(Received for publication, October 9, 1996, and in revised form, January 24, 1997)
From the Department of Pathology and Center of
Neurobiology and Behavior, College of Physicians and Surgeons, Columbia
University, New York, New York 10032, the § ABL-Basic
Research Program, Frederick, Maryland 21702, and the
¶ Montreal Neurological Institute, McGill University,
Montreal, Quebec H3A 2B4, Canada
Many receptor tyrosine kinases possess an
"activation loop" containing three similarly placed tyrosine
autophosphorylation sites. To examine their roles in the TRK NGF
receptor, these residues (Tyr-670, Tyr-674, and Tyr-675) were mutated
singly and in all combinations to phenylalanine and stably expressed in
Trk-deficient PC12nnr5 cells. All mutant receptors showed significantly
diminished nerve growth factor (NGF)-stimulated autophosphorylation,
indicating impaired catalytic activity. NGF-induced neurite outgrowth
exhibited dose-responsive behavior when transfectants were compared by
relative receptor expression and exhibited a functional hierarchy: wild type > Y670F Y674F
Y675F
YY670/674FF = YY670/675FF
YY674/675FF > YYY670/674/675FFF. NGF-induced
tyrosine phosphorylation of Shc, ERKs, and SNT and immediate early gene
inductions generally paralleled neurogenic potential. However,
activation of phosphatidylinositol 3
-kinase and tyrosine
phosphorylation of phospholipase C
-1 was essentially abolished. The
latter effect appears due to selective inability of the mutated TRKs to
autophosphorylate the tyrosine residue (Tyr-785) required for binding
phospholipase C
-1 and indicates that the "activation loop"
tyrosines participate in NGF-dependent changes in receptor
conformation. Our findings stress the importance that expression levels
play in assessing the consequences of receptor mutations and that all
three activation loop tyrosines have roles regulating both overall and
specific NGF-mediated signaling through TRK.
For many growth factors, ligand-mediated activation of receptor
tyrosine kinases (RTKs)1 is the first
essential step leading to biological responses (1, 2). Nerve growth
factor (NGF) and other neurotrophins bind to and activate particular
members of the Trk receptor tyrosine kinase family (3, 4); NGF binds to
and activates TRKA (5, 6). The pheochromocytoma-derived PC12 cell line
(7) has been highly useful for studying NGF signal transduction and its molecular mechanisms of action. PC12 cells respond to NGF by undergoing neuronal differentiation, survival in serum-free medium, cell hypertrophy, and regulation of numerous biochemical markers (8). NGF
induces rapid tyrosine phosphorylation of TrkA and consequent phosphorylation and activation of signal transduction components including Shc, extracellular signal-regulated kinases (ERKs), phosphatidylinositol 3-kinase (PI3
K), phospholipase C
-1
(PLC
-1), and SNT (9). Activation of these signal transduction
molecules culminates in downstream signaling events, including the
induction of immediate early and late genes (10, 11).
As with other ligands and their cognate RTKs (1, 2), NGF appears to
initiate signaling through TrkA by the sequential steps of
dimerization, trans-autophosphorylation on tyrosine residues and kinase
activation, followed by binding and tyrosine phosphorylation of
substrates (9, 12, 13). In vitro studies indicate that TRKA
autophosphorylates at tyrosines 490, 670, 674, 675, and 785 (14, 15).
To analyze the significance of these phosphorylation events in NGF
signaling, we have introduced TRKA receptors modified at these residues
into the mutant PC12 cell line, PC12nnr5, that expresses no detectable
endogenous TrkA (16, 17). This analysis reveals that phosphotyrosines
490 and 785 are required for binding and activation of Shc and PLC
-1, respectively (14, 15, 18). The three remaining tyrosine
autophosphorylation sites, Tyr-670, Tyr-674, and Tyr-675, are contained
within the kinase domain of the receptor and are within a sequence
motif that is not typical for an SH2 protein binding site (19) or for
other protein-protein interactions (20, 21). Comparison of this
sequence motif with other protein kinases reveals homology with a
number of RTKs (22-27). Studies carried out largely with wild type and
mutated insulin, IGF and c-Met/HGF receptors indicate that these sites
are important for initial ligand-induced autophosphorylation and that
they are required for efficient signal transduction and promotion of
biological responses (28-36).
A physical model that begins to account for the roles of the three conserved kinase domain tyrosines is provided by the crystal structure of the non-phosphorylated insulin receptor kinase domain (37). This structure indicates that the three kinase domain tyrosines lie near the catalytic core of the kinase within an "activation loop" that prevents binding of ATP as well as physical approximation of the amino and carboxyl lobes of the kinase domain. The activation loop appears to be stabilized in this inhibitory conformation by interactions of Tyr-1162 (the homologue of Tyr-674 in TRK) with residues near the catalytic core of the kinase. This interaction also inhibits basal kinase activity by acting as a pseudosubstrate. Furthermore, it was suggested that ligand-promoted phosphorylation of activation loop tyrosines induces movement of the loop away from the catalytic core to permit efficient kinase activation.
Although studies on activation loop tyrosines in several systems collectively suggest that they function to regulate RTK activation, the roles of individual tyrosines are unclear and are subject to some inconsistency within the literature (29, 38-45). For example, tyrosine to phenylalanine mutation in the insulin receptor at the residue equivalent to TRK Tyr-670 in one case was reported to have no effect on in vitro kinase activity (35), whereas in several other studies the same mutation was reported to reduce in vitro kinase activity by approximately 80% (39) or more (41). It also appears that there may be differences between the roles of each of the activation loop tyrosines in the various receptors (34, 38, 39, 44). Moreover, past studies have indicated that mutation of individual activation loop tyrosines may selectively abolish some receptor-mediated biological responses while sparing others, although the mechanistic basis for these observations is unknown. In the present study, we have examined the activation loop tyrosines in the TRKA receptor with respect to their roles in regulating signaling and biological responses to NGF. To achieve this, we mutated the tyrosines singly and in all combinations and have stably expressed receptors containing these mutations in PC12nnr5 cells at various levels of expression. Our findings are consistent with a major role for tyrosines 670, 674, and 675, not only in regulating overall catalytic activity of the receptor but also in governing site-specific receptor autophosphorylation.
TRKA mutants were constructed using single
strand mutagenesis (Bio-Rad). Briefly, full-length TRKA was
used to generate antisense template, and sense oligonucleotides were
used to introduce the point mutations. For double and triple mutations,
oligonucleotides spanning all mutated sites were used. In the multiple
site mutation constructs, restriction site cassettes containing each
zone mutation (e.g. Y490F, Y785F etc.) were shuttled between
the autophosphorylation loop backbones and then sequenced for
confirmation. The mutant TRKs were then cloned into the
pLNCX5 retroviral expression vector using HindIII and
XhoI. The resulting constructs were then transfected into
2 cells (46), and cells resistant to G418 (500 µg/ml, Life
Technologies, Inc.) were selected, and the total population of cells
was propagated in G418 (200 µg/ml). Cellular supernatant from these
cells was used to infect PC12nnr5 cells (described below).
PC12 cells and PC12nnr5-derived mutants were grown on collagen-coated tissue culture plates in RPMI 1640 medium (Life Technologies, Inc.) supplemented with 10% heat-inactivated donor horse and 5% fetal bovine serum (both from JRH Biosciences), as described previously (7). Retroviral infections were carried out by adding 0.2-1 ml of virus-containing supernatant, recovered from packaging cell lines, to 50% confluent PC12nnr5 cell cultures (47). Transfections (used in generating cell lines bearing combinations of Y490F, Y751F, and Y785F superposed on triple activation loop mutant background) were carried out by electroporation as described previously (47). Infected/transfected cells were cultured for 1 week and then subjected to selection with G418 (Sigma) for 2 weeks. Surviving colonies were isolated and clonally expanded for characterization. Representative clones were chosen for biochemical assessment on the basis of level of receptor expression and similarity of cellular morphology with that of parental cells.
Neuritogenesis was assessed in cultures grown in RPMI 1640 medium
supplemented with 1% heat-inactivated horse serum, as described previously (7, 17). NGF-treated (100 ng/ml) and NGF-untreated cultures
were scored for times up to 1 week by determining the presence or
absence of neurites on cells chosen at random (n 300). Reported values represent the mean values of triplicate experiments conducted with each clonal line. Recombinant hNGF was a generous gift
from Genetech Inc.
NGF treatment
of cultures for biochemical assessments was routinely conducted 1 day
following exchange of the culture medium and was accomplished by
addition of an aliquot of concentrated stock to a final concentration
of 100 ng/ml. After indicated treatment times, cells were washed three
times with ice-cold phosphate-buffered saline, were lysed (10%
glycerol, 100 mM NaF, 10 mM EGTA, 1 mM Na3VO4, 1% Triton X-100, 50 mM Tris, pH 7.5, 150 mM NaCl, 10 µg/ml aprotinin, 5 µM ZnCl2, 2 mM
phenylmethylsulfonyl fluoride, and 1 µg/ml leupeptin), and the
lysates were clarified by ultracentrifugation after a 15-min incubation
on ice, all as described previously (48). Samples normalized for total
protein content were subjected to immunoprecipitation with the
indicated antibodies as described previously (15, 48, 49). Protein
A-Sepharose beads were from Pharmacia Biotech Inc., and antisera
against Shc and PLC-1 were from UBI. Anti-pan Trk (203) and
anti-phosphotyrosine (4G10) were used as described previously (15, 48,
49). Immunoprecipitated samples were washed three times in TNTG (20 mM Tris, pH 7.5, 10% glycerol, 0.1% Triton X-100, and 150 mM NaCl) and subjected to SDS-polyacrylamide gel
electrophoresis followed by electrophoretic transfer to nitrocellulose
(48). Western blotting was conducted with the indicated antibodies
using the protocol of Amersham Life Sciences, Inc., followed by
visualization by enhanced chemiluminescence (Amersham Corp.). For
quantification, data were scanned and analyzed using NIH Scion Image
v1.55 software. Blots were reprobed with antibody after stripping in
2% SDS, 100 mM 2-mercaptoethanol, and 62.5 mM
Tris, pH 6.8, and rocking at room temperature for
16 h.
ERK tyrosine phosphorylation was assessed by subjecting clarified
lysates (150 µg of protein) to SDS-polyacrylamide gel electrophoresis and Western immunoblotting with anti-phosphotyrosine. Anti-ERK C-16
antibody was from Santa Cruz Biotechnology. PI3K activity and SNT
tyrosine phosphorylation were assessed as described previously (49-51). Measurements of radiolabeled products in the PI3
K assay were
made using a Molecular Dynamics PhosphorImager.
Cells treated with NGF for 0, 30, 60, and 120 min were washed three times with ice-cold phosphate-buffered saline, and total RNA was extracted using Tri-Reagent (MRC). Purified RNA was quantified, and 20-µg samples were subjected to Northern blotting as described previously (14, 49, 52). Blots were UV cross-linked and hybridized with probes to c-fos, c-jun, tis 1, tis 8, and tis 11 as described previously (49, 53).
To study the biological importance of the tyrosine autophosphorylation sites in the activation loop of TRK, constructs of the human receptor were mutated from tyrosine to phenylalanine at residues 670, 674, and 675, both singly and in all combinations. These and wild type (WT) TRK were cloned into the pLNCX retrovirus vector (54), and the resultant recombinant retroviruses (pLNC-TRKA and mutants) were used to infect the Trk-deficient PC12-derived cell line, PC12nnr5 (16, 52). After selection, approximately two dozen independent clonal lines were isolated and expanded for each receptor construct.
Correlation between Mutant Receptor Expression Levels and NGF-promoted NeuritogenesisCell lines representative for a spectrum of WT and mutant TRK levels were chosen for each of the constructs on the basis of analyses carried out by receptor immunoprecipitation followed by quantitative immunoblotting with Trk antiserum (Table I). Expression in each line was compared with that of the PC12nnr5-T14 cell line that over-expresses wild type TRK at levels approximately 3-5-fold higher than PC12 cells (49, 52). Expression of the mutant and wild type TRKs ranged from equal to that of PC12nnr5-T14 cells to 20-50-fold higher. These cell lines were then assessed for NGF-induced neuritogenesis. In general, neurite outgrowth in the cell lines bearing mutant TRKs reached maximal levels by 3-4 days of NGF exposure (data not shown), which is comparable with previous observations for PC12nnr5-T14 cells and other TRK over-expressing PC12-derived cell lines (15, 52, 55).
|
Comparison of the maximal neuritogenic responses in cell lines
expressing comparable levels of each of the different TRK mutants revealed dramatic differences. For example, following a vertical path
in Fig. 1D at the level of TRK expression
corresponding to 10-fold that in PC12nnr5-T14 cells shows that none of
the multiply-mutated TRKs confer NGF-dependent
neuritogenesis, whereas the Y675F receptors confer responsiveness in
10-15% of cells, and Y670F and Y674F receptors confer responsiveness
in 50% of cells. Moreover, when neuritogenic extent was correlated
over a range of receptor expression levels, dose-response relationships
became apparent (Fig. 1). These plots revealed several important
points. First, receptor expression levels significantly affect
biological responsiveness (especially evident for the WT, Y670F, and
Y674F TRKs) and therefore must be considered when interpreting assessed
phenotypes. Second, each of the activation loop mutations impairs
receptor function to at least some degree. This is demonstrated by the
shifts in dose-responsiveness to NGF for cells expressing mutant TRKs
as compared with cells expressing wild type TRK (Fig. 1, D
and E). Even those mutant TRKs conferring the greatest
neurite outgrowth responses (i.e. Y670F and Y674F) had to be
expressed at levels 3-5-fold higher than present in PC12nnr5-T14 cells
to achieve significant neuritogenesis. Third, there exists a hierarchy
for restoration of neuritogenesis as a function of receptor
over-expression in the various TRKs: WT > Y670F Y674F
Y675F
YY670/674FF = YY670/675FF
YY674/675FF > YYY670/674/675FFF. Overall, the degree of
rescue achievable shows that the mutants fall into three general groupings (Fig. 1D). The WT, and Y670F and Y674F TRKs are
each capable of mediating near-complete levels of neuritogenesis,
although the two mutant TRKs require higher expression to achieve this. The second group of receptors (Y675F, YY670/674FF, and YY670/675FF), even when greatly over-expressed, mediate only partial restoration of
neurite outgrowth. An important point is that the degree of impairment
achieved by the Y675F mutation is much greater than that caused by the
other two single mutations, Y670F and Y674F. The third group includes
YY674/675FF and YYY670/674/675FFF. These lack the ability to mediate
neuritogenesis, irrespective of expression level. Collectively, these
observations indicate that TRKs mutated at different activation loop
tyrosines have differing capacities to functionally rescue
NGF-dependent responses. This is due to both the type of
mutation assessed and the level to which it is expressed.
NGF-inducible Tyrosine Autophosphorylation of Activation Loop Mutant TRK Receptors and Assessment of NGF-induced Signaling through Shc, the ERKs, SNT, and Immediate Early Genes
Our neuritogenesis studies revealed that for partially compromised receptors, the expression levels of TRK receptors can significantly influence the degree to which they mediate biological responses. To control for this, we therefore assessed additional parameters in cell lines expressing comparable levels of different mutant receptors, as well as in cell lines expressing different levels of each individual TRK mutant. Two cell lines were selected for each of the constructs, one expressing receptors at approximately 5-fold, and the second at approximately 10-25-fold higher than expressed by PC12nnr5-T14 cells. Cell lines with TRK expressed at lower levels were not assessed for biochemical responses, due to their lack of neuritogenic responses (Fig. 1).
To assess NGF-promoted Trk tyrosine autophosphorylation, cultures were
treated with or without 100 ng/ml NGF for 5 min. Lysates were
normalized for protein content, subjected to immunoprecipitation with
Trk antibody, and immunoprecipitates subjected to Western blotting and
sequentially probed with anti-phosphotyrosine and anti-Trk (Fig.
2). All of the TRK mutants showed NGF-inducible tyrosine
phosphorylation, including those in which all three of the activation
loop tyrosines were replaced with phenylalanine (Fig. 2A).
However, while autophosphorylation was evident with all of the mutants,
it was clearly reduced as compared with wild type Trk (as judged by
qualitative ratios of anti-phosphotyrosine to anti-Trk signals, even
after taking into consideration the numbers of mutated tyrosines).
Moreover, the deficits in NGF-induced autophosphorylation of the TRK
mutants were not rescueable by receptor over-expression (Fig.
2B) nor were they attributable to altered kinetics of
activation when assessed over a time course of several hours (data not
shown). Furthermore, the levels of receptor autophosphorylation did not
correlate well with the capacity of the TRK mutants to mediate neurite
outgrowth. For instance, although the single mutants (Y670F, Y674F, and
Y675F) showed comparable levels of NGF-stimulated TRK tyrosine
autophosphorylation, as noted above, TRK Y675F was much less effective
in mediating neuritogenesis.
Trk activation by NGF in PC12 cells and PC12nnr5 cells expressing wild
type TRK leads to rapid tyrosine phosphorylation of the Shc (15, 56,
57) and ERK (58, 59) proteins, both elements of the Ras signaling
pathway. Studies using TRK mutants have revealed that Shc interacts
with TRK via phosphotyrosine 490 and that this interaction is required
for NGF-dependent Shc tyrosine phosphorylation (15, 60).
ERK activation is downstream of Shc and Ras activation and has been
implicated as a necessary component of the mechanism by which NGF
promotes neurite outgrowth in PC12 cells (15, 49, 58, 59, 61-67).
Immunoprecipitation and Western immunoblotting were used to assess
NGF-promoted Shc tyrosine phosphorylation at a 5-min time point in cell
lines expressing wild type and activation loop mutants of TRK.
Observations generally correlated with those found for TRK
autophosphorylation and neuritogenesis in that single mutants were
significantly more functional than combination mutants and that even
single mutants required over-expression (as compared with WT receptors)
to yield significant Shc phosphorylation (Fig.
3A). In addition, as anticipated, lines with
10-25-fold over-expression showed greater activation than those with
5-fold over-expression (data not shown). The one case in which Shc
phosphorylation and neuritogenesis potential did not correlate well was
for the Y675F mutant which was about equal in activity to Y670F and
Y674F but significantly less effective in mediating neurite
outgrowth.
Studies to assess NGF-promoted tyrosine phosphorylation of the ERK kinases in lines with WT and mutant TRKs were carried out at the 5-min time point by subjecting cell lysates to Western immunoblotting. NGF-stimulated ERK tyrosine phosphorylation signal intensities closely paralleled the neuritogenic behavior of the lines (Figs. 1 and 3B). A time course study (up to 10 h) with lines expressing the singly mutated receptors revealed that the Y675F construct showed both lower signal intensity and significantly shorter signal duration when compared with WT, Y670F, and Y674F TRKs (data not shown). This further supports the correlation between neuritogenic activities of the receptors and capacity to stimulate ERK tyrosine phosphorylation.
PC12 cells, or PC12nnr5 cells expressing WT TRK, undergo
NGF-dependent tyrosine phosphorylation of the p13 suc1
agarose associating tyrosine-phosphorylated nuclear localized protein
(SNT), which appears to be a differentiation-specific signaling
molecule in these cells (49, 51). A recent study (49) further supports a role for SNT in PC12 cell neuronal differentiation by establishing that deletion of a conserved juxtamembrane motif (KFG) in TRK selectively renders it incapable of activating the pathway leading to
phosphorylation of SNT and that PC12nnr5 cells expressing these mutant
receptors are unable to promote neuritogenesis in response to NGF.
Although SNT phosphorylation requires the KFG motif (49), it is not
dependent on phosphorylation of Tyr-490 or Tyr-785. To determine if the
activation loop mutations in TRK affect the NGF-induced tyrosine
phosphorylation of SNT, cell lines expressing wild type and activation
loop mutant receptors were assessed for this parameter both before and
after treatment with NGF for 5 min. As illustrated in Fig.
4, all activation loop mutations impair SNT tyrosine
phosphorylation in response to NGF, and very high over-expression of
mutant receptors (e.g. YY670/674FF) can rescue NGF-promoted
SNT phosphorylation to levels near those observed in wild type PC12
cells. Comparison of these data with those in Fig. 1 reveals that SNT
phosphorylation was detectable in all lines capable of NGF-stimulated
neurite outgrowth and was undetectable in lines incapable of
neuritogenesis. This correlation is consistent with a required role for
SNT phosphorylation in promotion of neurite outgrowth. In addition,
these findings indicate that although SNT tyrosine phosphorylation does
not require autophosphorylation of TRK Tyr-490 and Tyr-785, it is
dependent on autophosphorylation of the activation loop tyrosines.
Stimulation of Trk and downstream signaling pathways by NGF promotes the induction of a number of immediate early genes (68, 69). To determine the effects of the activation loop Trk mutations and consequent alterations in intracellular signaling on induction of these genes, cell lines expressing wild type or mutant TRKs were treated with NGF for 0, 30, 60, and 120 min and assessed by Northern blotting for levels of c-fos, c-jun, tis 1 (NGFI-B), tis 8 (NGFI-A), and tis 11 mRNA. These experiments revealed that the extent of immediate early gene induction generally paralleled neuritogenic potential and ERK activation. Thus, at over-expression levels 5-10-fold that of PC12nnr5-T14 cells, the single mutants all exhibited NGF-promoted levels of gene inductions comparable with those of PC12nnr5-T14 cells; the YY670/674FF and YY670/675FF bearing cell lines showed induction only when the receptors were over-expressed by 10-20-fold relative to the level of TRK expressed in PC12nnr5-T14 cells; the YY674/675FF lines do not respond unless expressed to levels over 30-fold higher than PC12nnr5-T14 cells; and the YYY670/674/675FFF lines that we have assessed had no detectable responses. The one anomaly was the Y675F lines that exhibited immediate early gene responses similar to those of lines with the other single activation loop mutations but which showed relatively poor neuritogenesis.
NGF-mediated Tyrosine Phosphorylation of PLCAutophosphorylation of TRK at Tyr-785 results in
binding, tyrosine phosphorylation, and activation of PLC-1 (14, 15, 18, 70). To assess the effect of activation loop mutations on
NGF-promoted tyrosine phosphorylation of PLC
-1, lysates were prepared from cells treated with NGF for 5 min and were subjected to
immunoprecipitation with anti-PLC
-1 antibody. Immunoprecipitated PLC
-1 was sequentially probed in Western blot experiments with anti-phosphotyrosine and anti-PLC
-1 antibodies. As shown in Fig. 5, NGF-induced PLC
-1 tyrosine phosphorylation was
undetectable, or greatly diminished, in all activation loop mutant cell
lines tested, including those with high receptor over-expression and those that mediate robust neurite outgrowth. In contrast, NGF treatment
of cells expressing wild type Trk (PC12, PC12nnr5-T14 and
PC12nnr5-WT.13) resulted in PLC
-1 tyrosine phosphorylation. Therefore, any mutation of the activation loop tyrosines renders TRKA
highly impaired for tyrosine phosphorylation of PLC
-1.
To determine if this impairment was attributable to abrogated
interaction between PLC-1 and TRK activation loop mutants, we
assessed the ability of these proteins to co-immunoprecipitate. Samples
prepared as above were subjected to immunoprecipitation with
anti-PLC
-1 antibody, Western blotted, and sequentially probed with
antisera/antibodies against Trk, phosphotyrosine (4G10), and PLC
-1.
Lysates from NGF-treated cells bearing WT receptors yielded
co-immunoprecipitation of PLC
-1 and an anti-Trk immunoreactive band
migrating at 140 kDa (data not shown). This Trk-immunoreactive band
co-migrates with a prominent anti-phosphotyrosine-immunoreactive band
(Fig. 5), consistent with its identification as tyrosine-phosphorylated TRKA. In contrast, no anti-Trk signals were detected in PLC
-1 immunoprecipitates from NGF-treated cells expressing even single Tyr to
Phe activation loop mutations (data not shown). Re-probing of the blots
with anti-phosphotyrosine confirmed that little or no tyrosine
phosphorylated TRK co-immunoprecipitates with PLC
-1 in any of the
activation loop mutants, even at very high levels of over-expression
(Fig. 5). Therefore, the inability of TRK activation loop mutant
receptors to phosphorylate PLC
-1 appears to be due to impaired
interaction between the receptors and PLC
-1.
Phosphatidylinositol 3-kinase (PI3
K) activity is an
additional signaling enzyme that is activated by NGF in PC12 cells (50) and implicated as a mediator of both neuritogenesis and survival (71,
72). The mechanism of PI3
K activation is not clear, but recent
findings appear to implicate tyrosine 490 as a major determinant of
NGF-mediated PI3
K activation (70).2 PI3
K
activity was assessed in vitro in cell lines expressing wild
type and activation loop mutant TRKs treated for 5 min with NGF. As
illustrated in Fig. 6, PI3
K activity was induced by NGF 2-3-fold in PC12 cells, 6-10-fold in PC12nnr5-T14 cells, and
3-6-fold in the PC12nnr5-WT.13 cell line. In contrast, no PI3
K
activity was reproducibly induced by NGF treatment in any of the cell
lines expressing the mutant TRKs, including those with very high levels of receptor over-expression. Thus, as in the case of PLC
-1, all of
the activation loop mutations, including those affecting single tyrosines, abolished detectable NGF-induced PI3
K activation. An
additional effect revealed by our analyses was that, on a per mg of
cell protein basis, the basal levels of PI3
K activity in those lines
with highest over-expression of mutant receptors were consistently
elevated 3-10-fold when compared with basal levels in PC12nnr5-T14
cells (data not shown). The latter observation raises the possibility
that very high over-expression of mutated TRKs may lead to at least
some degree of constitutive PI3
K activation.
Mutation of Any TRK Activation Loop Tyrosine Compromises Autophosphorylation of Tyr-785
To extend our experiments on
autophosphorylation and activation of signaling molecules, we generated
and examined cell lines expressing TRK mutants in which the activation
loop triple mutant was combined with tyrosine to phenylalanine
mutations of residues Tyr-490, Tyr-751, and Tyr-785, singly and in
combination. As noted above, the latter are the TRK tyrosine
autophosphorylation sites not contained in the activation loop and are
responsible for binding and/or activating Shc, PI3K, and PLC
-1.
Initial characterization of these cell lines revealed that, like the
triple mutants, they failed to mediate both NGF-promoted ERK activation
and neuritogenesis (data not shown). As shown in Fig. 7,
analysis of the various lines indicated that basal and NGF-promoted
tyrosine autophosphorylation of the mutant receptors were maintained by
those mutants that retained Tyr-490 and were absent in those that had
this site mutated, despite the simultaneous presence of Tyr-785 and
Tyr-751. Previous work has demonstrated that the Y490F mutation alone
in otherwise unmodified hTRK receptors does not impair TRK tyrosine
autophosphorylation, either overall or at Tyr-785 (15, 73) and thus is
not a first step in the TRK autophosphorylation mechanism. The present
findings indicate that the tyrosine autophosphorylation observed in the triple activation loop TRK mutants occurs solely at the Tyr-490 position. This observation, taken together with the receptor
autophosphorylation and PLC
-1 signaling data, is consistent with the
prediction that mutation of any of the activation loop tyrosines
disrupts TRK autophosphorylation at Tyr-785.
The purpose of the present study was to characterize the roles of the putative autophosphorylation activation loop tyrosines in the TRK receptor. This was achieved by mutating these tyrosines singly, and in all combinations, and then examining the signaling properties of each mutant receptor when stably expressed at various levels in PC12nnr5 cells that lack endogenous Trk. The use of PC12-derived cells permitted us to carry out our investigation in a background that displays neuronal phenotypic properties that include neurite outgrowth.
Level of Mutant TRK Expression Affects Responsiveness to NGFAn important feature here is that TRK-transfected cell lines were studied over a range of receptor expression. Examining NGF-induced responses in this manner provided means to take TRK protein expression into account and revealed that each of the tyrosines in the activation loop plays an important role in regulating NGF responsiveness. In many cases, the presence and degree of functional impairment induced by particular receptor loop mutations could be masked by over-expression. Thus, lines expressing several of the activation loop receptor mutants exhibited wild-type responses, and functional impairment of the mutant receptors was detected only by comparing dose-response curves for cell lines expressing mutant and non-mutant receptors. Such findings raise a general cautionary note for studies in which mutant receptors are functionally evaluated by exogenous introduction into cell lines; in these cases, expression level is likely to be an important determinant of apparent preservation of function.
Activation Loop Mutations Affect Total Receptor AutophosphorylationOur findings demonstrate that mutation of any one of the three activation loop tyrosines in TRK results in substantial and essentially equal reduction of NGF-mediated receptor tyrosine autophosphorylation. Likewise, further decreases in TRK tyrosine autophosphorylation occur with the combined mutation of any two tyrosines, and an additional reduction occurs in response to mutation of the third tyrosine. Autophosphorylation impairment appears to be independent of both receptor expression level and autophosphorylation kinetics. Additionally, the decrements in autophosphorylation do not appear to be attributable simply to reduction of the number of available substrate tyrosine residues, because the relative loss of TRK tyrosine phosphorylation is not proportional to the number of sites mutated, especially with regard to single tyrosine mutants. One potential contribution to the dramatic loss of tyrosine autophosphorylation during the transition from WT to single activation loop tyrosine mutant is provided by our finding that tyrosine 785 is not autophosphorylated in activation loop mutant receptors. Observations with other RTKs, and principally the insulin receptor, indicate that the extent of autophosphorylation correlates with activation of kinase activity (1, 34, 74-79). Therefore, an additional major factor in the reduction of autophosphorylation observed in the mutated TRK receptors appears to be impairment of receptor kinase activity necessary for efficient autophosphorylation.
Mutations homologous to those studied here have been carried out with several other RTKs, and they appear to show some variation from one case to the next with respect to their effect on both ligand-stimulated autophosphorylation and biological responses (34, 44, 80, 81). However, all combinations of these mutations have not been assessed in each of these systems. Findings for autophosphorylation of the insulin receptor closely resemble those for TRK in that single mutations substantially, and about equally, decrease ligand-stimulated receptor autophosphorylation, and mutation of additional tyrosines results in more severe impairment (38, 39). With regard to biological responses, however, there are differences. For example, mutation of the insulin receptor tyrosine equivalent to TRK Tyr-670 abolished thymidine incorporation but not metabolic responses (38, 41), whereas mutation of the tyrosine equivalent to TRK Tyr-674 and Tyr-674/675 compromised 2-deoxyglucose uptake and activation of glycogen synthase but not thymidine incorporation (29, 38). This somewhat contrasts with our findings for TRK-mediated signaling, in that we observed no such dissection of function, as both of our downstream correlates of receptor function (neurite outgrowth and immediate early gene induction) were adversely affected by mutation of any of the activation loop tyrosines.
For the c-Met/hepatocyte growth factor (HGF) receptor, the consequences
for activation loop mutations yielded a hierarchical loss of RTK
autophosphorylation which, when expressed in sites equivalent to those
in TRKA, were WT = Y670F > Y674F Y675F and in which
the mutant equivalent to YY674/675FF lost all activity (34). It was
further reported that mutation of sites equivalent to either Tyr-674 or
Tyr-675 abolished a cell migration response to HGF (34) or to EGF in a
chimeric-receptor paradigm (33). In the case of the IGF-I receptor,
mutations equivalent to Y670F and Y674F appeared to cause a moderate
decrease in receptor autophosphorylation and to have no effect on
mitogenic responsiveness to IGF, whereas the mutation equivalent to
Y675F abolished both receptor autophosphorylation and mitogenicity in
response to IGF (42, 44). In contrast, assessment of
IGF-dependent growth on soft agar showed functional impairment for all of the singly mutated receptors (44). Collectively, these findings further illustrate that there are both similarities and
distinctions between the roles of individual homologous activation loop
tyrosines in different RTKs.
TrkB, which is highly homologous to TrkA in kinase domain sequence and presumably in overall intracellular structure, has been mutated at the equivalent of TRKA positions Tyr-670 and Tyr-674/675 and expressed in cell lines (80, 81). The single mutation was reported to be without effect on either autophosphorylation or activation of a transcription reporter gene, whereas cells bearing the double mutants were greatly impaired in both assessed phenotypes. Although the effects of the TrkB Y670F mutation appear to be in contrast with our findings, a more likely explanation is that, as with TRKA, a high degree of function may have been rescued by over-expression.
Effect of Activation Loop Mutations on Substrate Tyrosine PhosphorylationEffects of mutations on receptor signaling may be
due to global actions on catalytic activity as well as to differential
effects on phosphorylation of specific tyrosine residues and/or of
specific substrates. A surprising and novel observation here was that
mutation of any one or more of the activation loop tyrosines in TRK
blocks the NGF-dependent induction of PI3K activity and
tyrosine phosphorylation of PLC
-1. In contrast, NGF-promoted Shc
phosphorylation, although compromised, was not significantly reduced in
the cases of single site mutations and several of the double site
mutations. The most likely explanation for the effect on PLC
-1
tyrosine phosphorylation is that mutation of any of the activation loop
tyrosines selectively compromises NGF-promoted receptor
autophosphorylation of Tyr-785 in the C terminus of the receptor. This
mechanism would account for the loss of NGF-induced
co-immunoprecipitation of PLC
-1 and mutated TRK, and the loss of
PLC
-1 tyrosine phosphorylation in response to NGF treatment in all
of the TRK mutants assessed. We directly demonstrated this mechanism in
the triply-mutated TRK background, where NGF-stimulated TRK
autophosphorylation was retained only in receptors with an intact
Tyr-490 (Fig. 7), therefore indicating that Tyr-785 was not being
phosphorylated. This potential mechanism recapitulates previous studies
in which TRK tyrosine 785 was mutated to phenylalanine, which
eliminated phosphorylation at this position, and consequently abolished
binding and activation of PLC
-1 (14, 18). Taken together, our
observations indicate that mutation of any of the activation loop
tyrosines selectively abrogates tyrosine phosphorylation of Tyr-785
and, consequently, binding and activation of PLC
-1.
Although loss of PI3K activation would have a similar mechanistic
explanation if association of this enzyme with TRK was mediated via
phospho-Tyr-751 (60, 82), recent findings suggest that TRK-evoked PI3
K
activation is mediated by Tyr-490 (70).2 In
this case, the differential loss of PI3
K activity, vis à vis the partially preserved Shc tyrosine phosphorylation, could be
explained by a difference in the threshold of TRK kinase activity necessary for generation of a functional and biochemically detectable signal. For example, if PI3
K activity is dependent upon Shc-mediated activation of Ras (83, 84), then the reduction of Shc tyrosine phosphorylation observed for the single mutants could completely impair
PI3
K activation by falling below a given critical level, while
simultaneously maintaining partial activation of other signaling molecules downstream of Ras (e.g. ERKs). In agreement with
this idea of a threshold effect, wild type PC12 cells show relatively poor NGF-mediated PI3
K activation, and TRK over-expression results in
substantially enhanced responses. An alternative suggestion for the
lack of PI3
K activation is provided by recent findings of a feedback
mechanism in which phosphatidylinositol kinase products block the
association of phosphatidylinositol kinases with
tyrosine-phosphorylated proteins/RTKs (85). We found that basal PI3
K
activity was elevated in cell lines highly over-expressing activation
loop mutant TRKs, which is consistent with the production of
phosphatidylinositol kinase products in the absence of NGF. It is
possible that these products block association of the p85 subunit of
PI3
K with TRK, even in the presence of NGF, thereby blocking
NGF-dependent increases in PI3
K activity.
The differential consequences that activation loop tyrosine mutations have on autophosphorylation of specific sites in the TRK receptor may also pertain to other RTKs. Tavare and Dickens (91) presented evidence that mutation of the site homologous to TRK Tyr-674 in the insulin receptor leads to abolition of autophosphorylation at two C-terminal tyrosine residues. Although effects on autophosphorylation at other sites were not reported in this case, it is of interest that autophosphorylation of insulin receptor substrate 1, which binds to insulin receptors toward the N-terminal side of the kinase domain, is only partially impaired in response to mutation of the tyrosine equivalent to TRK Tyr-670 (38, 39). Differential, site-specific effects on autophosphorylation may also account for the observation that mutation of the insulin receptor site equivalent to TRK Tyr-670 abolishes insulin-stimulated thymidine incorporation but not activation of glycogen synthetase (41).
Despite loss of signaling through PI3K and PLC
-1, TRK receptors
with single activation loop mutations were still able to mediate
differentiative responses to NGF. This is consistent with past
observations that PLC
-1 tyrosine phosphorylation is not required for
neurite outgrowth (14, 73). Our present results extend these
observations, for both PLC
-1 and PI3
K, to NGF-inducible downstream
signaling responses such as induction of immediate early genes. It has
been reported that wortmannin, an inhibitor of PI3
K, blocks
NGF-stimulated neurite outgrowth (71). If such effects are entirely due
to PI3
K inhibition, then our findings suggest that the observed
elevated basal PI3
K activity reported for over-expressing activation
loop mutant cell lines, rather than NGF-stimulated PI3
K activity, is
sufficient for neuritic outgrowth. Alternatively, the wortmannin used
in previous studies may have inhibited the activity of other proteins,
in addition to PI3
K, required for this response.
The presence of biological responses to NGF in cells bearing receptors
mutated at activation loop tyrosines must be interpreted with respect
to those pathways that although impaired are partially functional. At
present, this includes the Shc/Ras pathway and the pathway defined by
the TRK KFG mutation that involves SNT. Past findings have indicated
that both of these pathways may play roles in neuritogenesis and
immediate early gene regulation in PC12 cells (15, 49, 73). This is
consistent with findings here in which neurite outgrowth and gene
regulation generally correlate with the extent of NGF-stimulated Shc
and SNT tyrosine phosphorylation. Nevertheless, there were several
apparent exceptions to this observation. One was that for the Y675F
mutants, neuritogenic responses and ERK activation were relatively weak
even when Shc tyrosine phosphorylation was strong. This suggests that
there may be an additional TRK/Tyr-675-regulated element that plays a
role in the signaling between Shc and ERKs. A second discrepancy was
that the triple activation loop TRKs appeared capable of
autophosphorylating Tyr-490 but showed little if any phosphorylation of
Shc. One possible interpretation of this is that the kinase activity in
these mutants is sufficient to autophosphorylate the receptor and
thereby promote binding of Shc but is impaired with respect to
phosphorylation of this substrate; such a mechanism appears to occur in
the TRK Y751F mutant.3
As a first approximation, activation of TRK by NGF likely parallels the intensively studied process by which insulin receptors are activated. In the latter case, the activation loop appears to block access of ATP and of substrates to the catalytic core of non-activated receptors (37). The crystal structure of the insulin receptor kinase domain has suggested that blockade of substrate access is due, at least in part, to interaction of tyrosine 1162 (corresponding to Tyr-674 in TRK) with a critical aspartate residue in the catalytic core. Ligand binding appears to cause a change in receptor conformation (which, in the case of Trk would include receptor dimerization), which permits trans-autophosphorylation of the activation loop tyrosines (86-88). This phosphorylation, and consequent change in charge, is hypothesized to bring the activation loop into a conformation which no longer inhibits substrate access and which permits the activated receptor to further trans-phosphorylate itself as well as receptor-associated substrates (37, 89, 90). Even for the insulin receptor, the roles in this process of the activation loop tyrosines other than Tyr-1162 are presently unknown.
As appears to be the case for the insulin receptor and at least several other RTKs that possess homologous activation loops, phosphorylation of all three tyrosines is required for optimal activation of TRK. Our dose-response observations concerning neurite outgrowth and receptor occupancy indicate that there is a hierarchical order in which mutation of these sites, singly and in combinations, impairs function. Significantly, we also found evidence that autophosphorylation of TRK Tyr-785 appears to be abolished by mutation of even a single activation loop tyrosine. This suggests that phosphorylation of all three activation loop tyrosines causes, and is required for, a change in conformation that permits interaction between the catalytic core and C-terminal tyrosine residues. One model to account for this would be that after the activation loop tyrosines are phosphorylated, each interacts with specific nearby basic residues to stabilize a conformation that promotes full activation of the receptor kinase, including access to the C-terminal region. In this model, autophosphorylation of the activation loop tyrosines would function both to relieve inhibition of kinase activity as well as to stabilize a new, optimally active conformation.
R. M. S. and D. R. K. thank George VandeWoude and the ABL-BRP for their generous support.