in
Tris-buffered saline-Tween. The membranes were incubated at 0.5-1
µg/ml primary antibody overnight at 4 °C, washed, and incubated
with the appropriate horseradish peroxidase-linked secondary reagent
for 40 min at room temperature. The Pierce SuperSignal ECL kit was used
to develop the membranes, and images were captured on a Roche
LumiImager. Where necessary, the bands were quantitated using
ImageQuant software.
ERK and Akt in Vitro Kinase Assays--
In vitro
kinase assays for ERK-2 and HA-Akt were performed essentially as
described earlier (35, 43). In brief, cells were lysed in TN-1 lysis
buffer, and cleared supernatants were incubated with 2-4 µg of
anti-HA or anti-ERK for 2 h followed by incubation with protein
A/G-Sepharose for 1 h. Immune complexes were washed 4-6 times in
lysis buffer and twice in assay buffer (20 mM MOPS, pH 7.2, 25 mM sodium glycerophosphate, 1 mM activated Na3VO4, 1 mM dithiothreitol), and
resuspended in the latter. To this suspension 10-20 µCi of
[-32P]ATP was added along with 10-20 µg of histone
H2B for Akt and myelin basic protein for ERK. After incubation
at 30 °C for 10-20 min, the reactions were stopped by the addition
of 5× sample buffer. The supernatants were analyzed by SDS-PAGE and
transfer to nitrocellulose, and the substrates quantitated using a
Molecular Dynamics Storm system or by Coomassie staining to visualize
the substrate followed by liquid scintillation counting of the excised bands.
MEK1 in Vitro Kinase Assay--
A modification of the assay
described in Ref. 44 was used. Cells were lysed in radioimmune
precipitation lysis buffer (150 mM NaCl, 50 mM
Tris, pH 8.0, 10 mM EDTA, 10 mM NaF, 10 mM Na4P2O7, 1% Triton
X-100, 0.5% sodium deoxycholate, and 0.1% SDS), and MEK1 was
immunoprecipitated overnight. Immune complexes were washed three times
in radioimmune precipitation buffer and twice in kinase buffer (100 mM 
-glycerophosphate, 160 mM HEPES, pH 7.2, 200 µM sodium vanadate, 40 mM
MgCl2). The beads were incubated in 30 µl of kinase
buffer at 30 °C for 30 min with 10 µg of kinase-inactive ERK2 and
4000 dpm/pmol [-32P]ATP (166 µM) with
gentle agitation. Substrate was analyzed as detailed above. The
specificity of phosphorylation was confirmed by blocking the reaction
with the MEK inhibitor PD98059.
Ras Assay--
The assay was performed essentially as described
in Ref. 38. Briefly, the day prior to the experiment, GST-Raf-RBD beads and GST control beads were prepared. The freshness of the fusion protein was found to be critical to the success of the experiment, so
the beads were not stored for more than 48 h at 4 °C. Cells were stimulated and treated as described earlier and lysed, and Ras-GTP
was precipitated from the lysates using the GST-Raf-RBD beads. The
precipitated Ras was detected by immunoblot with the anti-pan-Ras
(Ab-3) monoclonal antibody. The immunoblots were quantitated using a
Roche LumiImager. Samples were run in triplicate or quadruplicate.
The experiment shown in Fig. 5 is a "blinded" trial in which the
tubes were relabeled by a colleague after the postnuclear spin. The
identity of the samples was revealed at the end of the experiment.
Transient Transfections--
A20 and its derivatives were
transfected as described in Ref. 45. 1 × 107 cells
were electroporated with plasmid DNA in a 4-mm gap cuvette containing
warm RPMI, using a Bio-Rad GenePulser at 310 V and 960 microfarads. 5 µg of GST-ERK or HA-Akt DNA, 25-50 µg of Shc Y239F/Y240F/Y317F or Grb2R86K DNA, 25 µg of V12Ras or N17Ras
DNA, and 5-50 µg of p85inter-SH2 DNA was added to each cuvette,
depending on the experiment. The cells were resuspended in 8-10 ml of
warm growth medium. Stimulations and immunoprecipitations were
performed as above after incubation overnight at 37 °C in an
incubator. To normalize for protein expression, whole lysates of the
transfected cells were run in parallel and subjected to Western blot
with anti-HA (in the case of HA-Akt) or anti-GST (in the case of
GST-ERK). In some cases, the nitrocellulose used for the in
vitro kinase assay itself was cut, and the top half was subjected
to Western blot.
Measurement of Intracellular Calcium--
Cells were washed and
resuspended in growth medium (1 × 107/ml) and loaded
with 5 µM Fluo-4/AM for 30 min at 37 °C. The cells were washed, resuspended in growth medium without phenol red, and
excited at 495 nm in a PerkinElmer Life Sciences LS50B luminescence spectrometer using a stirred cuvette maintained at 37 °C. The emission was measured at 516 nm. The intracellular calcium
concentration was calculated using the formula [Ca2+] = Kd (F 
Fmin)/(Fmax Fmin). F represents the instantaneous fluorescence reading of the loaded cells. Fmax,
the fluorescence of the indicator when saturated with calcium, was
obtained by lysing the cells with Triton X-100, and
Fmin, the fluorescence in the absence of
calcium, was obtained by the subsequent addition of EGTA. The
Kd of Fluo-4 as given by the manufacturer is 345 nM.
| |
RESULTS |
Activation of ERK by the BCR Requires PI 3-Kinase Activity--
We
treated murine splenic B cells with F(ab')2 anti-Ig to
stimulate the BCR and examined the resulting phosphorylation of ERK in
the presence of the PI 3-kinase inhibitor LY294002 or carrier alone. As
seen in Fig. 1A, ERK
phosphorylation in carrier-treated B cells peaks within 1 min of
stimulation and is still above base line at 30 min. In cells pretreated
with LY294002, ERK phosphorylation is greatly reduced and peaks much
later, around 5 min. Fig. 1B shows that the use of
wortmannin, another PI 3-kinase inhibitor, has the same effect on ERK
phosphorylation. The inhibition of PI 3-kinase is demonstrated by the
lack of Akt phosphorylation in the presence of these compounds (Fig.
1B, bottom panel). At these
concentrations, both compounds are reported to be highly specific for
PI 3-kinase (46, 47). Note that in Fig. 1, A and
B, the different secondary reagents used in the immunoblot detect the endogenous B cell immunoglobulin heavy and light chains that
are expressed on the cells used in the experiments. The equal intensity
of these bands across all lanes demonstrates equivalent loading of the
cell lysates.
View larger version (34K):
[in this window]
[in a new window]
|
Fig. 1.
ERK activation by the B cell receptor is
sensitive to inhibition of PI 3-kinase. A, B cells were
isolated from the spleens of male Balb/c ByJ mice, preincubated with
the carrier Me2SO (lanes 2-6) or the
PI 3-kinase inhibitor LY294002 at 10 µM (lanes
7-11), and stimulated with F(ab')2 rabbit
anti-mouse Ig for varying lengths of time. The presence of
phosphorylated ERK in whole lysates was detected by immunoblot with
anti-phospho-ERK antibody. The position of phosphorylated ERK
(p-ERK1 and p-ERK2) and the endogenous
immunoglobulin heavy chain (Ig H) is indicated. The
first lane contains unstimulated cells, and the
last lane contains cells stimulated for 10 min
with 20 ng/ml PMA; they represent background and maximal ERK
phosphorylation, respectively. B, B cells were isolated as
in A and pretreated with the carrier or the indicated
concentrations of the PI 3-kinase inhibitors LY294002 (LY)
or wortmannin (Wtm) and then stimulated with
F(ab')2 rabbit anti-mouse Ig for 2 min. Whole lysates were
prepared, and aliquots run in parallel were immunoblotted for
phospho-ERK (top panel) or phospho-Akt
(p-Akt; bottom panel). The positions
of these proteins and of endogenous immunoglobulin light chain (Ig L
chain) are indicated. The first and last
lanes are the controls described for A. C, B cells were isolated from the spleens of male BALB/c ByJ
or male C57 BL/6 mice, stimulated as in B in the presence or
absence of 10 µM LY294002, and the activity of
immunoprecipitated ERK2 was determined by in vitro kinase
assay. The average of three trials is plotted as a percentage of
activity in the stimulated samples. Black bars,
C57/BL6; gray bars, Balb/cByJ mice.
Error bars represent S.D.
|
|
We also directly measured ERK activity by in vitro kinase
assay (Fig. 1C). For these experiments, splenic B cells from
male BALB/cByJ and C57/BL6 mice were isolated and preincubated with the
PI 3-kinase inhibitors LY294002 or carrier and stimulated with
F(ab')2 anti-mouse Ig. The activity of immunoprecipitated ERK2 was assayed in vitro. Fig. 1C represents the
average values from three independent experiments done with B cells
from both BALB/c ByJ and C57/BL6 mice. Preincubation of the B cells
with 10 µM LY294002 completely inhibits the activation of
ERK. The PI 3-kinase inhibitor had no direct affect on ERK in the
in vitro kinase reaction, ruling out the possibility that it
directly inactivates ERK.
The data shown in Fig. 1 suggest that PI 3-kinase is required for the
phosphorylation and activation of ERK in response to BCR ligation. To
confirm this observation, we transfected the murine B cell line A20
with a GST-tagged ERK2 reporter in combination with p85inter-SH2.
The latter is a mutant construct of the PI 3-kinase regulatory subunit
p85 lacking the minimal binding site for the catalytic subunit p110.
This mutant has been used to block PI 3-kinase signaling in a
dominant-negative fashion (31). Fig. 2
shows that p85inter-SH2 inhibits GST-ERK activation by BCR in a
dose-dependent manner. Together with the inhibitor studies shown in Fig. 1, the data indicate that the induction of ERK by the B
cell antigen receptor requires PI 3-kinase activity.
View larger version (12K):
[in this window]
[in a new window]
|
Fig. 2.
ERK activation in B cells is inhibited by
p85inter-SH2. A20 cells were
electroporated with GST-ERK, in combination with a 10-fold excess of
vector (0) or with p85inter-SH2 cDNA added in the
same amount (1), in 2-fold excess (2), or in
10-fold excess (10). The kinase activity of anti-GST
immunoprecipitates was determined by in vitro ERK kinase
assay and normalized to the expression of GST-ERK protein.
White bars, activity in unstimulated cells;
black bars, -fold increase in samples treated for
2 min with F(ab')2 rabbit anti-mouse Ig. The average of two
trials is shown. Error bars represent S.D.
|
|
The assembly of the Shc-Grb2-Sos Complex Is Unaffected by PI
3-Kinase Inhibition--
To examine which of the steps in the cascade
from antigen receptor to ERK is dependent on PI 3-kinase, we studied
the assembly of the Shc-Grb2-Sos complex. The need for Shc and Grb2 in
Ras induction is based on experiments with fibroblasts
stimulated with growth factors and has not been studied in the context
of BCR signaling. We investigated this issue using dominant-negative mutants of Shc and Grb2. Shc Y239F/Y240F/Y317F is unable to bind Grb2 (41), and Grb2R86K has an inactivated SH2 domain and is therefore
unable to bind Shc (42). A20 B cells were co-transfected with the
reporter GST-ERK in combination with cDNA encoding these mutant
proteins, and the kinase activity of immunoprecipitated GST-ERK was
measured in vitro. As seen in Fig.
3, both Shc and Grb2 mutants reduced the
activation of GST-ERK by about 50% (compare gray
bars). This finding is consistent with a need for the
Shc-Grb2 complex in Ras activation by BCR.
View larger version (20K):
[in this window]
[in a new window]
|
Fig. 3.
ERK activation is partially dependent on
Shc-Grb2-Sos assembly. A20 cells were electroporated with GST-ERK,
in combination with an excess of vector; Shc Y239F/Y240F/Y317F
(Shc Y F) cDNA or Grb2R86K
cDNA as indicated. The cells were stimulated as before, and the
activity of anti-GST immunoprecipitates was determined as before.
Black bars, activity in unstimulated cells;
gray bars, -fold increase in samples treated with
F(ab')2 rabbit anti-mouse Ig. The average of two trials is
shown. Error bars represent S.D.
|
|
We next investigated whether the assembly of Shc-Grb2-Sos is dependent
on PI 3-kinase. Cell lysates were incubated with a GST-Grb2 fusion
protein as described earlier (35), and co-precipitating Shc was
detected by immunoblot. Fig. 4 shows that
inhibition of PI 3-kinase with LY294002 had no impact on the
anti-Ig-induced phosphorylation of Shc, and phosphorylated Shc was
competent to bind the SH2 domain of Grb2 (compare lanes
2 and 3). We also examined the association of
Grb2 and Sos by co-immunoprecipitation using anti-Grb2 antibodies, as
previously described (48). As shown in Fig. 4B, the
anti-Ig-induced association of Sos and Grb2 was also unaffected by the
presence of LY294002. These results suggest that the assembly of the
Shc-Grb2-Sos complex does not require PI 3-kinase activity.
View larger version (33K):
[in this window]
[in a new window]
|
Fig. 4.
The assembly of the Shc-Grb2-Sos complex is
unaffected by LY294002. A, IIA1.6 B cells were
preincubated with carrier or LY and activated with rabbit anti-mouse Ig
for 2 min, and lysates were incubated with a GST-Grb2-SH2 fusion
protein, followed by glutathione-agarose, or the latter alone
(control). The position of Shc in the precipitates and in whole lysate
from resting cells (lysate) is indicated. B, IIA1.6 B cells
were treated as in A, and lysates were incubated with normal
rabbit Ig (control) or anti-Grb2 antibody. Associated Sos was detected
by immunoblot.
|
|
PI 3-Kinase Activity Affects the Activation of Ras and MEK--
We
directly measured Ras activation by BCR using the affinity
precipitation method (38). For these experiments, B cell lysates were
incubated with a GST fusion protein containing the Ras binding domain
of Raf. Active Ras was detected by immunoblotting the precipitated proteins with a pan-anti-Ras antibody. The samples were measured in
triplicate, and the identity of the samples was "blinded" before the assay. Fig. 5 shows a representative
experiment; in this case, a 32% decrease in Ras-GTP loading was
observed in B cells treated with LY294002. Although the amount of
active Ras detected by this method varied from experiment to
experiment, in every case we observed a decrease in Ras activation in
the presence of LY294002. However, in contrast to ERK activation, in no
case was the GTP-loading of Ras completely blocked by inhibition of PI
3-kinase.
View larger version (10K):
[in this window]
[in a new window]
|
Fig. 5.
Ras activation is decreased in the presence
of PI 3-kinase inhibitor. Splenic B cells were isolated from
BALB/c ByJ mice, pretreated with carrier () or LY294002, and
stimulated as above. GTP-bound Ras was precipitated from the lysates
using a GST-Raf-RBD fusion protein, visualized by immunoblot, and
quantitated using a Roche LumiImager. Shown is a representative
experiment; the values are the average of triplicate samples.
Error bars represent S.D.
|
|
The activity of MEK1, which is immediately upstream of ERK in the Ras
cascade, was determined by in vitro kinase assay using recombinant inactivated ERK2 as a substrate. The results are presented in Fig. 6A. We found that the
activation of MEK1 kinase activity by BCR is very sensitive to the
presence of LY294002, since MEK activity was completely blocked with 10 µM LY294002. The induction of MEK kinase activity
requires phosphorylation by Raf (49) and can be used as an indicator of
Raf activity in cells (50, 51). We examined MEK phosphorylation by
immunoblotting with anti-phospho-MEK antibody (Fig. 6B) and
found it to be similarly affected by inhibition of PI 3-kinase. These
data suggest that PI 3-kinase is required upstream of Raf and MEK
activation.
View larger version (21K):
[in this window]
[in a new window]
|
Fig. 6.
The activation of MEK1 by the B cell receptor
is dependent on PI 3-kinase activity. A, BALB/c ByJ
splenic B cells were preincubated with carrier or the indicated
concentrations of LY294002 and stimulated, and the activity of
immunoprecipitated MEK1 was determined by in vitro kinase
assay. The average of three independent trials is shown. B,
whole lysates were made from B cells stimulated in the presence of
carrier or 10 µM LY294002. The presence of phosphorylated
MEK in these lysates was detected using an anti-phospho-MEK antibody.
Half the amount of lysate was loaded in the PMA-stimulated sample as in
the others. Phospho-MEK (p-MEK) is the upper
band of the doublet, as confirmed by reprobe with anti-MEK1
antibody shown in the lower panel. A
representative experiment is shown.
|
|
ERK Activation Requires PLC- Activity--
The
activation of ERK has been reported to require intracellular calcium
influx (18). PLC- activation and consequently the mobilization of
calcium are at least partially dependent on PI 3-kinase (27, 28).
Therefore, the requirement for PI 3-kinase activity in BCR-stimulated
ERK activity might reveal an effect on PLC- and calcium flux. We
confirmed that BCR-induced ERK activation requires calcium mobilization
(data not shown) using the intracellular calcium chelator,
1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraacetic acid. To establish a corresponding requirement for PLC- activity, we
used the PLC inhibitor U73122 to block BCR-induced calcium flux. The
efficacy of U73122 was first tested in a dose-response experiment,
shown in Fig. 7A. The emission
of cells loaded with the fluorescent calcium-binding dye Fluo-4 was
monitored spectrofluorimetrically before and after BCR stimulation. We
found that a 30-s preincubation with U73122 at 1 µM is
sufficient to inhibit greater than 80% of BCR-induced calcium flux. 1 µM U73122 was not toxic to B cells, as assessed by trypan
blue dye exclusion (data not shown). We then assayed the
phosphorylation of ERK after treatment with U73122 using the same
conditions. As seen in Fig. 7B, ERK phosphorylation by BCR
is completely inhibited, indicating a requirement for PLC- activity.
This observation is consistent with earlier findings that calcium
mobilization lies distal to PI 3-kinase and proximal to ERK
activation.
View larger version (25K):
[in this window]
[in a new window]
|
Fig. 7.
The activation of ERK is dependent upon PLC
activity. A, titration of U73122. Splenic B cells were
loaded with Fluo-4/AM, and the fluorescence of the cells was monitored
over time in a luminescence spectrometer. The concentration of the PLC
inhibitor U73122 added is indicated as follows. Closed
diamonds, carrier; open inverted
triangles, 50 nM; open
squares, 200 nM; closed
triangles, 1 µM. The first
arrow represents the addition of carrier (Me2SO)
or inhibitor, and the second arrow represents the
addition of F(ab')2 rabbit anti-mouse Ig. The concentration
of intracellular calcium was calculated as described under
"Experimental Procedures." B, effect of U73122 on ERK
phosphorylation. Splenic B cells were treated with carrier or 1 µM U73122 followed by F(ab')2 rabbit
anti-mouse Ig as in A. Aliquots of whole lysates run in
parallel were immunoblotted for p-ERK1/2 (top
panel) or total ERK (lower panel). A
representative experiment is shown.
|
|
These results raised the possibility that deficient calcium
mobilization might account for the PI 3-kinase requirement in the
induction of ERK. To test this, we asked whether calcium flux induced
by the calcium ionophore ionomycin could reconstitute the necessary
signal in the absence of PI 3-kinase activity. High concentrations of
ionomycin (>1 µM) alone activate ERK (not shown); therefore, we first established an appropriate ionomycin concentration that mimics the level of calcium flux similar to that induced by BCR
ligation. The titration shown in Fig.
8A established that 50 nM ionomycin very closely mimics BCR-induced calcium
influx. To see whether increased cytoplasmic calcium caused by
ionomycin could restore ERK activity when PI 3-kinase is inhibited, we
assessed B cell lysates for phospho-ERK in the presence and absence of LY294002 and 50 nM ionomycin. The results (Fig.
8B) show that 50 nM ionomycin does not by itself
induce ERK phosphorylation (lane 4 versus lane 1); nor does it enhance
ERK phosphorylation induced by BCR stimulation (lane
6 versus lane 2).
Furthermore, the addition of ionomycin to B cells incubated in the
presence of LY294002 did not restore BCR-induced ERK phosphorylation
(lane 7). These findings demonstrate that
although PI 3-kinase affects BCR-induced calcium influx (27, 28), PI
3-kinase influences ERK by a calcium-independent pathway.
View larger version (29K):
[in this window]
[in a new window]
|
Fig. 8.
The reconstitution of calcium flux with
ionomycin does not restore ERK phosphorylation in the presence of
LY294002. A, titration of ionomycin. Splenic B cells
were loaded with Fluo-4/AM, and the fluorescence was monitored as in
Fig. 7. The arrow represents the addition of the following
reagents. Open inverted triangles, 100 nM ionomycin; closed diamonds, 50 nM ionomycin; open diamonds, 10 nM ionomycin; open circles, 20 µg/ml F(ab')2 rabbit anti-mouse Ig. B, effect
of ionomycin on ERK phosphorylation. Splenic B cells were pretreated
with carrier or 10 µM LY294002 as indicated and then
stimulated with F(ab')2 rabbit anti-mouse Ig, 50 nM ionomycin, or both reagents in combination as indicated.
The buffer used during stimulation was identical to that used in
A. The phosphorylation of ERK was determined as before. Half
the amount of lysate was loaded in the PMA-stimulated sample as in the
others. A representative experiment is shown.
|
|
PI 3-Kinase Is Downstream of Ras in B Cell Receptor
Signaling--
Experiments in fibroblasts indicated that PI 3-kinase
activation by growth factors is dependent on Ras (21-23). To examine whether the same is true in B cells, we used the activation of transiently transfected Akt as an indirect measurement for PI 3-kinase
activity. A20 murine B cells were transfected with HA-tagged Akt
cDNA in combination with an excess of vector or V12Ras, a GTPase-deficient mutant known to potently stimulate
Ras-dependent events (52). After stimulation, cell lysates
were immunoprecipitated with anti-HA monoclonal antibody, and the
immunoprecipitates were subjected to an in vitro kinase
assay, as described earlier (43). As can be seen in Fig.
9A, basal activity of HA-Akt
(Vector; white bar) is stimulated
about 5-fold by the presence of active Ras. Furthermore, the induction
of Akt by active Ras is completely blocked by inhibition of PI
3-kinase. These data are consistent with the notion that V12Ras induces
Akt by activating PI 3-kinase.
View larger version (17K):
[in this window]
[in a new window]
|
Fig. 9.
Ras is upstream of PI 3-kinase in B cell
receptor signaling. A, A20 cells were co-transfected
with HA-Akt cDNA and an excess of vector or V12Ras cDNA as
indicated, and the kinase activity of anti-HA immunoprecipitates was
determined from resting cells. White bars, cells
pretreated with carrier; black bars, cells
pretreated with 25 µM LY294002. An average of three
independent trials is shown; error bars represent
S.D. B, IIA1.6 B cells were co-transfected with HA-Akt in
combination with excess N17Ras cDNA as indicated, and the activity
of HA-Akt was determined from resting samples (white
bars) and samples stimulated with rabbit anti-mouse Ig
(black bars). An average of two trials is shown;
error bars represent S.D.
|
|
To examine this issue in the context of BCR signaling, B cells were
transiently transfected with HA-tagged Akt cDNA, in combination with an excess of vector or N17Ras, a dominant-negative mutant of Ras
(53). As seen in Fig. 9B, stimulation of the BCR increases HA-Akt activity (Vector, white bar) by
3-5-fold (Vector, black bar), as
earlier reported (43). However, in the presence of N17Ras, both basal
(N17Ras, white bar) and BCR-stimulated
(N17Ras, black bar) HA-Akt activity is
completely inhibited. These findings establish that the activation of
PI 3-kinase and its effector Akt by BCR is downstream of Ras, as
demonstrated in other systems (21-23).
| |
DISCUSSION |
The results presented here demonstrate that PI
3-kinase is required for the activation of ERK by the BCR. In the
presence of the PI 3-kinase inhibitor LY294002 or a dominant-negative
mutant of PI 3-kinase, ERK phosphorylation and activation is blocked at
early time points, with weak and abortive phosphorylation occurring after 2 min (Figs. 1 and 2). In our attempt to identify the step in the
Ras cascade that requires PI 3-kinase, we found that assembly of the
Shc-Grb2-Sos complex is unaffected by PI 3-kinase inhibitors (Fig. 4),
whereas MEK1 phosphorylation and activation displays similar
sensitivity to these agents as ERK (Fig. 6). The assembly of the
Shc-Grb2-Sos complex is at least partially responsible for Ras
activation (Fig. 3), since the activation of ERK is partially inhibited
by dominant negative mutants of Grb2 and Shc. The incomplete inhibition of ERK activation may arise from incomplete competition of
the mutant proteins with their endogenous counterparts. Alternatively, there may be other pathways that link the BCR to Ras activation that
are independent of Shc and Grb2. Supporting this possibility, the
results in Fig. 5 show that PI 3-kinase makes a small but significant
contribution to Ras activation.
ERK activation is also dependent on PLC- activity (Fig.
7B), as suggested by earlier studies indicating a
requirement for intracellular calcium mobilization (18). Since PI
3-kinase inhibitors cause a partial block in BCR-induced calcium flux
(27, 28), we investigated whether this may contribute to the defect in
ERK activity. We found that reconstitution of calcium with ionomycin failed to restore ERK activation (Fig. 8B), indicating that
PI 3-kinase affects ERK through a calcium-independent mechanism.
This report provides evidence for a PI 3-kinase-dependent
event downstream of Ras. Paradoxically, we also found that Ras acts upstream of PI 3-kinase in B cells, as it does fibroblasts (Fig. 9). The effect of Ras on PI 3-kinase is presumably through a direct interaction of Ras-GTP with the p110 subunit of PI 3-kinase. This is in
stark contrast to T cell receptor signaling, where this interaction
does not take place (54).
The fact that Ras activation is not as sensitive to LY294002 as ERK
activation suggests that PI 3-kinase provides essential pathway support
at steps downstream of Ras activation. One mechanism might be the PI
3-kinase-dependent activation of PAK, which activates Raf-1
in other systems (15). In human tonsillar B cells, ERK activation by
BCR is partially dependent on PI 3-kinase, whereas the enhancement of
ERK activation through the co-ligation of CD19 is completely dependent
on PI 3-kinase (55). ERK activation by T cell receptor in Jurkat T
cells (31) and by Fc
RI in human basophils (56) absolutely requires
PI 3-kinase. In the former case, PI 3-kinase feeds into the Ras cascade
downstream of MEK, whereas in the latter case PI 3-kinase is apparently
required for the activation of Ras itself. Interestingly, the class IB PI 3-kinase p110 links G protein-coupled receptors to ERK activation through its protein kinase activity rather than through lipid phosphorylation (33). Whether this is also true of class IA PI
3-kinases is currently unknown. In any case, these earlier reports
together with our studies on B cells show that the requirement for PI
3-kinase in ERK activation is more universal than previously recognized. The findings suggest that signal transduction pathways are
not isolated entities, but rather there is considerable cross-talk between them. Further investigation is necessary to identify the precise link between PI 3-kinase and ERK.
We have summarized our data in the model shown in Fig.
10. Ligation of the B cell receptor
causes the induction of Ras through the translocation of the
Shc-Grb2-Sos complex and possibly through other mechanisms as well.
Active Ras induces the Raf cascade as well as PI 3-kinase, with the
latter exerting a positive feedback on Ras activation. PI 3-kinase also
contributes to the activation of ERK downstream of Ras and to the
induction of PLC-. PLC- in turn induces calcium release, which
supports the activation of ERK.
View larger version (16K):
[in this window]
[in a new window]
|
Fig. 10.
Model of ERK activation by the B cell
receptor. BCR induces Ras through the assembly of the Shc-Grb2-Sos
complex as well as through other mechanisms. Ras causes the activation
of the ERK and PI 3-kinase. PI 3-kinase contributes to the activation
of PLC-2 as well as to that of ERK, feeding into the Ras pathway
both upstream and downstream of Ras itself. PLC-2 causes the
mobilization of calcium, which is also required for the activation of
ERK. Thus, signals from Ras, PI 3-kinase, and PLC-2 converge on the
activation of ERK. Closed arrowheads indicate
links investigated in this study.
|
|
These results demonstrate the intricate relationship
between the Ras, PLC-, and PI 3-kinase pathways in B cells. These
proteins can no longer be thought of as initiating separate signal
transduction cascades; rather, they are part of a complex network. We
have documented connections between the pathways at several levels, from proximal events such as the induction of PI 3-kinase to distal ones such as that of ERK. Last, the induction of ERK by the B cell
receptor appears to be under the simultaneous control of PI 3-kinase,
Ras, and PLC-. Such multilayered regulation may be necessary to
protect against inappropriate activation of ERK, given the established
importance of this enzyme in cell cycle progression and differentiation.
| |
FOOTNOTES |
*
This work was supported by National Institutes of Health
Grants CA64268 and AI49264.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.
¶
Present address: Rm. 415 Heart and Lung Institute, 473 W. 12th
Ave., Columbus, OH 43210.
Scholar of the Leukemia and Lymphoma Society
(formerly Leukemia Society of America). To whom correspondence should
be addressed: The Oklahoma Medical Research Foundation, Immunobiology
and Cancer Program, 825 N.E. 13th St., Oklahoma City, OK 73104. Tel.:
405-271-7905; Fax: 405-271-8568; E-mail:
mark-coggeshall@omrf.ouhsc.edu.
Published, JBC Papers in Press, April 25, 2002, DOI 10.1074/jbc.M202485200
| |
ABBREVIATIONS |
The abbreviations used are:
BCR, B cell
receptor;
ERK, extracellular signal-regulated kinase;
GST, glutathione S-transferase;
MEK, mitogen-activated protein
kinase/extracellular signal-regulated kinase kinase;
PI 3-kinase, phosphoinositide 3-kinase;
PLC, phospholipase C;
RBD, Ras-binding
domain;
SH2, Src homology 2;
PMA, phorbol 12-myristate 13-acetate;
MOPS, 4-morpholinepropanesulfonic acid.
| |
REFERENCES |
| 1.
|
Gold, M. R.
(2000)
Curr. Top. Microbiol. Immunol.
245,
77-134[Medline]
[Order article via Infotrieve]
|
| 2.
|
Reth, M.,
Wienands, J.,
and Schamel, W. W.
(2000)
Immunol. Rev.
176,
10-18[CrossRef][Medline]
[Order article via Infotrieve]
|
| 3.
|
Hutchcroft, J. E.,
Harrison, M. L.,
and Geahlen, R. L.
(1992)
J. Biol. Chem.
267,
8613-8619[Abstract/Free Full Text]
|
| 4.
|
Ma, H.,
Yankee, T. M., Hu, J.,
Asai, D. J.,
Harrison, M. L.,
and Geahlen, R. L.
(2001)
J. Immunol.
166,
1507-1516[Abstract/Free Full Text]
|
| 5.
|
Gold, M. R.,
and Aebersold, R.
(1994)
J. Immunol.
152,
42-50[Abstract]
|
| 6.
|
Vanhaesebroeck, B.,
and Waterfield, M. D.
(1999)
Exp. Cell Res.
253,
239-254[CrossRef][Medline]
[Order article via Infotrieve]
|
| 7.
|
Chan, T. O.,
Rittenhouse, S. E.,
and Tsichlis, P. N.
(1999)
Annu. Rev. Biochem.
68,
965-1014[CrossRef][Medline]
[Order article via Infotrieve]
|
| 8.
|
Suzuki, H.,
Terauchi, Y.,
Fujiwara, M.,
Aizawa, S.,
Yazaki, Y.,
Kadowaki, T.,
and Koyasu, S.
(1999)
Science
283,
390-392[Abstract/Free Full Text]
|
| 9.
|
Fruman, D. A.,
Snapper, S. B.,
Yballe, C. M.,
Davidson, L., Yu, J. Y.,
Alt, F. W.,
and Cantley, L. C.
(1999)
Science
283,
393-397[Abstract/Free Full Text]
|
| 10.
|
Aronheim, A.,
Engelberg, D., Li, N.,
al-Alawi, N.,
Schlessinger, J.,
and Karin, M.
(1994)
Cell
78,
949-961[CrossRef][Medline]
[Order article via Infotrieve]
|
| 11.
|
Malumbres, M.,
and Pellicer, A.
(1998)
Front. Biosci.
3,
887-912
|
| 12.
|
Lankester, A. C.,
van Schijndel, G. M.,
Rood, P. M.,
Verhoeven, A. J.,
and van Lier, R. A.
(1994)
Eur. J. Immunol.
24,
2818-2825[Medline]
[Order article via Infotrieve]
|
| 13.
|
Saxton, T. M.,
van Oostveen, I.,
Bowtell, D.,
Aebersold, R.,
and Gold, M. R.
(1994)
J. Immunol.
153,
623-636[Abstract]
|
| 14.
|
Smit, L.,
de Vries-Smits, A. M.,
Bos, J. L.,
and Borst, J.
(1994)
J. Biol. Chem.
269,
20209-20212[Abstract/Free Full Text]
|
| 15.
|
Sun, H.,
King, A. J.,
Diaz, H. B.,
and Marshall, M. S.
(2000)
Curr. Biol.
10,
281-284[CrossRef][Medline]
[Order article via Infotrieve]
|
| 16.
|
Leevers, S. J.,
Paterson, H. F.,
and Marshall, C. J.
(1994)
Nature
369,
411-414[CrossRef][Medline]
[Order article via Infotrieve]
|
| 17.
|
Roovers, K.,
and Assoian, R. K.
(2000)
Bioessays
22,
818-826[CrossRef][Medline]
[Order article via Infotrieve]
|
| 18.
|
Iritani, B. M.,
Forbush, K. A.,
Farrar, M. A.,
and Perlmutter, R. M.
(1997)
EMBO J.
16,
7019-7031[CrossRef][Medline]
[Order article via Infotrieve]
|
| 19.
|
Richards, J. D.,
Dave, S. H.,
Chou, C. H.,
Mamchak, A. A.,
and DeFranco, A. L.
(2001)
J. Immunol.
166,
3855-3864[Abstract/Free Full Text]
|
| 20.
|
Kawauchi, K.,
Lazarus, A. H.,
Sanghera, J. S.,
Man, G. L.,
Pelech, S. L.,
and Delovitch, T. L.
(1996)
Mol. Immunol.
33,
287-296[CrossRef][Medline]
[Order article via Infotrieve]
|
| 21.
|
Rodriguez-Viciana, P.,
Warne, P. H.,
Vanhaesebroeck, B.,
Waterfield, M. D.,
and Downward, J.
(1996)
EMBO J.
15,
2442-2451[Medline]
[Order article via Infotrieve]
|
| 22.
|
Rodriguez-Viciana, P.,
Warne, P. H.,
Dhand, R.,
Vanhaesebroeck, B.,
Gout, I.,
Fry, M. J.,
Waterfield, M. D.,
and Downward, J.
(1994)
Nature
370,
527-532[CrossRef][Medline]
[Order article via Infotrieve]
|
| 23.
|
Kodaki, T.,
Woscholski, R.,
Hallberg, B.,
Rodriguez-Viciana, P.,
Downward, J.,
and Parker, P. J.
(1994)
Curr. Biol.
4,
798-806[CrossRef][Medline]
[Order article via Infotrieve]
|
| 24.
|
Kurosaki, T.,
and Tsukada, S.
(2000)
Immunity
12,
1-5[CrossRef][Medline]
[Order article via Infotrieve]
|
| 25.
|
Falasca, M.,
Logan, S. K.,
Lehto, V. P.,
Baccante, G.,
Lemmon, M. A.,
and Schlessinger, J.
(1998)
EMBO J.
17,
414-422[CrossRef][Medline]
[Order article via Infotrieve]
|
| 26.
|
Bae, Y. S.,
Cantley, L. G.,
Chen, C. S.,
Kim, S. R.,
Kwon, K. S.,
and Rhee, S. G.
(1998)
J. Biol. Chem.
273,
4465-4469[Abstract/Free Full Text]
|
| 27.
|
Kiener, P. A.,
Lioubin, M. N.,
Rohrschneider, L. R.,
Ledbetter, J. A.,
Nadler, S. G.,
and Diegel, M. L.
(1997)
J. Biol. Chem.
272,
3838-3844[Abstract/Free Full Text]
|
| 28.
|
Hippen, K. L.,
Buhl, A. M.,
D'Ambrosio, D.,
Nakamura, K.,
Persin, C.,
and Cambier, J. C.
(1997)
Immunity
7,
49-58[CrossRef][Medline]
[Order article via Infotrieve]
|
| 29.
|
Duckworth, B. C.,
and Cantley, L. C.
(1997)
J. Biol. Chem.
272,
27665-27670[Abstract/Free Full Text]
|
| 30.
|
Wennstrom, S.,
and Downward, J.
(1999)
Mol. Cell. Biol.
19,
4279-4288[Abstract/Free Full Text]
|
| 31.
|
Von Willebrand, M.,
Jascur, T.,
Bonnefoy-Berard, N.,
Yano, H.,
Altman, A.,
Matsuda, Y.,
and Mustelin, T.
(1996)
Eur. J. Biochem.
235,
828-835[Medline]
[Order article via Infotrieve]
|
| 32.
|
Lopez-Ilasaca, M.,
Crespo, P.,
Pellici, P. G.,
Gutkind, J. S.,
and Wetzker, R.
(1997)
Science
275,
394-397[Abstract/Free Full Text]
|
| 33.
|
Bondeva, T.,
Pirola, L.,
Bulgarelli-Leva, G.,
Rubio, I.,
Wetzker, R.,
and Wymann, M. P.
(1998)
Science
282,
293-296[Abstract/Free Full Text]
|
| 34.
|
Pirola, L.,
Zvelebil, M. J.,
Bulgarelli-Leva, G.,
Van Obberghen, E.,
Waterfield, M. D.,
and Wymann, M. P.
(2001)
J. Biol. Chem.
276,
21544-21554[Abstract/Free Full Text]
|
| 35.
|
Tridandapani, S.,
Chacko, G. W.,
Van Brocklyn, J. R.,
and Coggeshall, K. M.
(1997)
J. Immunol.
158,
1125-1132[Abstract]
|
| 36.
|
Tridandapani, S.,
Phee, H.,
Shivakumar, L.,
Kelley, T. W.,
and Coggeshall, K. M.
(1998)
Mol. Immunol.
35,
1135-1146[CrossRef][Medline]
[Order article via Infotrieve]
|
| 37.
|
Gardner, A. M.,
Vaillancourt, R. R.,
and Johnson, G. L.
(1993)
J. Biol. Chem.
268,
17896-17901[Abstract/Free Full Text]
|
| 38.
|
Taylor, S. J.,
Resnick, R. J.,
and Shalloway, D.
(2001)
Methods Enzymol.
333,
333-342[CrossRef][Medline]
[Order article via Infotrieve]
|
| 39.
|
Montessuit, C.,
and Thorburn, A.
(1999)
J. Biol. Chem.
274,
9006-9012[Abstract/Free Full Text]
|
| 40.
|
Stokoe, D.,
Stephens, L. R.,
Copeland, T.,
Gaffney, P. R.,
Reese, C. B.,
Painter, G. F.,
Holmes, A. B.,
McCormick, F.,
and Hawkins, P. T.
(1997)
Science
277,
567-570[Abstract/Free Full Text]
|
| 41.
|
Blaikie, P. A.,
Fournier, E.,
Dilworth, S. M.,
Birnbaum, D.,
Borg, J. P.,
and Margolis, B.
(1997)
J. Biol. Chem.
272,
20671-20677[Abstract/Free Full Text]
|
| 42.
|
Tanaka, M.,
Gupta, R.,
and Mayer, B. J.
(1995)
Mol. Cell. Biol.
15,
6829-6837[Abstract]
|
| 43.
|
Jacob, A.,
Cooney, D.,
Tridandapani, S.,
Kelley, T.,
and Coggeshall, K. M.
(1999)
J. Biol. Chem.
274,
13704-13710[Abstract/Free Full Text]
|
| 44.
|
Gardner, A. M.,
Lange-Carter, C. A.,
Vaillancourt, R. R.,
and Johnson, G. L.
(1994)
Methods Enzymol.
238,
258-270[Medline]
[Order article via Infotrieve]
|
| 45.
|
Astoul, E.,
Watton, S.,
and Cantrell, D.
(1999)
J. Cell Biol.
145,
1511-1520[Abstract/Free Full Text]
|
| 46.
|
Vlahos, C. J.,
Matter, W. F.,
Hui, K. Y.,
and Brown, R. F.
(1994)
J. Biol. Chem.
269,
5241-5248[Abstract/Free Full Text]
|
| 47.
|
Arcaro, A.,
and Wymann, M. P.
(1993)
Biochem. J.
296,
297-301[Medline]
[Order article via Infotrieve]
|
| 48.
|
Harmer, S. L.,
and DeFranco, A. L.
(1997)
Mol. Cell. Biol.
17,
4087-4095[Abstract]
|
| 49.
|
Kolch, W.
(2000)
Biochem. J.
351,
289-305[CrossRef][Medline]
[Order article via Infotrieve]
|
| 50.
|
Macdonald, S. G.,
Crews, C. M., Wu, L.,
Driller, J.,
Clark, R.,
Erikson, R. L.,
and McCormick, F.
(1993)
Mol. Cell. Biol.
13,
6615-6620[Abstract/Free Full Text]
|
| 51.
|
Tordai, A.,
Franklin, R. A.,
Patel, H.,
Gardner, A. M.,
Johnson, G. L.,
and Gelfand, E. W.
(1994)
J. Biol. Chem.
269,
7538-7543[Abstract/Free Full Text]
|
| 52.
|
Khwaja, A.,
Rodriguez-Viciana, P.,
Wennstrom, S.,
Warne, P. H.,
and Downward, J.
(1997)
EMBO J.
16,
2783-2793[CrossRef][Medline]
[Order article via Infotrieve]
|
| 53.
|
van Weering, D. H.,
de Rooij, J.,
Marte, B.,
Downward, J.,
Bos, J. L.,
and Burgering, B. M.
(1998)
Mol. Cell. Biol.
18,
1802-1811[Abstract/Free Full Text]
|
| 54.
|
Genot, E.,
Reif, K.,
Beach, S.,
Kramer, I.,
and Cantrell, D.
(1998)
Oncogene
17,
1731-1738[CrossRef][Medline]
[Order article via Infotrieve]
|
| 55.
|
Li, X.,
and Carter, R. H.
(2000)
Eur. J. Immunol.
30,
1576-1586[CrossRef][Medline]
[Order article via Infotrieve]
|
| 56.
|
Miura, K.,
and MacGlashan, D. W.
(2000)
Blood
96,
2199-2205[Abstract/Free Full Text]
|
Copyright © 2002 by The American Society for Biochemistry and Molecular Biology, Inc.
CiteULike 
Complore 
Connotea 
Del.icio.us 
Digg 
Reddit 
Technorati What's this?
TOP
ABSTRACT
INTRODUCTION
