(Received for publication, March 21, 1997, and in revised form, May 23, 1997)
From the Lombardi Cancer Center and Department of Pharmacology, Georgetown University, Washington, D. C. 20007
Pleiotrophin (PTN) is a developmentally regulated protein which exhibits neurite-outgrowth, mitogenic, and angiogenic properties. It has also been shown to be involved in tumor growth and metastasis. Here we used primary BEL (bovine epithelial lens) cells to investigate the signal transduction pathways involved in the mitogenic activity of recombinant PTN. PTN was purified from conditioned media of SW-13 cells transfected with the human PTN cDNA. We show that inhibitors of tyrosine kinase, mitogen-activated protein kinase, or phosphoinositide (PI) 3-kinase inhibit DNA synthesis stimulated by PTN. Analysis of tyrosine-phosphorylated proteins following PTN stimulation showed phosphorylation of two novel 190- and 215-kDa proteins in addition to SHC, ERK1, and ERK2. A mobility shift of phosphorylated ERK1 and ERK2 was detected with a panERK antibody confirming the phosphorylation of the two ERKs. Furthermore, in vitro immunocomplex kinase assay with Akt1, a natural substrate of PI 3-kinase, showed an activation of the kinase following PTN stimulation and a reversal by the PI 3-kinase inhibitor wortmannin. We conclude that the mitogenic activity of PTN is dependent on tyrosine kinase activation and utilizes the mitogen-activated protein kinase and the PI 3-kinase pathways to transduce a mitogenic signal.
Pleiotrophin (PTN)1 (1) is an 18-kDa secreted protein belonging to a new family of heparin-binding factors which includes midkine (2) and the chicken retinoic-inducible heparin-binding protein (3). Both, PTN and midkine are developmentally regulated proteins which exibit neurite outgrowth, angiogenic and mitogenic properties (reviewed in Ref. 4), and which enhance plasminogen activator activity (5). PTN and midkine share 50% of sequence homology, but they have no homology with the fibroblast growth factor family of heparin-binding growth factors which display several overlapping biological properties (reviewed in Ref. 6).
The mitogenic activity of PTN is a subject of controversy as conflicting results were reported by different laboratories. On one hand, PTN purified from tissues or expressed in bacteria and in insect cells is devoid of mitogenic activity but still promotes neurite outgrowth (7-9); however, Courty et al. (10) reported mitogenic activity after purification of PTN from bovine brain. On the other hand when expressed in eukaryotic cells, PTN is capable of stimulating thymidine incorporation and cell growth in different cell systems including fibroblasts (11), epithelial cells (11, 12), and endothelial cells (11, 13). The failure of purifying mitogenically active PTN in the former systems listed above may be explained by either loss of mitogenic activity during the purification or erroneous folding of the protein when highly expressed. This latter explanation would be in agreement with the findings of Laaroubi et al. (13) who demonstrated that PTN expressed in NIH3T3 cells is produced in two forms distinct in their structure and properties. These two forms can be separated in two peaks on a Mono S column; the first peak containing mitogenically active PTN and the second peak containing non-mitogenic PTN. Thus the mitogenic activity of PTN would depend on the balance between the active form(s) and the non active form(s). Further support of the role of PTN in cell growth is provided by experiments showing that transfection of the PTN cDNA in SW13 cells and NIH3T3 cells conferred a growth advantage in soft agar and tumorigenesis in nude mice (11, 14). In addition, recent results from our laboratory show that depletion of PTN from human melanoma and choriocarcinoma cells with ribozymes inhibits tumor growth, invasion, angiogenesis, and metastasis (15-17). Taken together these results point to an important role of PTN in cell proliferation and differentiation as well as in tumor progression. In this report we study the signal transduction pathways involved in the mitogenic activity of PTN and show an implication of the MAP kinase and PI 3-kinase pathways.
Orthovanadate, genistein, tyrphostin A25, and
pertussis toxin were purchased from LC Laboratories (Woburn, MA).
Wortmannin was from Sigma. PD98059 was obtained from Biolabs (Beverly,
MA). [3H]Thymidine and [-32P]ATP were
purchased from Amersham (Buckinghamshire, United Kingdom). Myelin basic
protein was obtained from Sigma. Bovine basic fibroblast growth factor
(bFGF) was from Collaborative Research (Bedford, MA). Anti-PTN antibody
was a generous gift of Dr. A. Seddon (American Cyanamide Co.).
Anti-phosphotyrosine antibody 4G10 was purchased from UBI (Lake Placid,
NY). Anti-panERK and anti-SHC antibodies were from Transduction
Laboratories (Lexington, KY). Anti-Akt1 antibodies were from Santa Cruz
(Santa Cruz, CA) and UBI.
Bovine epithelial lens (BEL) cells were a generous gift of Dr. J. Courty (Universite Paris 12, France) and routinely grown in Dulbecco's modified Eagle's medium supplemented with 10% FCS, 2.2 g/liter sodium bicarbonate (Life Technologies, Gaithersburg, MD), and 1 ng/ml bFGF. PTN overexpressing SW13 cells (SW-13/PTN cells clone W28), produced by stable transfection with the pRcCMV vector containing the PTN cDNA (11), were maintained in Iscove's modified Dulbecco's medium supplemented with 10% FCS (Life Technologies).
Thymidine Incorporation AssayThis assay was carried out essentially as described in Ref. 12. BEL cells were seeded in 24-well plates for 2-3 days in Dulbecco's modified Eagle's medium supplemented with 10% FCS and 2.2 g of sodium bicarbonate (Life Technologies). The cells were then serum starved for 24 h after which test samples were added. In the experiments involving inhibitors of signal transduction, the cells were pretreated with the drugs for 1 h prior to adding the growth factors. The cells were then incubated for 18 h at 37 °C and 5% CO2 and then [3H]thymidine was added. After an additional incubation period of 6 h the cells were fixed with 10% trichloroacetic acid, washed with water, and lyzed overnight with 0.3 N NaOH. Total radioactivity incorporated was counted using a Beckman scintillation counter. Each experiment included buffer or vehicle as controls.
Purification of PTN from Conditioned MediaConditioned
media from approximately 109 SW-13/PTN cells grown for 4 to
5 days in 1.5 liters of Dulbecco's modified Eagle's medium, 2% FCS
was adjusted to 50 mM Tris-HCl, pH 7.5, 0.5 M
NaCl and was passed through a 2-ml heparin-Sepharose column (Pharmacia, Piscataway). The column was then washed with 40 ml of 50 mM
Tris-HCl, pH 7.5, 0.5 M NaCl and heparin-bound proteins
were eluted with 10 ml of 50 mM Tris-HCl, pH 7.5, 1 M NaCl. The eluate was diluted to 50 mM
Tris-HCl, pH 7.5, 0.25 M NaCl and passed through a Mono S
column using an fast protein liquid chromatography system (Pharmacia). The column was washed extensively in the same buffer containing 0.45 M NaCl and the bound proteins eluted using a gradient from 0.45 to 2 M NaCl. Fractions of 1 ml were collected, quickly
aliquoted, and stored at 80 °C.
After separation in SDS-PAGE, proteins were transferred to a nitrocellulose membrane (Bio-Rad) for 2 h at 150 mAmps/gel unless indicated otherwise in 25 mM Tris, pH 8.3, 200 mM glycine, 20% methanol. The membrane was blocked in phosphate-buffered saline, 0.1% Tween 20, 5% powdered milk and probed with the antibodies at appropriate dilutions for 1 h at room temperature. The blots were then washed in phosphate-buffered saline, 0.1% Tween 20 and incubated with the appropriate secondary antibody coupled to horseradish peroxidase (Amersham) for 1 h. After additional washing in phosphate-buffered saline, 0.1% Tween 20, bound antibody was visualized using the enhanced chemiluminescence reagents system from Amersham.
ImmunoprecipitationsCells were grown to 80% confluence in 15-cm dishes, serum starved for 48 h, and then stimulated with PTN or bFGF for 10 min. Cell lysates were prepared by scrapping the cells in immunoprecipitation (IP) buffer (50 mM Tris-HCl, pH 8, 150 mM NaCl, 0.5% deoxycholic acid, 1% Nonidet P-40, 10% glycerol, 1 mM sodium orthovanadate, 1 µM okadaic acid, 50 mM sodium fluoride, 2 µg/ml leupeptin, 2 µg/ml aprotinin, 1 µg/ml pepstatin A) and incubating for 15 min at 4 °C in a rotating rack. The lysates were cleared by centrifugation and protein content was measured with the Bio-Rad protein assay kit. 0.5 to 1 mg of protein were incubated overnight at 4 ° C with 20 µl of 4G10 anti-phosphotyrosine antibody coupled to agarose beads (UBI). The beads were then washed in IP buffer and proteins were eluted by boiling in SDS-PAGE sample buffer and subjected to electrophoresis and Western blotting.
Immunocomplex Kinase AssayCell lysates, prepared as
described above and precleared with protein G-Sepharose, were incubated
for 4 h at 4 °C with 3 µg of sheep anti-Akt1 antibody (UBI).
The immunocomplexes were captured with protein G-Sepharose at 4 °C
for 1 h. The beads were then washed with 50 mM
Tris-HCl, pH 7.5, 10 mM MgCl2, 1 mM
dithiothreitol and the kinase assay was carried out as described in
Ref. 18 with a slight modification: the beads were resuspended in a
kinase buffer (50 mM Tris-HCl, pH 7.5, 10 mM
MgCl2, 1 mM dithiothreitol, 5 µM
ATP, 1 µM protein kinase A inhibitor peptide, 25 µg/ml
myelin basic protein, and 2 µCi [-32P]ATP) and
incubated for 30 min at 30 °C. The reaction was stopped by addition
of 5 × sample buffer and boiling. Samples were then electrophoresed, transferred to a nitrocellulose membrane, and the
membrane processed for autoradiography.
Unless stated otherwise data points were run in triplicate and experiments repeated at least twice. Typically the mean ± S.E. from a representative experiment is presented. As appropriate, Student's t test or ANOVA was used to assess the statistical significance of differences between measurements (Statview 4.02 program; Abacus Concepts Inc.; Berkeley, CA). The respective p values are given in the text. p < 0.05 was considered significant.
PTN was purified
from 1.5 liters of SW-13/PTN conditioned media by a two-step procedure.
The first step involved heparin-Sepharose chromatography and elution
with a buffer containing 1 M NaCl. For the second step of
purification, the 1 M NaCl eluate was diluted to 0.25 M NaCl and applied to a Mono S column on fast protein liquid chromatography. PTN was then eluted from the column with a
gradient of NaCl. PTN eluted from this column at 0.75 M
NaCl. The fractions containing the peak were analyzed by SDS-PAGE and silver staining for purity and by Western blot to identify PTN. As
shown in Fig. 1A, a >95% purification was
achieved. Two major bands of apparent molecular mass of 14 and 18 kDa
were detected by silver staining and were identified as PTN by Western
blotting (Fig. 1, A and B). Although elution of
the two PTN forms appears to overlap, it is obvious from Fig.
1A that the 14-kDa protein is eluted first and thus has a
slightly lower affinity for the column. This result is consistent with
a truncation of positively charged amino acids. As the C terminus of
the protein is rich in lysines, it is likely that the 14-kDa PTN
protein represents a C-terminally truncated form of PTN as demonstrated
using an anti-PTN antiserum raised against a 10-mer peptide from the N terminus of PTN.2
The mitogenic activity of PTN was assayed on serum-starved and growth-arrested BEL cells which have been shown to be stimulated by this growth factor (12). Fig. 1C shows that the heparin-Sepharose 1 M NaCl fraction and Mono S fractions 2 and 3 induced thymidine incorporation by 5-6-fold. Fraction 1 contained only weakly active material and fraction 4 showed no activity. Conditioned medium from cells transfected with the empty pRc/CMV vector processed for purification under the same conditions showed no mitogenic activity (data not shown). These results indicate that the purified PTN was a mixture of mitogenic and non-mitogenic proteins. Since the mitogenically active form eluted first from the column, it is conceivable that mitogenic activity is mostly due to the truncated protein. The Mono S fraction number 3 was used in the following experiments.
The Mitogenic Activity of PTN Is Independent from the Mitogenic Activity of bFGFIt has been demonstrated previously that bFGF is
a potent mitogen for BEL cells (12). To rule out the possibility of
contamination of the PTN fractions by bFGF produced endogenously by
SW-13 cells (19) and to demonstrate that the mitogenic activity of PTN
is independent from that of bFGF, we carried out the experiments shown
in Fig. 2. A dose-response curve of bFGF is shown in
Fig. 2B. The plateau of stimulation was reached at 1 ng/ml
bFGF. When BEL cells were stimulated with bFGF or PTN in the presence
of anti-bFGF neutralizing antibodies, only the bFGF activity was reduced (Fig. 2A) demonstrating that PTN is not contaminated
by bFGF. Finally, when BEL cells were stimulated with very high
concentrations of bFGF (2 and 10 ng/ml), addition of PTN still
stimulated the cells above the stimulation achieved by bFGF alone (Fig.
2C). This result indicates that the effects of PTN and bFGF
on DNA synthesis are mutually independent and suggests that the PTN
receptor is different from the FGF receptor.
Effects of Inhibitors of Tyrosine Kinase, MEK-1, and PI 3-Kinase on the Mitogenic Signal of PTN
To determine which signal transduction pathway(s) is(are) used for mitogenic signaling by PTN, we initially utilized different inhibitors of signal transduction and bFGF, as well as serum, as positive controls. bFGF is known to signal through membrane receptors with tyrosine kinase activity (20) and serum contains a mixture of factors that use different signal transduction pathways.
Pertussis toxin had no effect on DNA synthesis stimulated by PTN and
bFGF, but markedly inhibited DNA synthesis induced by serum (Fig.
3A). This result indicates that the mitogenic
signals of PTN and bFGF are not mediated via pertussis toxin-sensitive G proteins. The tyrosine kinase inhibitors genistein and tyrphostin A25
strongly inhibited DNA synthesis induced by PTN, bFGF, and serum,
whereas the tyrosine phosphatase inhibitor orthovanadate did not (Fig.
3A). Rather, orthovanadate slightly enhanced PTN-, bFGF-,
and serum-induced thymidine incorporation. These results indicate that
PTN like bFGF stimulates DNA synthesis through tyrosine kinase pathways
and that probably the PTN receptor is not a tyrosine phosphatase.
Interestingly, tyrphostin A25 was less potent against PTN than against
bFGF since 2 µM of this inhibitor inhibited the bFGF
effect by more than 60% and the PTN effect by less than 30% (p < 0.01 for inhibition of PTN versus
inhibition of bFGF). This suggests that some of the tyrosine kinases
involved in the signaling of both growth factors are distinct.
The effects of inhibitors of the MAP kinase and the PI 3-kinase pathways on PTN activity were also studied. The MEK-1 inhibitor PD98059 inhibited PTN-, bFGF-, and serum-induced DNA synthesis in a dose-dependent manner (Fig. 3B). Interestingly, PTN-stimulated mitogenesis was more sensitive than bFGF- and serum-stimulated mitogenesis. The PTN effect was completely inhibited at 10 µM of the inhibitor whereas a less than 50% inhibition was seen for the other two factors. Similarly, the PI 3-kinase inhibitor wortmannin strongly inhibited the PTN effect (by 75%; p < 0.01 for PTN versus control) and less efficiently the bFGF effect (by 35%; p < 0.01 for bFGF versus control; Fig. 3C). Serum-induced DNA synthesis was not affected by wortmannin at 10 nM (Fig. 3C). Taken together, these results indicate that the MAP kinase and the PI 3-kinase pathways are involved in the mitogenic signal of PTN as well as of bFGF. The apparent selectivity of different inhibitors signifies that the coupling of the signaling steps in the PTN and bFGF pathways are distinct and/or that additional pathways may be used by bFGF and not by PTN. Furthermore, the incomplete inhibition of DNA synthesis by wortmannin indicates that mitogenesis is only partly dependent on a functional PI 3-kinase pathway.
PTN Stimulates Protein Tyrosine PhosphorylationIn BEL cells
PTN stimulates tyrosine phosphorylation of a predominant 190-kDa
protein as assessed by Western blotting of total cell lysate or after
immunoprecipitation and Western blotting with an anti-phosphotyrosine
antibody (Fig. 4, top). A less prominent 215-kDa protein is tyrosine phosphorylated in addition to the 190-kDa
species (Fig. 4, bottom, and Fig. 5,
top). The phosphorylation of p190 and p215 was specific for
PTN since both proteins were not phosphorylated after bFGF stimulation
(Fig. 4, bottom) although ERK1 and ERK2 were found tyrosine
phosphorylated in response to bFGF (data not shown). In addition,
several low molecular weight proteins are tyrosine phosphorylated
following PTN stimulation. These proteins have apparent molecular
masses of 66, 52, 46, 44, and 42 kDa corresponding to the 3 molecular
forms of SHC and to ERK1 and ERK2, respectively (Fig. 5,
bottom). A Western blot for SHC (Fig. 5, bottom)
and for ERK (see Fig. 6) confirmed that indeed SHC and
ERK1/ERK2 were phosphorylated after PTN stimulation of the cells.
Pretreatment of the cells with the PI 3-kinase inhibitor wortmannin did
not influence phosphorylation of any of the above proteins as expected
from the separate signaling pathways.
To independently confirm phosphorylation of ERK1 and ERK2 following PTN stimulation, cell extracts from unstimulated and stimulated cells were analyzed by Western blotting using a panERK antibody. After PTN stimulation a discrete increase in upward-shifted forms of ERK1 and ERK2 were observed in the Western blots (Fig. 6). This mobility shift is typical of phosphorylated forms of the ERKs. Upon closer inspection a single band of ERK1 was detected in the control cells corresponding to the non-phosphorylated form. Following PTN stimulation, all of the ERK1 was shifted to an apparently higher molecular mass suggesting complete phosphorylation of ERK1 (Fig. 6). For ERK2, a doublet was detected in the control cells corresponding to both non-phosphorylated and phosphorylated forms. Upon PTN stimulation, all of the non-phosphorylated ERK2 shifted to the higher mobility form as expected from pERK2. These results are corroborated by the anti-phosphotyrosine blots in Fig. 5 (bottom). As expected from the separate signaling pathways, pretreatment of the cells with wortmannin did not affect phosphorylation of either ERK1 or ERK2.
Activation of the PI 3-Kinase Pathway following PTN StimulationSince wortmannin inhibited PTN-induced mitogenesis,
we decided to also assay for PI 3-kinase activation and used an
in vitro assay of the Akt1 kinase to address that. Akt1
(protein kinase B) has been previously shown to be a substrate of PI
3-kinase and to be activated by phosphorylation (21). For our studies, Akt1 was immunoprecipitated from lysates of unstimulated or stimulated cells and immunoprecipitates were used for in vitro
phosphorylation of myelin basic protein. The data presented in Fig.
7 show an increase of phosphorylation of myelin basic
protein following PTN stimulation and a reversal by pretreatment with
10 nM wortmannin. These results indicate that Akt1
activation by PTN was mediated by PI 3-kinase. We conclude from this
that PTN also activates the PI 3-kinase pathway to exert its mitogenic
effect.
PTN is a heparin-binding growth factor that is involved in cell growth and differentiation processes. It stimulates neurite outgrowth, fibroblast, endothelial, and epithelial cell growth (reviewed in Ref. 4). We report here a role of MAP kinase and PI 3-kinase pathways in the mitogenic activity of PTN. Experiments carried out in the presence of signal transduction inhibitors showed that drugs interfering with the tyrosine kinase pathway, genistein and tyrphostin A25, inhibited the mitogenic effect of PTN whereas an inhibitor of the G-protein coupled pathway, pertussis toxin, did not. This result demonstrates that PTN stimulates cell division through a tyrosine kinase pathway and that the PTN receptor is not a G protein-coupled receptor. Interestingly, the different inhibitors showed a different sensitivity of the PTN- versus the bFGF-induced DNA synthesis which indicates to us a differential sensitivity either of the respective receptor tyrosine kinases or of their coupling to the pathway downstream. Furthermore, we also found two novel, yet unidentified 190- and 215-kDa phosphoproteins in response to the PTN stimulus and not after bFGF stimulation. The apparent molecular mass of the p190 is consistent with that of a protein described to be phosphorylated after PTN stimulation of NIH3T3 cells (22). In our opinion these proteins are most likely receptor molecules for PTN.
We utilized several well characterized inhibitors to dissect the downstream signaling pathways of PTN in more detail and found that the MEK1 inhibitor PD98059 as well as the PI 3-kinase inhibitor wortmannin inhibited the mitogenic activity of PTN (Fig. 3). This demonstrates that the growth factor exerts its mitogenic effect through both the MAP kinase and the PI 3-kinase pathways. MEK1 is a component of the MAP kinase pathway which is downstream of activated receptor tyrosine kinases (23, 24). Intermediary steps involve the docking and phosphorylation of adaptor proteins (25) and we demonstrate here that the adaptor protein SHC becomes phosphorylated upon stimulation of BEL cells by PTN (Fig. 5, bottom panel). Activated SHC has been shown to bind the complex Grb2 (growth factor receptor-bound 2) and SOS (son of sevenless) which activates Ras by GTP exchange. Ras activates Raf, which in turn activates MEK1. The next step in the cascade is the activation by phosphorylation on tyrosine, serine, and threonine of the MAP kinases ERK1 and ERK2 by MEK1 which culminates in activation of several transcription factors (26). Following stimulation by PTN, ERK1 and ERK2 were indeed phosphorylated as demonstrated by Western blotting and the mobility shift of the proteins (Figs. 5 and 6). Furthermore, tyrosine kinase and MEK1 inhibitors blocked PTN-induced mitogenesis (Fig. 3, A and B), suggesting that the activation of the above signaling molecules was crucial for the growth factor activity of PTN.
Finally, we studied the participation of PI 3-kinase in the PTN signaling. PI 3-kinase is a heterodimeric protein kinase formed by two subunits of 85 and 110 kDa (27). The p85 subunit is a regulatory protein that mediates, via its SH2 domains, binding of PI 3-kinase to activated receptor tyrosine kinases. The p110 subunit possesses the catalytic domain of the protein. Following binding to a receptor tyrosine kinase, PI 3-kinase phosphorylates phosphoinositides which serve as second messengers in the activation of downstream kinases. Two pathways diverge from PI 3-kinase: one leads to phosphorylation of the p70S6K ribosomal subunit and the other one to activation of the Akt1 and Akt2 proteins (21, 28). Recent studies show that antisense Akt2 RNA inhibited tumor growth of transfected pancreatic cancer cells linking the PI 3-kinase pathway to tumor growth (29). Furthermore, PI 3-kinase and Akt were implicated in the prevention of apoptosis (reviewed in Ref. 30). Our results show that stimulation of cells with PTN leads to activation of Akt1 (Fig. 7) and this activation as well as mitogenesis of PTN was inhibited by the PI 3-kinase inhibitor wortmannin (Figs. 3C and 7). Taken together, these results show that the PI 3-kinase pathway is important for the mitogenic signaling of PTN. It is important to note that pretreatment of cells with wortmannin did not affect tyrosine phosphorylation of proteins involved in the Ras/Raf/MAP kinase pathway, indicating that it functions independently from the PI 3-kinase pathway and that both pathways are essential for a full mitogenic signal.
We thank Joannah Hackenbruck for help in some of the experiments.