(Received for publication, May 4, 1995; and in revised form, November 10, 1995)
From the
Regulation of the activity of the extracellular signal regulated kinase (ERK) mitogen-activated protein kinases was examined in Rat-1 HIR, a fibroblast cell line overexpressing the human insulin receptor. Insulin or phorbol ester induced partial activations of ERKs, while a combination of insulin and phorbol ester resulted in a synergistic activation. Preincubation with phorbol ester increased the subsequent response to insulin. Phorbol ester did not enhance tyrosine phosphorylation of the insulin receptor. Insulin did not enhance activation of phospholipase D in response to phorbol ester. Lysophosphatidic acid also acted synergistically with insulin to induce ERK activation. Lysophosphatidic acid alone had little effect on ERK, and did not activate phospholipase D. The combination of phorbol ester and insulin maintained tyrosine phosphorylation of focal adhesion kinase, while insulin alone decreased its tyrosine phosphorylation. Phorbol ester induced phosphorylation of Shc on serine/threonine, while insulin induced tyrosine phosphorylation of Shc and Shc-Grb2 binding. These results suggest that full activation of ERKs in fibroblasts can require the cooperation of at least two signaling pathways, one of which may result from a protein kinase C-dependent phosphorylation of effectors regulating ERK activation. In this manner, phorbol esters may enhance mitogenic signals initiated by growth factor receptors.
The ERK ()mitogen-activated protein kinases (MAPKs),
which are activated in response to a wide variety of growth factors,
hormones, and other mitogenic stimuli, have been linked to the
induction of cell proliferation(1) . The insulin receptor, a
tyrosine kinase, can elicit both metabolic and mitogenic
responses(2) . The insulin receptor binds to several effectors,
with binding to insulin receptor substrate-1 (IRS-1) mediating most of
the metabolic effects of insulin. Mutation or deletion of some of the
phosphorylatable tyrosines in the insulin receptor can enhance its
mitogenic activity(3) , suggesting that multifunctionality of
the receptor may compromise its mitogenic potential. Phorbol ester
tumor promoters can act additively or synergistically with insulin to
induce mitogenesis(4, 5) .
The mitogenic activity of the insulin receptor has been correlated with its ability to activate MAPK, a response that is mediated predominantly through interaction of the insulin receptor with Shc(6) . IRS-1 and Shc compete for binding to Grb2, such that IRS-1 may either inhibit (7) or enhance (8) activation of MAPK. Tyrosine-phosphorylated Shc binds to the adapter Grb2, causing disassembly of SOS from Grb2 resulting in GDP-GTP exchange on Ras(9) . GTP-bound Ras promotes activation of Raf-1 kinase(1, 10) . Raf-1 phosphorylates and activates MEK (mitogen-activated protein kinase kinase/ERK kinase), which phosphorylates and activates MAPK. One downstream effector of MAPK is RSK, another protein serine/threonine kinase. It is clear that the insulin receptor initiates signals that are independent of MAPK activation (reviewed in (11) ). Activation of Ras is not required for metabolic signaling by insulin(12) , and activation of MAPK is not sufficient for these metabolic responses(13, 14) .
Focal adhesion kinase (FAK), a tyrosine kinase localized to focal adhesions, is involved in the association of cells with the extracellular matrix via integrins. While FAK is constitutively phosphorylated on tyrosine in quiescent fibroblasts(15) , its phosphorylation is increased in response to phorbol esters(16) . Phosphorylation of FAK enhances its binding to Grb2 (17) and phosphatidylinositol 3-kinase(18) , and results in activation of the MAPK cascade(17) . Insulin induces dephosphorylation of FAK in Rat-1 HIR cells(15) . Similar results have been reported for another cell line(19) .
Phorbol esters, which activate isoforms of
protein kinase C (PKC), are general activators of the MAPK cascade. The
pathway involved in this response is not clear. Activation of MAPK via
PKC appears to involve the Ras/Raf-1 pathway in some
cases(20, 21) , but not in others(22) . PKC
can phosphorylate the insulin receptor on serine and threonine
residues, including serine 1327(23) . These phosphorylations
can decrease the tyrosine kinase activity of the receptor (24) and may have additional effects on its substrate
recognition(23) . Activation of PKC interferes with
phosphorylation of IRS-1 by the insulin receptor (24) . PKC
activation results in enhanced association of Shc with a cytosolic
protein tyrosine phosphatase, PTP-PEST(25) . Thus, PKCs can
potentially affect insulin receptor signaling at several levels.
In this study, we have examined the activation of MAPK in Rat-1 fibroblasts expressing the human insulin receptor. A strikingly synergistic activation of MAPK was observed in confluent cells incubated with both insulin and phorbol ester. The mechanism of the synergism appears to reflect a requirement for activation of two signaling pathways for full induction of MAPK activity.
Protein kinase assays were performed as described previously(46) . Myelin basic protein (MBP) and a peptide derived from the carboxyl terminus of ribosomal protein S6 (S6 peptide; RRLSSLRA) were used as in vitro substrates for MAPK and RSK, respectively. MBP was obtained from Sigma or Upstate Biotechnology, Inc. S6 peptide was synthesized by the Peptide Synthesis Facility at the Medical University of South Carolina.
Separation of MAPK isoforms by Mono Q chromatography was performed as described previously(28) . Cytosolic extract prepared from eight 150-mm dishes of cells was applied to a Mono Q column (1-ml bed volume) using a fast protein liquid chromatography system (Pharmacia Biotech Inc.). Proteins were eluted with a gradient from 0-500 mM NaCl developed over 100 min at a flow rate of 1 ml/min. MAPK activity was assayed in each fraction immediately after completion of the chromatography.
Figure 1: Effects of insulin and PMA on MBP and S6 peptide kinase activities in Rat-1 HIR cells. Confluent, serum-starved Rat-1 HIR cells were incubated for 5 min with 100 nM insulin, 100 nM PMA, or both. PMA + Ins indicates that PMA was added approximately 5 s prior to insulin, while Ins + PMA indicates that insulin was added prior to PMA. MAPK and RSK activities were assayed in the same experiment using MBP or S6 peptide as substrates, respectively. Each data point represents the mean ± S.D. of values obtained from duplicate dishes of cells.
Since insulin has previously been reported to markedly activate MAPK in Rat-1 HIR cells(27, 31) , a number of experimental variables were examined in order to identify factors contributing to the relative insulin resistance observed in our studies. Insulin or phorbol ester alone activated cytosolic MBP kinase activity by less than 3-fold in most experiments (Fig. 2). MBP kinase activity measured in detergent-solubilized membrane fractions was activated in the same manner as that measured in cytosol (data not shown). Factors potentially contributing to variations in responsiveness were examined. These included composition of the cell lysis buffer (e.g. inclusion of additional inhibitors of serine/threonine and tyrosine phosphatases), passage number of the cells, presence of glucose in the incubation medium, presence of serum (with and without serum starvation), duration of serum starvation (1-5 days), starvation conditions (DME versus DME/F-12 medium), and state of confluence of the cells. None of these factors was found to consistently increase MBP kinase activation in response to insulin or PMA alone. Similar responses were seen in the absence or presence of serum for both subconfluent cells (Fig. 2) and confluent cells ( Fig. 2and data not shown).
Figure 2: Effects of agonists on MBP kinase activity in subconfluent and confluent cells. Cells were plated on day 1. Cytosolic extracts were prepared on day 3 from cells that were 50% confluent and growing in serum, on day 4 from cells that were 50% confluent and had been serum-starved overnight, and on day 5 from cells that were confluent and serum-starved overnight. Each data point represents the mean ± S.D. of values obtained from duplicate dishes of cells.
In order to
confirm that the activated MBP kinase activity represented MAPK (i.e. ERKs), cytosolic proteins were partially purified by
Mono Q chromatography. Three peaks of MBP kinase activity were resolved (Fig. 3A). Using immunoblotting with a pan-ERK
antiserum, immunoreactive proteins were observed in column fractions
containing MBP kinase activity (Fig. 3B). The first
peak, which was the major peak with respect to both kinase activity and
immunoreactivity, contained an immunoreactive protein of approximately
42 kDa. This protein probably represents ERK2, which elutes at this
salt concentration under our chromatography conditions. The second peak
(45 kDa) is an unidentified MAPK isoform. The third peak (
44
kDa) likely represents ERK1, which elutes here under the conditions
used. These results indicate that the MBP kinase activity that is
synergistically stimulated by PMA and insulin represents MAPK isoforms.
Figure 3: Characterization of MAPKs from Rat-1 HIR cells. Confluent cells were incubated with 100 nM insulin and 100 nM PMA for 5 min. Cytosolic extracts prepared from the cells were partially purified by chromatography on Mono Q, using a linear gradient from 0-500 mM NaCl. For Panel A, MAPK activity was assessed in each fraction, using MBP as substrate. For Panel B, proteins in the fractions containing MBP kinase activity were separated by SDS-PAGE. MAPKs were identified by immunoblotting with an anti-ERK antibody. In Panel C, anti-ERK immunoprecipitates were prepared and then immunoblotted using anti-ERK (left portion) and anti-phosphotyrosine (right portion). The lane labeled wce contains whole-cell extract prepared from cells treated with PMA. The lanes labeled s contain molecular size markers.
The ability of PMA and insulin to induce phosphorylation of MAPK was studied. MAPK was immunoprecipitated and then subjected to immunoblotting for MAPK and phosphotyrosine (Fig. 3C). ERK2 was detected as a 42-kDa band in the immunoprecipitates. An additional band of lower mobility, labeled ERK2`, was detected in cells treated with PMA, insulin, or PMA plus insulin. Shifts in the electrophoretic mobility of MAPK are typically seen following its phosphorylation and activation. The combination of insulin and PMA caused a more complete shift in MAPK mobility than was seen for either agent alone. Phosphotyrosine was detected in a band that co-migrated with the shifted band of ERK2 seen in cells treated with both PMA and insulin, but was not detected in ERK2 from cells treated with insulin or PMA alone. The results shown in Fig. 3C confirm that co-application of insulin and PMA results in enhanced activation of MAPK.
The time course of the response to insulin and PMA, alone and in combination, was examined. Combined data from two experiments in which partial activation of MAPK was seen in response to insulin and PMA are shown in Fig. 4A. Activation of MAPK was maximal within 10 min in response to either insulin or PMA alone. The response to the combination of insulin and PMA followed a similar time course. These results show that the synergistic effect increases the magnitude of the response, rather than its duration.
Figure 4: Time course of the effects of agonists on MAPK activity. In Panel A, confluent Rat-1 HIR cells were incubated for the indicated times with 100 nM insulin, 100 nM PMA, or a combination of insulin and PMA. MAPK activity was assessed in cytosolic extracts prepared from the cells. Each point represents the mean ± S.D. of values obtained from two separate experiments that were each performed with duplicate dishes of cells. In Panel B, an experiment was performed as described for Panel A, except that the cells were incubated with insulin, PMA, or insulin and PMA for 5 or 30 min in the absence or presence of 5 µg/ml actinomycin D. Actinomycin D was added to the cells 5 min prior to the addition of insulin and/or PMA. Each data point represents the mean ± S.D. of values obtained from duplicate dishes of cells.
The duration and magnitude of agonist-induced MAPK activation can be regulated by induction of dual-function MAPK phosphatases, some of which are encoded by immediate-early genes(32, 33) . Inhibition of phosphatase induction by one agent could potentially enhance responsiveness to another. The time course of the response was measured in the absence and presence of actinomycin D (Fig. 4B). The response to insulin plus PMA was similar, at 5-10-min incubation, in the presence or absence of actinomycin D. The responses to insulin or PMA alone, which were negligible in this experiment, were not enhanced by actinomycin D. These data suggest that rapid induction of a phosphatase (or other protein) is not involved in regulating the magnitude of the acute responses to insulin, PMA, or insulin plus PMA. Thus, the observed synergism, which was routinely detected at 5 min, was not mediated by effects of insulin or PMA on inducible phosphatases.
Concentrations of 100 nM insulin and 100
nM PMA were generally used in these studies. The dose-response
relationships for insulin and PMA were examined (data not shown). The
EC values for the effects of insulin and PMA on MAPK
activity could not be accurately determined, due to the relatively low
responses. The synergistic effects of insulin and PMA (100 nM)
were observed with 10 nM and 1 µM insulin, but
not with 1 nM insulin. The EC
for insulin in the
presence of 100 nM PMA was approximately 3 nM. This
value is consistent with the dose-response relationship observed for
other insulin responses in these cells(3) . MAPK activation was
not observed with 1 nM PMA plus 10 nM insulin. Full
activation was observed with 10 nM or 1 µM PMA
plus 100 nM insulin. EC
values for effects of PMA
on MAPK activity are typically
3 nM. Since typical
effective doses of both PMA and insulin were required for synergistic
activation of MAPK, these results suggest that one agent does not alter
the dose-response relationship for the other.
We examined whether PMA enhanced responsiveness to insulin, or vice versa, reasoning that a ``priming'' effect might be detected subsequent to treatment with insulin or PMA. When PMA was added 10 min prior to insulin, MAPK activity was similar to that seen when both agents were added at the same time (Fig. 5). When insulin was added 10 min prior to PMA, MAPK activation was reduced as compared to simultaneous addition. Little synergism was noted when PMA was added 30 or 60 min prior to insulin (data not shown). These data suggest that PMA enhances the ability of insulin to activate MAPK.
Figure 5: Effects of insulin, PMA, and LPA on MAPK activity. Confluent Rat-1 HIR cells were incubated with 100 nM insulin, 100 nM PMA, 10 µM LPA, or combinations of these agents, for the indicated times. For some samples, PMA or insulin was added for 10 min, followed by addition of insulin or PMA for 5 min (total incubation time of 15 min with the first agent, and 5 min with the second agent). Each data point represents the mean ± S.D. of values obtained from duplicate dishes of cells.
The effects of LPA, a mitogenic agonist for fibroblasts, were also examined (Fig. 5). LPA alone did not significantly increase MAPK activity, but enhanced MAPK activation in response to insulin. The synergistic effect of LPA was usually less than that observed for PMA. In experiments in which the synergistic responses to LPA and PMA were similar, and in which PMA alone caused significant activation of MAPK, there was still no significant response to LPA alone (see Fig. 7). Similar effects were seen in subconfluent and confluent cells (data not shown). Thus, while LPA alone does not significantly activate MAPK in these cells, its ability to synergistically enhance MAPK activation mimics that of phorbol ester.
Figure 7: Effects of agonists on the electrophoretic mobilities of MAPK and Shc. In Panel A, whole-cell extracts were prepared from confluent Rat-1 HIR cells that had been incubated for 10 min with no addition (C), 100 nM insulin (I), 100 nM PMA (P), 10 µM LPA (L), PMA plus insulin (P + I), or LPA plus insulin (L + I). Duplicate dishes of cells were used for each experimental condition. Proteins were resolved by SDS-PAGE on 12.5% Laemmli gels. For the experiment shown in the upper blot, the lower molecular size markers were run off the bottom of the gel to enhance separation of MAPK and Shc species. In the upper blot, immunoblotting was carried out for the upper portion of the gel using an anti-Shc antibody, and for the lower portion using a polyclonal pan-ERK antibody. The positions of the molecular size markers (lane s) are indicated on the right. In the lower blot, a replicate experiment is shown for immunoblotting with anti-Shc. Within each experiment, equivalent amounts of cellular protein were loaded on each lane. In Panel B, Shc was immunoprecipitated from cells treated for 10 min with no addition (C), 100 nM PMA (P), or PMA plus 100 nM insulin (P+I). The immunoprecipitates, shown on the left-hand side of the blot, were incubated with (+) and without(-) calf intestinal phosphatase (p'tase) as described in the text. The right-hand side of the blot contains whole-cell extracts prepared from cells incubated with no addition, PMA, 100 nM insulin (I), or PMA plus insulin (P+I). Proteins were resolved on 12.5% gels. The transferred gels were immunoblotted with anti-Shc.
Figure 6:
Effects of insulin and PMA on PLD activity
in confluent cells. Confluent Rat-1 HIR cells were incubated for 18 h
with [H]palmitic acid to label cellular lipid.
The cells were then incubated for 15 min in the presence of 0.5%
ethanol with 100 nM insulin, 100 nM PMA, 10
µM LPA, insulin and PMA, or insulin and LPA. Production of
[
H]phosphatidylethanol was assessed following
separation of extracted phospholipids by thin layer chromatography.
Each data point represents the mean ± S.D. of values obtained
from quadruplicate dishes of cells.
To determine whether the observed shifts in mobility were due to Shc phosphorylation, immunoprecipitated Shc was dephosphorylated with calf intestinal phosphatase. As shown in Fig. 7B, phosphatase treatment reversed the effects of PMA and PMA plus insulin on the mobilities of the 52- and 66-kDa forms of Shc. Similar results were seen for Shc from insulin-treated cells (data not shown). The data shown indicate that the lower mobility bands seen in our experiments represent phosphorylated Shc.
To further investigate this phenomenon, the
effects of insulin and PMA on tyrosine phosphorylation were examined (Fig. 8A). As described previously for Rat-1 HIR cells,
insulin induced phosphorylation of an 90-kDa protein corresponding
to the size of the insulin receptor
subunit. Phosphorylation of
the insulin receptor was not induced by PMA. In some experiments, PMA
caused a slight decrease in insulin-induced receptor phosphorylation,
consistent with previous reports(24) . Like PMA, LPA had no
effect on the tyrosine phosphorylation state of the insulin receptor
(data not shown). In some experiments, phosphorylation of a protein
migrating at
185 kDa, which probably represents IRS-1, was
observed in response to insulin or PMA plus insulin (data not shown).
These results suggest that PMA does not significantly alter the ability
of insulin to phosphorylate IRS-1. Insulin caused a decrease in the
phosphorylation state of a protein migrating at approximately 120 kDa (Fig. 8A), corresponding to the molecular size of FAK.
Migration of FAK at this position was confirmed by immunoblotting with
anti-FAK antibodies (data not shown). This decrease in FAK
phosphorylation was not seen when cells were incubated with a
combination of PMA and insulin. Similar results were seen for a
combination of LPA and insulin (data not shown). These data establish
that enhancement of MAPK activation by PMA is not due to enhancement of
tyrosine phosphorylation of the insulin receptor, but suggest that
co-incubation with PMA may block the ability of insulin to induce
dephosphorylation of FAK.
Figure 8: Effects of agonists on tyrosine phosphorylation and Shc-Grb2 association in Rat-1 HIR cells. Confluent Rat-1 HIR cells were incubated with no additions (C), 100 nM insulin (I), 100 nM PMA (P), 10 µM LPA (L), PMA plus insulin (P+I) or LPA plus insulin (L+I) for 10 min. The positions of the molecular size markers are indicated on the right. In all cases, each lane contains extracts or immunoprecipitates prepared from equivalent numbers of cells. In Panel A, whole cell extracts were prepared, and proteins were resolved on 12.5% SDS-PAGE gels. Lanes containing molecular size markers are indicated by s. Immunoblotting was performed using anti-phosphotyrosine. In Panel B, Shc immunoprecipitates were prepared from cells treated as described in Panel A. In addition, some cells were incubated for 10 min with one agent, followed by addition of the second agent for an additional 10 min (P, I = PMA, then insulin; I, P = insulin, then PMA). The immunoprecipitates were subjected to immunoblotting for phosphotyrosine. In the far right lane of the blot, a whole-cell extract from PMA-treated cells was immunoblotted for Shc. In Panel C, anti-Shc immunoprecipitates were prepared as described for Panel B; proteins were resolved on 12.5% SDS-PAGE gels. The gels were immunoblotted using anti-Grb2. The lane on the far right contains whole-cell extract prepared from cells treated with LPA plus insulin. Equivalent immunoprecipitation of Shc was confirmed by immunoblotting the upper portion of the gel for Shc (data not shown).
The effects of insulin and PMA on the tyrosine phosphorylation of Shc were next examined. As shown in Fig. 8B (left), insulin alone induced tyrosine phosphorylation of the major 52-kDa species of Shc. Phosphotyrosine was also present, at barely detectable levels, in the 46-kDa form of Shc. Tyrosine phosphorylation of the 66-kDa form of Shc was not detected, but was likely below the level of detection of our assay. PMA (Fig. 8B, right) and insulin (data not shown) caused the usual shifts in mobility of the 52- and 66-kDa forms of Shc in this experiment, as detected in whole-cell extracts. The combination of insulin and PMA did not enhance tyrosine phosphorylation of 52-kDa Shc over that seen with insulin alone. Similar results were seen for LPA plus insulin (data not shown). When PMA was added 10 min prior to insulin, tyrosine phosphorylation of Shc was similar to that seen when insulin was added first. These results indicate that only insulin induces phosphorylation of Shc on tyrosine. Therefore, PMA-induced Shc phosphorylation (Fig. 7) likely occurs on serine/threonine residues.
The association of Shc with Grb2 was also examined (Fig. 8C). The amount of Grb2 detected in anti-Shc immunoprecipitates was increased by insulin, but not by PMA (Fig. 8C) or LPA (data not shown). The amount of Grb2 present in immunoprecipitates from cells incubated with PMA plus insulin, or LPA plus insulin, was similar to that seen from cells incubated with insulin alone. Taken together, these results indicate that insulin promotes the association of Shc with Grb2, but that PMA does not further enhance this association.
In these studies, we have shown that insulin and phorbol
ester can cause a synergistic activation of MAPK in Rat-1 HIR cells.
The current study used confluent, serum-starved cells, as have other
studies of MAPK activation in Rat-1 cells(27, 31) .
Synergistic activation of MAPK by PMA and insulin was observed in both
quiescent and proliferating cells (Fig. 2). It is not clear why
greater insulin-induced MAPK activation was detected in these cells in
previous studies(27, 31) . Differences may include
variations between Rat-1 HIR cell lines, differences in assay
conditions, or other factors. The results are consistent with a
previous report that PMA enhances the ability of insulin to induce MAPK
activation and mitogenesis in Balb/c 3T3 fibroblasts expressing the
human insulin receptor(5) , but are in contrast with
PMA-induced inhibition of insulin-stimulated Shc tyrosine
phosphorylation and mitogenesis observed in Chinese hamster ovary cells
transfected with the human insulin receptor and PKC(35) .
Thus, responses may vary with cell type, levels of PKC isoform
expression, and levels of insulin receptor expression.
One interpretation of the synergistic effects of insulin and PMA is that two separate signaling pathways must be engaged for maximal MAPK activation. Insulin activates one of these pathways, while PMA activates the other. It is clear that insulin and PMA elicit different responses in confluent Rat-1 cells. For example, PMA causes changes in cell shape (data not shown) and activates PLD. These effects are either absent or reduced, respectively, in response to insulin.
A second interpretation of our results is that PMA can enhance insulin responsiveness via direct effects on the insulin receptor. Although phosphorylation of the receptor by PKC reduces its tyrosine kinase activity(24) , this effect is not necessarily inhibitory to MAPK activation. Since removal of some of the tyrosine phosphorylation sites on the receptor enhances its ability to activate MAPK(3) , it is possible that phosphorylation of the receptor by PKC alters effector binding to the receptor to favor MAPK activation. However, this possibility seems unlikely in view of our observation that LPA, which unlike PMA does not activate PLD and MAPK when added alone, can also act synergistically with insulin.
A third possibility is that PMA alters the abilities of effector proteins to interact with the insulin receptor and/or to activate the MAPK pathway. Our study provides at least two observations suggesting that this is the case. First, PMA enhances phosphorylation of Shc on serine/threonine residues. Since either insulin alone or PMA plus insulin induces similar binding of Grb2 to Shc, it appears that the enhanced phosphorylation of Shc observed in response to PMA plus insulin may play additional regulatory roles. In a previous study, an insulin receptor mutant with severely impaired ability to phosphorylate Shc on tyrosine was nonetheless able to partially activate Ras(36) . These investigators suggested that further enhancement of Shc tyrosine phosphorylation could result in synergistic activation of Ras. Our data suggest that serine/threonine phosphorylation of Shc may also play a role in regulating Shc activity. While an increase in tyrosine phosphorylation of Shc, or of binding of Grb2 to Shc, was not detected in cells treated with both PMA and insulin, it is likely that serine/threonine phosphorylation enhances the interaction of Shc with receptors or effectors(25) . The role of Shc in insulin signaling is underscored by a recent report showing that epidermal growth factor and insulin preferentially phosphorylate different forms of Shc(37) . Second, our results indicate that PMA can counteract the dephosphorylation of FAK observed in response to insulin. Since the latter response appears to be deleterious for MAPK activation(16) , this effect of PMA may represent one aspect of its synergistic activity. In fact, since phosphorylated FAK has been shown to bind Grb2 (38) , maintenance or enhancement of FAK phosphorylation may represent a second ``pathway'' leading to MAPK activation in these cells.
Activation of PLD has been proposed to play a role in mitogenesis by
providing a sustained source of diglyceride for PKC activation, via
conversion of PA to diglyceride by PA phosphohydrolase. LPA, which can
be produced from PA via the action of a PA-utilizing phospholipase
A, is another potential messenger produced in response to
activation of PLD. LPA induces stress fiber formation and activates FAK
in fibroblasts(39) . PA can promote actin polymerization in
fibroblasts (40) ; this response could be mediated by LPA.
Although LPA did not activate PLD in Rat-1 HIR cells, in contrast to
results obtained by other investigators using Rat-1
fibroblasts(41) , it acted synergistically with insulin to
activate MAPK. The role of LPA as an autocrine factor produced via PLD
activation deserves further consideration.
We have shown that insulin can cause a partial activation of PLD in intact Rat-1 HIR cells. The mechanism responsible for this effect has not yet been identified. Activation of PLD by insulin may either reflect direct coupling of the insulin receptor to an effector involved in PLD activation (e.g. rho), or may be subsequent to activation of PKC. For the platelet-derived growth factor receptor, activation of phosphatidylinositol-phospholipase C is necessary for PLD activation, while interaction of the receptor with Ras GTPase-activating protein, phosphatidylinositol 3-kinase, or Syp is not required(42) . Likewise, epidermal growth factor-induced activation of PLD is dependent on activation of phosphatidylinositol-phospholipase C and PKC in fibroblasts(43) .
It is likely that PMA and LPA enhance
responsiveness to insulin by activating a separate signaling
pathway(s). The lack of enhancement of insulin's effects on
Shc-Grb2 association by PMA (Fig. 8) suggest that this is the
case. Cooperative activation of MAPK by -adrenergic
agonists and PMA was recently reported in Chinese hamster ovary cells;
the
-adrenergic response was
Ras-independent(44) . Two independent signals, one of which is
PKC-dependent, are needed for maximal activation of MAPK by the
G-protein-coupled anaphylatoxin C5a receptor(45) . Recently,
activation of MAPK by LPA in Rat-I cells was shown to be mediated by
both G proteins and ras, but to be independent of PKC(46) .
These data support the recent demonstration that more than one
signaling pathway can contribute to MAPK activation(47) , and
are consistent with the suggestion that the effects of PKC activation
on MAPK can likely be mediated at several upstream sites in the MAPK
cascade(48) .
The results described herein suggest that phorbol esters can sensitize cells to the mitogenic effects of growth factors. This capability potentially represents a significant feature of the tumor-promoting activity of phorbol esters.