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J. Biol. Chem., Vol. 276, Issue 11, 7709-7712, March 16, 2001
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From the
Received for publication, December 11, 2000, and in revised form, January 17, 2001
Nerve growth factor (NGF) binding to both p75 and
TrkA neurotrophin receptors activates the transcription factor nuclear
factor The biological responses to neurotrophins such as
NGF1 include neuronal
survival and differentiation (1). Two receptors, TrkA and p75,
participate in the formation of the high affinity NGF binding site (2).
TrkA enhances both NGF responsiveness and cell survival (3). The
transcription factor nuclear factor Cell Culture and Reagents--
Cultures of human embryonic
kidney 293 (HEK 293) or NIH-3T3 cells were maintained in high glucose
Dulbecco's modified Eagle's medium containing 10% fetal calf serum.
Subconfluent cells were transfected by the calcium phosphate method.
PC12 cells were grown on cultureware coated with rat tail collagen in
RPMI containing 10% horse serum and 5% fetal calf serum and
antibiotics (50 units/ml penicillin and 50 mg/ml streptomycin). PC12 or
NIH-3T3 cells were routinely transfected using LipofectAMINE 2000 (Life
Technologies, Inc.). 2.5 S NGF was purchased from Bioproducts for
Science (Indianapolis, IN). The monoclonal 12CA5 anti-HA and anti-Flag
antibodies were from Sigma. The rabbit anti-Myc, anti-TRAF6, anti-TrkA,
and anti-IKK antibodies were from Santa Cruz Biotechnology. The
monoclonal anti-p62 was obtained from BD Transduction Laboratories.
Immunoprecipitation and Western Blot Analysis--
To detect
endogenous proteins in PC12 cells or those cotransfected into HEK
cells, lysates were prepared from subconfluent cultures of cells grown
on 100-mm dishes. Typically cells were transfected for 36-42 h with
5-10 µg of construct and pcDNA3 plasmid to give 30 µg of total
DNA. After transfection, cells were stimulated or not with 50 ng/ml
NGF. Cells were then harvested and lysed in PD buffer (40 mM Tris-HCl pH 8.0, 500 mM NaCl, 0.1% Nonidet P-40, 6 mM EDTA, 6 mM EGTA, 10 mM
Measurement of NF- Because aPKC is critically involved in the NGF prosurvival
signaling pathway (13, 18), we decided to investigate whether neurotrophin binding would stimulate the formation of a complex between
NGF receptor components, TrkA and p75, and p62. PC12 cell lysates were
prepared from NGF-treated cells followed by pull-down assays (19)
employing GST-TrkA or GST-p75 (Fig.
1A). p62 associated with TrkA
but not with p75. To confirm this finding in a more in vivo
setting, p62 was coexpressed with either TrkA or p75 in HEK cells (17),
and the coprecipitation of p62 with either receptor was examined. The
results, shown in Fig. 1B, confirmed that p62 selectively
associates with TrkA but not with p75. As in this experiment both TrkA
and p62 were over-expressed, their interaction took place even in the
absence of any stimulus. To demonstrate that endogenous p62 and TrkA
interact in vivo and that this interaction may be induced in
response to NGF, PC12 cells were stimulated with NGF for different
times after which the coprecipitation of endogenous p62 with TrkA was
examined. The results shown in Fig. 1C demonstrate that
there is a significant portion of p62 bound to TrkA under basal
conditions but that this interaction was reproducibly enhanced in the
NGF-treated cells (Fig. 1C), indicating that this is an
NGF-regulated process. To establish which region of p62 is required for
interaction with TrkA, deletion mutants of p62 were transfected into
HEK cells along with HA-tagged TrkA, and their association was
determined by immunoprecipitation as above (17). The region
encompassing amino acids 266-446 of p62 binds TrkA, whereas the
binding of p62 to TRAF6 has been mapped to amino acids 225-251 (Ref.
17 and Table I). This indicates that p62 may accommodate both TrkA and TRAF6 simultaneously. Deletion of the
TRAF6 binding site did not effect TrkA binding to p62, thus further
strengthening the notion that p62 interacts with TrkA and TRAF6 through
two independent binding domains (Table I).
TRAF6 has been reported to interact with p75 (5). To determine whether
TRAF6 interacts with TrkA as well, both p75 and TrkA were coexpressed
in HEK cells along with Flag-TRAF6. Whereas p75 associated with TRAF6
in an NGF-dependent manner (Fig.
2A) as previously reported
(5), TRAF6 failed to associate directly with TrkA. The interaction of
p75 with TRAF6 was mapped to the C-proximal TRAF-C domain, a region
that also accommodates p62 (17). Coexpression experiments in HEK cells
revealed that TRAF6 can bind both p75 and p62 simultaneously (not
shown). Because p62 interacts with TRAF6 (17), it is conceivable that
p62 may be brought into a p75 complex via TRAF6 serving as a bridge. If this model is correct we should be able to coimmunoprecipitate p62 with
p75 only in the presence of TRAF6. The results shown in Fig.
2B strongly suggest that these predictions are correct. Thus, in HEK cells transfected with different expression vectors, a
small amount of p75 was found to associate with p62, likely through
endogenous TRAF6. Upon coexpression of TRAF6, recruitment of p75 into
the p62 complex was significantly enhanced (~2.5-fold). The ability
of TrkA to coassociate with TRAF6 was dramatically and
consistently enhanced by the presence of exogenous p62 (Fig. 2B). We next determined whether NGF could stimulate the
formation of an endogenous TRAF6-p62 complex in PC12 cells (Fig.
2C). In the absence of NGF little or no association of TRAF6
with p62 or aPKC could be detected. However, the addition of NGF
resulted in a rapid interaction of TRAF6 with p62 and consequently with aPKC. Close examination revealed that the kinetics of association between TRAF6 and p62 (maximum 1-5 min) occurs prior to the
recruitment of p62 to the TrkA receptor (Fig. 1C, peaks at
15 min), suggesting that it is a two-step process. Collectively, these
results reveal that p62 interacts with TRAF6 in response to NGF and may
likely serve as a bridge between both p75 and TrkA receptor
components.
ACCELERATED PUBLICATION
The Atypical Protein Kinase C-interacting Protein p62 Is a
Scaffold for NF-
B Activation by Nerve Growth Factor*
§,,,
, and Department of Biological Sciences, Program
in Cell and Molecular Biosciences, Auburn University, Auburn,
Alabama 36849, ¶ Centro Biologia Molecular "Severo Ochoa"
(CSIC), Universidad Autonoma, Canto Blanco, 28049 Madrid, Spain, and
the Centre for Neuronal Survival, Montreal Neurological
Institute, McGill University, Montreal H3A 2B4, Canada
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
B (NF-B). Here we show that the atypical protein kinase
C-interacting protein, p62, which binds TRAF6, selectively
interacts with TrkA but not p75. In contrast, TRAF6 interacts with p75
but not TrkA. We demonstrate the formation of a TRAF6-p62 complex that
serves as a bridge linking both p75 and TrkA signaling. Of functional relevance, transfection of antisense p62-enhanced p75-mediated cell
death and diminished NGF-induced differentiation occur
through a mechanism involving inhibition of IKK activity. These
findings reveal a new function for p62 as a common platform for
communication of both p75-TRAF6 and TrkA signals. Moreover, we
demonstrated that p62 serves as a scaffold for activation of the
NF-B pathway, which mediates NGF survival and differentiation responses.
INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
B (NF-B) is activated by both
TrkA and p75 receptor components (4). Moreover, p75 has been shown to
interact with TRAF6 (5), a critical adapter in the activation of
NF-B by interleukin-1 and other cytokines (6). In addition,
inhibition of NF-B increases p75-mediated apoptosis in this system
(7), demonstrating a prosurvival requirement for this transcription
factor (8, 9). Furthermore, mice deficient in IKK, the enzyme that
phosphorylates and targets the inhibitory molecule IB leading to
NF
B activation, leads to a defect in neureulation (10).
Similarly, TRAF6-deficient mice also display a failure of neural tube
closure and exencephaly (11). Collectively, these findings underscore
the importance of NFB in the nervous system. The activation of IKK
and NF-B has been shown to require atypical protein kinase C (aPKC)
in both neuronal and non-neuronal systems (reviewed in Ref. 12). Moreover, aPKC over-expression enhances NGF prosurvival signaling through up-regulation of NF-B (13). In contrast, proapoptotic signaling inhibits aPKC and blocks NF-B (14). Additionally, the
selective aPKC-binding protein, p62 (15, 16), has been shown to
interact with TRAF6 and to be essential during interleukin-1 signaling
to NF-B (17). Here we report that p62 plays a novel role as a
scaffold for the activation of NF-B by nerve growth factor, linking
both p75 and TrkA receptor components.
EXPERIMENTAL PROCEDURES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
-glycerophosphate, 10 mM NaF, 10 mM phenyl
phosphate, 300 µM Na3V04, 1 mM benzamidine, 2 mM phenylmethysulfonyl
fluoride, 10 µg/ml aprotinin, 1 µg/ml leupeptin, 1 µg/ml
pepstatin, 1 mM dithiothreitol). Extracts were centrifuged at 15,000 × g for 15 min. Protein was determined, and
equal amounts of whole-cell lysate were diluted in PD buffer and
incubated with antibody as indicated for 2 h. Then protein A or G
beads were added for an additional hour at 4 °C. The
immunoprecipitates were then washed five times with PD buffer. As
control an aliquot of the cell lysate (1/10) volume was also analyzed
by immunoblotting. Samples were fractionated on 7.5%
SDS-polyacrylamide gel electrophoresis, transferred to nitrocellulose,
and subjected to Western blot analysis with the corresponding
antibodies. Proteins were detected with ECL reagents (Amersham
Pharmacia Biotech).
B Activity--
NF-B activation was
measured using a reporter gene assay. HEK, 3T3, or PC12 cells were
transfected with a B-luciferase reporter gene plasmid, 3EconA-Luc
(17). After 24 or 48 h, the cells were stimulated with NGF and
activity determined using a Promega luciferase assay kit. Individual
constructs were transfected in duplicate and each assay measured in
triplicate. Values are reported as the mean ± S.E. of three
individual experiments.
RESULTS AND DISCUSSION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
View larger version (32K):
[in a new window]
Fig. 1.
Interaction of p62 with TrkA.
A, equivalent amounts of NGF-stimulated (50 ng/ml, 15 min)
PC12 cell lysates were bound to GST-TrkA, GST-p75, or GST alone (18).
The associated p62 protein was determined by Western blotting
(WB) (15). B, Myc-p75 or HA-TrkA was coexpressed
with either HA-p62 or Myc-p62 in HEK cells followed by treatment with
NGF. Coassociation was determined by immunoprecipitation
(IP)/Western blotting (21). A fraction of the lysate was
blotted with anti-HA or anti-Myc antibody to check for expression of
p75, TrkA, or p62 as indicated. C, lysates prepared from
NGF-stimulated (50 ng/ml, 0-60 min) PC12 cells were immunoprecipitated
with either TrkA or p62 antibody followed by Western blotting with
either p62 or TrkA antibody as indicated. A fraction of the cell lysate
was analyzed by blotting with p62 or TrkA antibody. Similar results
were obtained in four separate experiments.
Mapping of p62-TrkA interaction domains
View larger version (43K):
[in a new window]
Fig. 2.
p62 links TrkA to TRAF6-p75.
A, subconfluent cultures of HEK cells were cotransfected
with expression plasmid for Flag-tagged TRAF6 and either Myc-p75 or
HA-TrkA followed by stimulation with NGF (50 ng/ml) for 15 min. The
interaction was determined by immunoprecipitation (IP) and
Western blotting (WB). A fraction of the lysate was blotted
with anti-Myc, HA, or FLAG antibody to check for expression of p75,
TrkA, or TRAF6. B, TRAF6 enhances the interaction of p62
with p75. HEK cells were cotransfected with expression plasmid for
Flag-tagged TRAF6 or HA-p75. Endogenous p62 was immunoprecipitated from
3 mg of cell lysate followed by Western blotting with either HA or Flag
antibody. A fraction of the lysate was blotted with HA, Flag, or p62
antibody to check for expression of p75 or TRAF6. HEK cells were
cotransfected with expression plasmid for Flag-tagged TRAF6, Myc-62, or
HA-TrkA. Cell lysates (750 µg) were immunoprecipitated with antibody
to HA followed by Western blotting with either p62 or Flag antibody. A
fraction of the lysate was blotted with HA, Flag, or Myc antibody to
check for expression of TrkA, TRAF6, or p62. Similar results were
obtained in three separate experiments. C, the interaction
of endogenous TRAF6 with p62 was determined by stimulating PC12 cells
with NGF (50 ng/ml) for up to 1 h followed by immunoprecipitation
of equivalent cell lysates with either aPKC or p62 antibody as
indicated. A fraction of the lysate was blotted with aPKC or p62
antibody. Similar results were obtained in five separate
experiments.
As TRAF6 interaction with p75 results in activation of NF-B (7), it
was of interest to determine whether the down-regulation of p62 with a
p62 antisense construct (17) would block the induction of NF-B as
measured by a luciferase reporter system. The results shown in Fig.
3A demonstrate that this is
the case, because there was a dramatic reduction of NF-B
activation by the expression of p75 and TRAF6 in cells transfected with
the p62 antisense construct as compared with the nontransfected cells.
On the other hand, the transfection of a p62 expression vector, that by
itself does not activate NF-B in this system (17), dramatically
enhanced p75-TRAF6 or TrkA-TRAF6 activation of NF-B (Fig.
3B). In contrast, p62/ZIP2, which lacks the TRAF6 binding
site (16), failed to activate NF-B (Fig. 3B). Altogether
this indicates that the recruitment of p62 to the NGF receptor
signaling complex is critical for the activation of NF-B. Consistent
with this notion, overexpression of p62 in PC12 cells resulted in a
dose-dependent enhancement of both basal as well as
NGF-stimulated activation of NF-B (Fig. 3C). We next
conducted experiments to investigate whether the antisense construct of
p62 would block NGF-induced activation of NF-B in cells expressing
either one or both NGF receptors. Interestingly, antisense p62 blocked
NGF-induced activation of NF-B in PC12 cells expressing both
receptors (Fig. 3D). Likewise, p62 down-regulation in
NIH-3T3 cells expressing either p75 or TrkA receptor (20) (Fig.
3D) also abrogated NGF-induced activation of NF-B.
Collectively these findings demonstrate that p62, like aPKC (13), is
essential in the activation of NF-B by NGF and that it serves to
scaffold proximal NGF receptor components in this pathway.
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The functional relevance of the presence of p62 in these complexes was
addressed further in the following series of experiments. Overexpression of p75 in HEK cells results in ligand-independent cell
death that is prevented by TRAF6 (7, 8). Consistent with the role of
NF-B in cell survival signaling (4), the expression of antisense p62
enhanced p75 mediated-cell death (Fig. 4A), whereas expression of
TRAF6 or p62 blocked cell death. The activation of NF-B is likewise
required for neuronal differentiation (9) and TrkA responsiveness (4).
Transfection of antisense p62 significantly impaired NGF-induced
neurite outgrowth, whereas overexpression of p62 enhanced NGF
responsiveness (Fig. 4A). The mechanism whereby p62
regulates activation of NFB likely involves recruitment of TRAF6
and aPKC onto the p62 scaffold, thus enabling aPKC-mediated
phosphorylation of IKK (21). To provide evidence for the involvement of
p62 in this process, we assessed the activity of endogenous IKK
activity in an in vitro kinase assay using GST-I
as
the substrate (4, 21). Transfection of antisense p62 suppressed NGF-stimulated activation of IKK (Fig. 4B).
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The findings reported here provide new insight into the proximal
components of the NGF/NF-B pathway and demonstrate formation of a p62 bridge that scaffolds together both p75 and TrkA receptors for
the activation of NF-B (Fig. 4C). Our results stress the role of p62 as a common and critical intermediary that channels different signaling pathways toward IKK activation. Understanding the
mechanism whereby the TRAF6-p62 complex is regulated in vivo is an area of ongoing study. Together, these findings underscore the
importance of p62 as a scaffold for NF-B and as a common platform
for communication of both p75 and TrkA receptor signals.
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ACKNOWLEDGEMENTS |
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We are indebted to Moses Chao and Rick Dobrosky for constructs, Gordon Guroff for support and cell lines, Laura Sanz for advice, and Esther Garcia for technical assistance.
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FOOTNOTES |
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* This study was funded by grants from the National Institutes of Health (to M. W. W.), the Ministry of Science and Education Spain (to M. W. W. and J. M.), and the European Union and Glaxo Wellcome Spain (to J. M.).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.
§ To whom correspondence should be addressed: Dept. of Biological Sciences, 331 Funchess Hall, Auburn University, AL 36849. Tel.: 334-844-9226; Fax: 334-844-9234; E-mail: Wootemw@auburn.edu.
Published, JBC Papers in Press, January 22, 2001, DOI 10.1074/jbc.C000869200
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ABBREVIATIONS |
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The abbreviations used are:
NGF, nerve growth
factor;
NF-B, nuclear factor B;
IKK, IB kinase;
aPKC, atypical protein kinase C;
HEK cells, human embryonic kidney cells;
GST, glutathione S-transferase;
HA, hemagglutinin.
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
REFERENCES
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Y. Hirano, S. Yoshinaga, K. Ogura, M. Yokochi, Y. Noda, H. Sumimoto, and F. Inagaki Solution Structure of Atypical Protein Kinase C PB1 Domain and Its Mode of Interaction with ZIP/p62 and MEK5 J. Biol. Chem., July 23, 2004; 279(30): 31883 - 31890. [Abstract] [Full Text] [PDF]
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J. I.S. MacDonald, C. J. Kubu, and S. O. Meakin Nesca, a novel adapter, translocates to the nuclear envelope and regulates neurotrophin-induced neurite outgrowth J. Cell Biol., March 15, 2004; 164(6): 851 - 862. [Abstract] [Full Text] [PDF]
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K. Nakamura and G. L. Johnson PB1 Domains of MEKK2 and MEKK3 Interact with the MEK5 PB1 Domain for Activation of the ERK5 Pathway J. Biol. Chem., September 26, 2003; 278(39): 36989 - 36992. [Abstract] [Full Text] [PDF]
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S. P. Lad, D. A. Peterson, R. A. Bradshaw, and K. E. Neet Individual and Combined Effects of TrkA and p75NTR Nerve Growth Factor Receptors: A ROLE FOR THE HIGH AFFINITY RECEPTOR SITE J. Biol. Chem., June 27, 2003; 278(27): 24808 - 24817. [Abstract] [Full Text] [PDF]
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C. Croci, J. H. Brandstatter, and R. Enz ZIP3, a New Splice Variant of the PKC-zeta -interacting Protein Family, Binds to GABAC Receptors, PKC-zeta , and Kvbeta 2 J. Biol. Chem., February 14, 2003; 278(8): 6128 - 6135. [Abstract] [Full Text] [PDF]
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T. Geetha and M. W. Wooten Association of the Atypical Protein Kinase C-interacting Protein p62/ZIP with Nerve Growth Factor Receptor TrkA Regulates Receptor Trafficking and Erk5 Signaling J. Biol. Chem., February 7, 2003; 278(7): 4730 - 4739. [Abstract] [Full Text] [PDF]
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 T. Hirai and K. Chida Protein Kinase C{zeta} (PKC{zeta}): Activation Mechanisms and Cellular Functions J. Biochem., January 1, 2003; 133(1): 1 - 7. [Abstract] [Full Text] [PDF]
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A. Suzuki, K. Akimoto, and S. Ohno Protein Kinase C {lambda}/{iota} (PKC{lambda}/{iota}): A PKC Isotype Essential for the Development of Multicellular Organisms J. Biochem., January 1, 2003; 133(1): 9 - 16. [Abstract] [Full Text] [PDF]
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A. Avila, N. Silverman, M. T. Diaz-Meco, and J. Moscat The Drosophila Atypical Protein Kinase C-Ref(2)P Complex Constitutes a Conserved Module for Signaling in the Toll Pathway Mol. Cell. Biol., December 15, 2002; 22(24): 8787 - 8795. [Abstract] [Full Text] [PDF]
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B. Cariou, D. Perdereau, K. Cailliau, E. Browaeys-Poly, V. Bereziat, M. Vasseur-Cognet, J. Girard, and A.-F. Burnol The Adapter Protein ZIP Binds Grb14 and Regulates Its Inhibitory Action on Insulin Signaling by Recruiting Protein Kinase C{zeta} Mol. Cell. Biol., October 15, 2002; 22(20): 6959 - 6970. [Abstract] [Full Text] [PDF]
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B. Torocsik, J. M. Angelastro, and L. A. Greene The Basic Region and Leucine Zipper Transcription Factor MafK Is a New Nerve Growth Factor-Responsive Immediate Early Gene That Regulates Neurite Outgrowth J. Neurosci., October 15, 2002; 22(20): 8971 - 8980. [Abstract] [Full Text] [PDF]
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V. Mamidipudi, X. Li, and M. W. Wooten Identification of Interleukin 1 Receptor-associated Kinase as a Conserved Component in the p75-Neurotrophin Receptor Activation of Nuclear Factor-kappa B J. Biol. Chem., July 26, 2002; 277(31): 28010 - 28018. [Abstract] [Full Text] [PDF]
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 C. Yan, Y. Liang, K. D. Nylander, J. Wong, R. M. Rudavsky, H. U. Saragovi, and N. F. Schor p75-Nerve Growth Factor as an Antiapoptotic Complex: Independence versus Cooperativity in Protection from Enediyne Chemotherapeutic Agents Mol. Pharmacol., April 1, 2002; 61(4): 710 - 719. [Abstract] [Full Text] [PDF]
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M. W. Wooten, M. L. Vandenplas, M. L. Seibenhener, T. Geetha, and M. T. Diaz-Meco Nerve Growth Factor Stimulates Multisite Tyrosine Phosphorylation and Activation of the Atypical Protein Kinase C's via a src Kinase Pathway Mol. Cell. Biol., December 15, 200 |
