Receptor-like Protein-tyrosine Phosphatase alpha  Specifically Inhibits Insulin-increased Prolactin Gene Expression*

Kirsten K. JacobDagger , Jan Sap§, and Frederick M. StanleyDagger §par

From the Dagger  Department of Medicine, § Department of Pharmacology, and  Kaplan Cancer Center, New York University Medical Center, New York, New York 10016

    ABSTRACT
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Abstract
Introduction
Procedures
Results
Discussion
References

A physiologically relevant response to insulin, stimulation of prolactin promoter activity in GH4 pituitary cells, was used as an assay to study the specificity of protein-tyrosine phosphatase function. Receptor-like protein-tyrosine phosphatase alpha  (RPTPalpha ) blocks the effect of insulin to increase prolactin gene expression but potentiates the effects of epidermal growth factor and cAMP on prolactin promoter activity. RPTPalpha was the only protein-tyrosine phosphatase tested that did this. Thus, the effect of RPTPalpha on prolactin-chloramphenicol acetyltransferase (CAT) promoter activity is specific by two criteria.

A number of potential RPTPalpha targets were ruled out by finding (a) that they are not affected or (b) that they are not on the pathway to insulin-increased prolactin-CAT activity. The negative effect of RPTPalpha on insulin activation of the prolactin promoter is not due to reduced phosphorylation or kinase activity of the insulin receptor or to reduced phosphorylation of insulin receptor substrate-1 or Shc. Inhibitor studies suggest that insulin-increased prolactin gene expression is mediated by a Ras-like GTPase but is not mitogen-activated protein kinase dependent. Experiments with inhibitors of phosphatidylinositol 3-kinase suggest that insulin-increased prolactin-CAT expression is phosphatidylinositol 3-kinase-independent. These results suggest that RPTPalpha may be a physiological regulator of insulin action.

    INTRODUCTION
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Abstract
Introduction
Procedures
Results
Discussion
References

Prolactin production is abnormal in humans with diabetes (1), and studies with animal and cell culture models of diabetes suggest that a decrease in steady-state prolactin mRNA levels secondary to decreased prolactin gene expression accounts for these findings (2, 3). The GH4 pituitary tumor cells have proven invaluable for studies of prolactin gene regulation by hormones and growth factors. Physiological insulin concentrations increase the level of prolactin and prolactin mRNA production approximately 7-10-fold in GH3 cells (4). Runoff transcription experiments indicate that the predominant effect of insulin is on the transcription of the prolactin gene. The >10-fold insulin stimulation of prolactin promoter/chloramphenicol acetyltransferase (CAT)1 reporter plasmid expression in GH4 cells confirms these results (5).

The effects of insulin are mediated through the insulin receptor that is a tyrosine kinase. Autophosphorylation of the insulin receptor upon ligand binding activates its kinase activity. The insulin receptor then phosphorylates IRS-1 at multiple sites. This activates IRS-1 for interaction with several signaling systems that have been proposed to mediate the diverse effects of insulin (6). Recently, the adapter protein Shc has also been shown to associate with the insulin receptor through interaction of the PTB domain of Shc with phosphotyrosine 960 of the insulin receptor. Thus, Shc may also act as a mediator of insulin signaling (50).

The Ras/MAP kinase pathway appears to mediate the responses of several growth factors acting through tyrosine kinases, including insulin (7). The phosphorylation of IRS-1 by the insulin receptor promotes the association of Grb2 with IRS-1 (7). This may activate Ras by recruiting SOS, a GTP/GDP exchange protein. Several studies indicate that the activation of Ras is essential for some insulin-mediated effects (8, 9). Activated Ras then recruits Raf to the plasma membrane, apparently in association with other proteins (10). This activates the kinase activity of Raf and the phosphorylation of MAP kinase kinase (MEK-1), MAP kinase, p90rsk, and nuclear transcription factors such as Elk-1 (11). Other studies indicate that phosphorylation of Shc protein and the ensuing Grb2 recruitment may be an important mechanism of Ras activation (12). A second insulin response pathway is activated by the association of phosphorylated IRS-1 with the SH2 domain of the 85-kDa subunit of PI 3-kinase. This association was shown to activate the enzyme. GTP-Ras was also shown to associate with and activate the catalytic subunit of PI 3-kinase. PI 3-kinase may participate in the increase in glucose transport in response to insulin (13) and in insulin-stimulated mitogenesis (14). However, the mechanism for these effects of PI 3-kinase is unknown.

Since tyrosine phosphorylation is the critical first step in signaling by insulin and other hormones and growth factors, dephosphorylation of phosphotyrosine must be of considerable physiological importance. The protein-tyrosine phosphatases (PTPases) can be divided into two classes: the receptor-like, membrane-spanning PTPases and the cytosolic PTPases. Receptor-like PTPases are characterized by an extracellular domain of variable length, a single membrane-spanning domain, and one or two catalytic domains on the intracellular portion of the molecule (15). Several candidate ligands for receptor-like PTPases have been defined, although none has so far been shown to modulate PTPase function (16, 17). The cytosolic PTPases have only a single PTPase domain and variable N- and C-terminal extensions. It has been postulated that these sequences target the cytosolic PTPases to specific intracellular locations (18).

These studies demonstrate a specific effect of RPTPalpha on a physiological response to insulin, activation of prolactin promoter activity. The RPTPalpha effect is specific by two criteria. First, no other PTPases tested have the same effect. Second, the response to EGF or elevated cAMP levels is not inhibited (and is actually enhanced) by RPTPalpha expression.

    EXPERIMENTAL PROCEDURES
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Abstract
Introduction
Procedures
Results
Discussion
References

Materials-- [32P]ATP (3000 Ci/mmol) and [14C]chloramphenicol (50 mCi/mmol) were obtained from ICN Biochemicals Corp. [32P]H3PO4 was from DuPont. Fast CAT®, reagents for fluorescent assay of CAT activity were purchased from Molecular Probes (Eugene, OR). Acetyl-CoA, myelin basic protein, and silica gel plates for thin layer chromatography were obtained from Sigma. Dulbecco's modified Eagle's medium containing 4.5 g/liter glucose (DMEM) was from Life Technologies, Inc., and iron supplemented calf serum was obtained from Hyclone Laboratories. LY294002 and PD98059 were from Calbiochem. Wortmannin was the gift of T. Payne (Sandoz, Basel, Switzerland). Rapamycin was provided by the Drug Synthesis and Chemistry Branch, Developmental Therapeutics Program, Division of Cancer Treatment, NCI, National Institutes of Health. All other reagents were of the highest purity available and were obtained from Sigma, Pierce, Behring Diagnostics, Bio-Rad, Eastman Kodak Co., Fisher, or Boehringer Mannheim.

Antibodies-- Antibodies to MAP kinase (anti Erk-1 and anti Erk-2), LAR, SHP1, SHP2, and horseradish peroxidase-conjugated goat anti-mouse and donkey anti-goat secondary antibodies were obtained from Santa Cruz Biotechnology (Santa Cruz, CA). Antibody to the T-cell PTPase was purchased from Oncogene Sciences. Antibodies directed against phosphotyrosine and Shc were the generous gift of Dr. J. Schlessinger (New York University Medical Center, New York). Anti-human insulin receptor antibody was supplied by Dr. K. Siddle (Cambridge, United Kingdom). Antibody to IRS-1 was the generous gift of M. White (Brigham and Women's Hospital, Boston, MA). Antibody against human influenza virus hemagglutinin was purchased from Boehringer Mannheim. Antisera against RPTPalpha and RPTPkappa were described previously (19, 20).

Plasmids-- The construction of pPrl-CAT plasmids containing -173/+75 of prolactin 5'-flanking DNA was described (4). The human insulin expression vector, pRT3HIR2, was the gift of Dr. J. Whittaker (Stony Brook, NY). The T-cell PTPase expression plasmids PTP TC and PTP TC-M (21) were generously contributed by Dr. N. Tonks (Cold Spring Harbor Laboratories) The expression plasmids for RPTPalpha (22), RPTPkappa (20), and SHP1 (previously known as PTP1C) have been previously described. The expression vector for SHP2 was provided by Dr. B. Neel (Beth Israel Hospital, Boston, MA) (23). The expression vector for the protein-tyrosine phosphatase LAR was the generous gift of Dr. B. Goldstein (Jefferson Medical College, Philadelphia, PA) (24). The HA-tagged MAP kinase expression plasmid was from Dr. E. Skolnik (New York University Medical Center). The dominant negative Raf, pRSV-Raf-C4, was from Ulf Rapp (NCI-Frederick Cancer Research and Development Center), while the dominant negative Ras, Rasn17, was the generous gift of Dr. L. Feig (Tufts University, Boston, MA).

Analysis of Prolactin Promoter Responsiveness Using Transient Transfection-- Electroporation experiments and CAT assays were performed as described (25). GH4 cells were harvested with an EDTA solution, and 20-40 × 106 cells were used for each electroporation. Trypan blue exclusion before electroporation ranged from 95 to 99%. The voltage of the electroporation was 1550 V. This gives trypan blue exclusion of 70-80% after electroporation. The transformed cells were then plated in multiwell dishes (Falcon Plastics) at 5 × 106 cells/9-cm2 tissue culture well in DMEM with 10% hormone-depleted serum. Cells were refed at 24 h with DMEM with 10% hormone depleted serum with or without insulin (1 µg/ml bovine insulin; Calbiochem), EGF (40 ng/ml recombinant human EGF; R & D Systems), or cAMP (0.1 mM, 8-(4-chlorophenylthio)-adenosine-3',5'-cyclic monophosphate; Sigma). After 48 h, the flasks were washed three times with normal saline and frozen. The cells were harvested, and CAT activity was assayed as described previously (26) except that in later experiments [14C]chloramphenicol was replaced with BODIPY chloramphenicol (Molecular Probes, Eugene, OR), and fluorescence intensity was measured using a FluorImager 575 (Molecular Dynamics, Sunnyvale, CA) with ImageQuant software.

Transfection efficiency was controlled for using an RSV-beta -galactosidase expression plasmid. Briefly, 2 µg of RSV-beta -galactosidase expression plasmid was included in all electroporations. The beta -galactosidase activity in the cell lysates was determined using o-nitrophenyl-beta -D-galactopyranoside. Transfection efficiency did not vary significantly among transfections performed at the same time. The percentage of acetylation was then corrected for minor variations in beta -galactosidase activity by converting the percentage of acetylation to percentage of acetylation/A430 beta -galactosidase activity/mg protein. The -fold stimulation or inhibition was then determined.

Immunoprecipitation and Western Immunoblot Analysis-- GH4 cells were harvested in a lysis buffer consisting of 50 mM HEPES, pH 7.5, 1% Triton X-100, 150 mM NaCl, 1.5 mM MgCl2, 1 mM EGTA, 10% glycerol, 1 mM Na3VO4, 50 mM Na4P2O7, 1 mM 4-(2-aminoethyl)-benzenesulfonylfluoride/HCl, and 10 µg/ml aprotinin. Protein was determined using the Bradford reagent (Bio-Rad). Immunoprecipitations were performed for 2-16 h at 4 °C in this buffer using 200 µg of protein. Samples were then incubated for an additional 2 h with protein A-agarose (1.5 mg/immunoprecipitation) and washed extensively. The immunoprecipitates were then dissolved in Laemmli sample buffer and analyzed by SDS-polyacrylamide gel electrophoresis using 10% gels. The proteins were then transferred to nitrocellulose membranes (Micron Separations) and immunoblotted using enhanced chemiluminescence (Pierce).

MAP Kinase Assay-- GH4 cells, transfected with HA-MAP kinase, were treated with hormones for various times or were left untreated as controls. They were then washed and frozen at -70 C. The kinase assay was performed with HA-MAP kinase immunoprecipitated with 10 µl of anti-HA. The assay was performed in a buffer containing 10 mM HEPES, pH 7.4, 50 µM [32P]ATP, 25 µM ATP, 10 mM MgCl2, 1 mM dithiothreitol, and 0.1 µg of myelin basic protein (27). The supernatant was electrophoresed on a 10% SDS-polyacrylamide gel.

32P Labeling and Immunoprecipitation of Insulin Signaling Molecules-- GH4 cells in 9-cm2 tissue culture wells were incubated for 2 h with phosphate-free DMEM containing 10% dialyzed, charcoal-treated calf serum. They were then washed and incubated for 2 h in phosphate-free DMEM containing 10% dialyzed, charcoal-treated calf serum with 0.5 mCi/ml [32P]H3PO4. Insulin was then added, and the incubation was continued for 1 h. The cells were rapidly chilled, washed three times with ice-cold saline, and frozen at -70 °C. The cells were then harvested, and immunoprecipitation was performed as described above.

Assay of Insulin Receptor Autophosphorylation-- The assay of the autocatalytic activity of the insulin receptor was performed as described by Wilden et al. (28). GH4 cells were harvested in lysis buffer (see above), and insulin receptor was partially purified by affinity chromatography on wheat germ-agarose. The insulin receptor binding activity in the eluants was then assayed. Kinase assays were performed using equal amounts of insulin receptor binding activity. Reactions (50 µl) contained 10 mM HEPES, pH 7.4, 5 mM MnCl2, 5 mM MgCl2, and 0.1% Triton X-100. Reactions were incubated with or without insulin for 10 min at 22 °C, and [32P]ATP (40 µCi/assay) was then added for an additional 20 min. The reaction was stopped by the addition of 2 × Laemmli sample buffer, and the 32P-labeled proteins were analyzed by SDS-polyacrylamide gel electrophoresis.

    RESULTS
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Abstract
Introduction
Procedures
Results
Discussion
References

Inhibition of Prolactin-CAT Expression by RPTPalpha -- GH4 cells were transfected with the prolactin-CAT reporter plasmid without or with increasing amounts of an expression vector for RPTPalpha . The cells were refed after 24 h, and 1 µg/ml insulin, 40 ng/ml EGF, or 0.1 mM cAMP was added to the cultures for an additional 24 h. The cells were harvested, and CAT activity was assayed to determine the effect of RPTPalpha on hormone-increased prolactin-CAT expression. Insulin increases prolactin-CAT expression almost 20-fold in GH4 cells transfected with only prolactin-CAT and insulin receptor (Fig. 1A). This stimulation is dramatically decreased by co-transfection of small amounts of an expression vector for RPTPalpha . Half-maximal inhibition of insulin-increased prolactin-CAT expression is achieved using only 0.5 µg of expression vector for RPTPalpha , and maximal inhibition of >90% is achieved with 15 µg or more of RPTPalpha . Maximal inhibition is achieved without a significant reduction in basal prolactin-CAT expression (1.30 ± 0.5% acetylation/10 µg of protein/h versus 1.35 ± 0.5% acetylation/10 µg of protein/h in control cells), although basal prolactin-CAT transcription decreased with the highest amounts of expression vector for RPTPalpha (0.91 ± 0.14% acetylation/10 µg of protein/h using 50 µg and more of RPTPalpha expression vector). In contrast to its inhibitory effect on insulin-increased prolactin promoter activity, the increase in prolactin-CAT expression in EGF- and cAMP-treated cells is augmented by expression of RPTPalpha . EGF increased prolactin-CAT expression 13-fold in control transfections, but this was increased to 36-fold when 15 µg of RPTPalpha expression vector were included. Likewise, cAMP increased prolactin-CAT 12-fold in control transfections but 20-fold with 15 µg of RPTPalpha . Further, the increase in prolactin-CAT expression due to EGF or cAMP was never significantly below that seen in control cultures, even using amounts of RPTPalpha expression vector that totally abolish the effect of insulin (50 and 150 µg; data not shown). Thus, under conditions where identical amounts of enzyme are produced, RPTPalpha expression specifically inactivates the insulin signaling pathway, while it enhances EGF and cAMP signaling.


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Fig. 1.   Effect of expression of RPTPalpha on insulin-increased prolactin-CAT. GH4 cells were cotransfected with 15 µg of Prl-(-173/+75)-CAT and with 5 µg of an expression vector for the human insulin receptor, pRT3HIR2. A vector expressing either RPTPalpha (A) or RPTPkappa (B) under the control of the cytomegalovirus promoter was included at the concentrations indicated in the figure. The average percentage of acetylation/10 µg of protein in control and insulin-, EGF-, or cAMP-treated cultures was determined and adjusted for beta -galactosidase expression, and the CAT activities from cells incubated with hormones were compared with control levels to determine the -fold stimulation (Fold-Control). The results are from three separate experiments done in duplicate.

A similar experiment performed with RPTPkappa (Fig. 1B) shows no significant inhibition of insulin-, EGF- or cAMP-increased prolactin-CAT expression at any concentration of expression vector tested. Insulin increased prolactin-CAT expression 21-fold in control cells and 19-fold in cells cotransfected with 32 µg of expression vector for RPTPkappa . Likewise, cAMP increased prolactin-CAT expression 17-fold in control cells and 15-fold in cells cotransfected with 32 µg of RPTPkappa expression vector. Only the effect of EGF was significantly affected by expression of RPTPkappa . EGF increased prolactin-CAT expression 18-fold in control cells but only 10-fold in cells expressing RPTPkappa (p < 0.05). The significant reduction in the effect of EGF and data indicating that RPTPkappa is overexpressed in GH4 cells cotransfected with the RPTPkappa expression vector suggest that the lack of effect of cotransfection with RPTPkappa is not due to insufficient expression of RPTPkappa , but results from the inability of RPTPkappa to regulate insulin signaling events.

The Effect of RPTPalpha Is Specific Both for Insulin and for RPTPalpha -- Several other PTPases were found to be without effect on insulin-increased prolactin-CAT expression. The receptor-like PTPases are classified by the structure of their extracellular domain. RPTPalpha is a type IV PTPase with a short glycosylated extracellular domain. RPTPkappa is a receptor-type PTPase of class II and is characterized by one Ig- and several fibronectin type III-like repeats in its extracellular domain. LAR is a receptor-like PTPase of type II that has three Ig-like repeats and nine fibronectin III-like repeats in its extracellular domain (29). PTP TC, PTP TC-M, SHP1, and SHP2 are cytosolic phosphatases. The T cell PTPase PTP-TC is a 48-kDa protein that is found exclusively in the particulate fraction of cellular lysates. Truncation of this PTPase with trypsin yields a 37-kDa protein with constitutive PTPase activity. We have used a plasmid PTP TC-M that has a premature stop codon inserted into the T cell PTPase cDNA so that it produces only this 37-kDa, constitutively active form of T-cell PTPase (21). SHP1 and SHP2 are cytosolic PTPases that have two SH2 domains in their N-terminal regions. These SH2 domains restrict the potential substrates for these phosphatases. The expression of the phosphatases used was checked by Western blotting (Fig. 2A). This technique does not allow the comparison of actual amounts of protein expressed; however, the relative difference in amount of the PTPase in control versus transfected cultures can be determined. All of the phosphatases except the truncated form of the T cell phosphatase, PTP TC-M, were found to be significantly overexpressed in transfected cells, and the level of overexpression was similar in all cases. The truncated T cell PTPase was not detected. This probably results from the removal of the epitope for the monoclonal antibody that was used for detection of this protein, since expression of this protein significantly affected EGF-increased prolactin-CAT expression (see below; Fig. 2B).


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Fig. 2.   Effect of various phosphatases on stimulated prolactin-CAT expression. GH4 cells were cotransfected with 15 µg of Prl-(-173/+75)-CAT, 2 µg of RSV-beta -galactosidase, and with 5 µg of an expression vector for the human insulin receptor, pRT3HIR2 without or with 10 µg of expression vector for the phosphatases shown. All phosphatase expression vectors used the same promoter. The cultures were then incubated in hormone-depleted medium for 24 h. The medium was exchanged, and hormones were added for an additional 24 h. A. Some cultures were scraped in lysis buffer, and various amounts of protein were electrophoresed on SDS-polyacrylamide gels and blotted to nitrocellulose as described under "Experimental Procedures." Western blot analysis was then performed using specific antibodies to the various PTPases as indicated above the lanes. The migrations of molecular weight standards are shown on the left of each immunoblot, while the arrow on the right indicates the expected size of the expressed phosphatase. The (-)-lane indicates protein from cells electroporated with vector alone, and the (+)-lane shows protein from cells electroporated with an expression vector for a PTPase. B, the cells were harvested, and CAT enzyme activity was determined. The average percentage of acetylation/10 µg of protein in control and hormone-treated cultures was determined and adjusted for beta -galactosidase expression, and the hormone incubations were compared with control levels to determine the -fold stimulation by insulin (Fold-Control). The results are from three separate experiments done in duplicate. The vector control had no effect on basal or stimulated prolactin-CAT expression. Basal prolactin-CAT expression was not significantly changed by expression of the PTPases (control, 1.66 ± 0.3%; RPTPalpha , 1.93 ± 0.4%; RPTPkappa , 2.53 ± 0.8%; PTP TC, 3.15 ± 0.2%; PTP TC-M, 1.83 ± 0.23%; SHP1, 2.4 ± 0.8%; SHP2 3.17 ± 0.39; LAR, 3.92 ± 0.99 (percentage of acetylation/10 µg of protein)). *, significance as follows: 0.05 > p > 0.25. **, significance as follows: 0.025 p > 0.01.

In control cells, prolactin-CAT expression was increased 11-fold by insulin, 4-fold by EGF, and 8-fold by cAMP. Co-transfection with RPTPalpha significantly inhibited the increase in prolactin-CAT expression seen in insulin-treated cells (2-fold control levels). RPTPalpha significantly enhanced the ability of EGF and cAMP to increase prolactin-CAT expression, consistent with the initial dose-response study (above). EGF increased prolactin-CAT expression almost 25-fold in RPTPalpha -expressing cells. This is >6-fold higher than the increase due to EGF in control transfections. cAMP-increased prolactin-CAT expression was also increased to 18-fold in RPTPalpha -expressing cells, and this is approximately 2.5-fold higher than in control transfections. Thus, the effect of RPTPalpha to reduce insulin-increased prolactin-CAT expression is not a general effect to block activation of prolactin-CAT expression but is hormone-specific. The effect of RPTPalpha to inhibit insulin-increased prolactin-CAT expression is also phosphatase-specific, since none of the other PTPases co-transfected in GH4 cells significantly reduced insulin-increased prolactin-CAT expression. Both insulin and EGF increased prolactin-CAT expression significantly more in cells expressing the T cell PTPase, PTP TC, than in control cells. Expression of the truncated TC-PTPase, PTP TC-M, increased the effect of EGF and cAMP on prolactin-CAT transcription. Finally, expression of SHP1 significantly increased the effect of EGF to activate prolactin-CAT expression. Neither SHP2 nor LAR was seen to have any effect on prolactin-CAT expression or its response to mediators.

These effects were confirmed using cells stably expressing high levels of RPTPalpha or RPTPkappa . GH4 cells were electroporated with vectors expressing the neomycin resistance gene and either RPTPalpha or RPTPkappa expression vectors. Clones that were resistant to G418 were selected. Fig. 3A shows levels of RPTPalpha and RPTPkappa in control cells and in representative RPTPalpha - and RPTPkappa -expressing clones, RPTPalpha 23 and RPTPkappa 5. RPTPalpha levels are low in control and in the RPTPkappa 5 clone (Fig. 3A). High levels of RPTPalpha are seen only in the clone RPTPalpha 23 that has the stably integrated RPTPalpha cDNA. Likewise, RPTPkappa levels are low in GH4 cells and in RPTPalpha 23 cells, while RPTPkappa levels are high in the clone RPTPkappa 5 that has an incorporated RPTPkappa cDNA.


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Fig. 3.   Prolactin-CAT expression in GH4 cells stably transformed with RPTPalpha and RPTPkappa . A, cell lysates prepared from control GH4 cells (lanes 1 and 4), RPTPalpha -transformed GH4 cells (lanes 2 and 5), and RPTPkappa -transformed GH4 cells (lanes 3 and 6) were electrophoresed on 10% SDS gels as described. The proteins were transferred to nitrocellulose membranes and Western blotted with antibody to RPTPalpha (lanes 1-3) or antibody against RPTPkappa (lanes 4-6). The position of migration of RPTPalpha and RPTPkappa is indicated. B, GH4 cells stably expressing RPTPalpha or RPTPkappa and control GH4 cells were transfected with 15 µg of Prl-(-173/+75)-CAT and with 5 µg of an expression vector for the human insulin receptor, pRT3HIR2. The cultures were then incubated in hormone-depleted medium for 24 h. The medium was exchanged, and hormones were added for an additional 24 h. The cells were harvested, and CAT enzyme activity was determined. The average percentage of acetylation/10 µg of protein in control and insulin-treated cultures was determined, and the insulin incubations were compared with control levels to determine the -fold stimulation by insulin (Fold-Control). The results are from three separate experiments done in duplicate.

Prolactin-CAT expression in insulin-, EGF- and cAMP-treated control cells and RPTPalpha - or RPTPkappa -overexpressing transformants is shown in Fig. 3B. Insulin treatment results in a 10-fold increase in prolactin-CAT expression in control cells, while insulin-increased prolactin-CAT expression is 15-fold in RPTPkappa -overexpressing cells. Insulin-increased prolactin-CAT expression is reduced 75%, to 2.5-fold, in GH4 cells overexpressing RPTPalpha . In contrast to the observations made using transient expression of RPTPalpha , experiments with cells stably overexpressing RPTPalpha showed no effect of RPTPalpha on increased prolactin-CAT expression due to EGF or cAMP. This could result from a failure to select cells expressing appropriate levels of RPTPalpha , since it is clear that the ability of RPTPalpha to enhance the effects of EGF and cAMP is dose-dependent (see Fig. 1). Alternately, it may result from the long term adaptation of the stably transformed cells. Levels of basal prolactin-CAT expression are also similar in the control (1.03 ± 0.3% acetylation/10 µg of protein) and in RPTPalpha -expressing clone 23 (1.49 ± 0.3% acetylation/10 µg of protein) and in the RPTPkappa -expressing clone 5 (0.85 ± 0.15% acetylation/10 µg of protein). Results from the RPTPalpha -expressing clone alpha 23 and RPTPkappa -expressing clone kappa 5 are typical. Four other alpha -expressing clones and three other kappa -expressing clones were also tested and gave identical results.

Insulin Receptor Phosphorylation in RPTPalpha - and RPTPkappa -overexpressing Cells-- Ligand binding to the insulin receptor results in autophosphorylation of several tyrosines on the insulin receptor beta -subunit. Some of these phosphorylations activate the receptor kinase, while others have been shown to be important as binding sites for signaling molecules. It was possible that RPTPalpha rapidly dephosphorylated the insulin receptor and interfered with its signaling. Experiments done to test this hypothesis are shown in Fig. 4. The magnitude of insulin stimulation of tyrosine phosphorylation of transfected human insulin receptor in control cells and in cells also transfected with RPTPalpha was determined by immunoprecipitation and Western blotting with antibody to phosphotyrosine (Fig. 4A). A 6-min insulin treatment results in a large increase in tyrosine phosphorylation of the insulin receptor in cells transfected with the human insulin receptor alone (control). However, there is no significant loss of insulin-increased human insulin receptor phosphorylation in cells transiently transfected with both the human insulin receptor and with RPTPalpha . These results are confirmed in stably transformed cells (Fig. 4B). An antibody that recognizes both the endogenous rat insulin receptor and the transfected human insulin receptor was used for these experiments. Neither the clone overexpressing RPTPalpha nor the clone overexpressing RPTPkappa shows any loss of insulin-increased tyrosine phosphorylation of the insulin receptor. Further, experiments using lysates from cells metabolically labeled with [32P]H3PO4 did not demonstrate any differences among control GH4 cells and clones expressing RPTPalpha or RPTPkappa in insulin-increased incorporation of 32P into insulin receptor (data not shown). Thus, expression of RPTPalpha does not indirectly reduce the level of Ser/Thr phosphorylation of the insulin receptor.


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Fig. 4.   Insulin receptor phosphorylation and autocatalytic activity in cells transfected with PTPases. A, control GH4 cells were transfected with 5 µg of pRT3HIR-2 alone (lanes 1 and 2) or RPTPalpha (lanes 3 and 4). The cells were incubated in hormone-depleted medium for 24 h. Insulin (1 µg/ml) was then added for 6 min. The medium was rapidly removed, and the cultures were washed with normal saline at 4 °C. Lysates were prepared, and immunoprecipitation was performed as described using 200 µg of lysate and a human insulin receptor-specific monoclonal antibody, 83-14 (from K. Siddle, London, UK). The immunoprecipitates were then separated on SDS-polyacrylamide gels and transferred to nitrocellulose. Western analysis was performed using a polyclonal antibody to phosphotyrosine and ECL reagents (Pierce). B, control cells (lanes 1 and 2) and cells stably expressing RPTPalpha (lanes 3 and 4) or RPTPkappa (lanes 5 and 6) were incubated in hormone-depleted medium for 24 h. The cultures were then treated as above except that immunoprecipitation was performed using a polyclonal antibody that recognizes the insulin receptor of the rat. C, the autocatalytic activity of wheat germ agglutinin-purified insulin receptor from control cells (lanes 1 and 2) and cells stably expressing RPTPalpha (lanes 3 and 4) or RPTPkappa (lanes 5 and 6) was determined. After partial purification of the insulin receptors from the various cell types, the insulin binding activity of the eluted insulin receptors was assayed using 125I-iodinated insulin. Equal amounts of binding activity were used for each assay. The reaction was stopped with SDS electrophoresis buffer, and the insulin receptor was resolved by electrophoresis on a 10% SDS-polyacrylamide gel. The position of migration of the insulin receptor is indicated.

Insulin Receptor Kinase activity in RPTPalpha - and RPTPkappa -overexpressing Cell Lines-- These results suggested that RPTPalpha did not reduce the general level of tyrosine phosphorylation of the insulin receptor. However, dephosphorylation of a phosphotyrosine critical to the activation of insulin receptor tyrosine kinase cannot be ruled out by these experiments. Therefore, the catalytic activity of the insulin receptor was directly tested. Insulin increases the autocatalytic activity of the insulin receptor 4.2-fold in GH4 cells (Fig. 4C). Insulin increased the kinase activity of its receptor 4.3-fold in cells overexpressing RPTPalpha and 3.6-fold in cells overexpressing RPTPkappa .

IRS-1 and Shc Phosphorylation in RPTPalpha - and RPTPkappa -overexpressing Cell Lines-- The previous experiments suggest that RPTPalpha does not decrease levels of insulin receptor kinase activity and that RPTPalpha does not reduce the increase in insulin receptor phosphorylation in insulin-treated cells. However, it is possible that RPTPalpha specifically dephosphorylates a tyrosine on the insulin receptor that impairs its ability to transmit signal to downstream events. Such a condition could occur if dephosphorylation by RPTPalpha inactivates a substrate binding site. Therefore, the effect of RPTPalpha expression on phosphorylation of insulin receptor substrates was examined. Two substrates of the insulin receptor kinase, IRS-1 and Shc, have been shown to be intermediates for some of the actions of insulin (6). Insulin increases the phosphorylation of IRS-1 3 ± 0.25-fold in GH4 cells (Fig. 5A). Levels of IRS-1 phosphorylation in GH4 cells stably expressing RPTPalpha were increased 3.5 ± 0.4-fold by insulin, while in RPTPkappa -overexpressing cells IRS-1 phosphorylation was increased 3.2 ± 0.15-fold by insulin. Thus, IRS-1 phosphorylation does not appear to be affected by overexpressing RPTPalpha or RPTPkappa .


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Fig. 5.   IRS-1 and Shc phosphorylation in cells stably expressing RPTPalpha and RPTPkappa . Control GH4 cells (lanes 1 and 2) and GH4 cells expressing high levels of RPTPalpha (lanes 3 and 4; A23) or RPTPkappa (lanes 5 and 6; K5) were metabolically labeled for 2 h with [32P]H3PO4. Insulin was then added for 1 h ((+)-lanes). The cultures were washed and frozen, and a cell lysate was prepared as described above. A, 200 µg of each lysate was immunoprecipitated with an antibody to IRS-1 (from M. White, Joslin Diabetes Center, Boston, MA). B, 200 µg of each lysate was immunoprecipitated with antibody against Shc (from J. Schlessinger, NYU Medical Center, New York). The immunoprecipitates were resolved by SDS-polyacrylamide gel electrophoresis, and the IRS-1 and Shc bands were quantitated using a Molecular Dynamics PhosphorImager and ImageQuant software. CHO, Chinese hamster ovary.

Insulin/growth factor-increased Shc phosphorylation has been linked to recruitment of Grb-2/SOS and Ras activation in some cell lines (12). The extent of Shc phosphorylation in insulin-treated cells (Fig. 5B) was determined. Shc levels are very low in GH4 cells, and only the 46-kDa form of Shc is immunoprecipitated in GH4 cells. In comparison, phosphorylation of all three forms of Shc is seen in Chinese hamster ovary cells (lanes 1-6 versus lanes 7 and 8). Insulin increased the phosphorylation of 46-kDa Shc by only 3-fold in GH4 cells versus 8-fold in Chinese hamster ovary cells. However, no difference is seen between levels of phosphorylation of this Shc isoform in control GH4 cells or in cells overexpressing RPTPalpha (lanes 1 and 2 versus lanes 3 and 4).

Dominant Negative Inhibition of Ras and Raf in GH Cells-- Dominant negative inhibitors of Ras were used to determine whether the Ras/Raf/MAP kinase signaling pathway might be involved in insulin signaling to prolactin-CAT expression. GH4 cells were cotransfected with the prolactin-CAT reporter and the human insulin receptor. Some electroporations also contained either p21S17N-Ras, a dominant negative Ras (30), or Raf-C4, which competes with wild type Raf for binding to Ras and Ras-related proteins and inhibits the downstream effects of these molecules (31). Insulin increased prolactin-CAT expression 10-fold in control cells (Fig. 6). Cotransfection of p21 S17N-Ras had no effect on insulin-increased prolactin gene expression, which was 8-9-fold at 10 µg of cotransfected inhibitor (Fig. 6A). Prolactin-CAT expression increased by cAMP was also not affected. It was 11-fold in control cells and 8-9-fold in p21 S17N-Ras-transfected cells. This does not result from failure of the p21 S17N-Ras to be expressed in GH4 cells, since EGF-increased prolactin-CAT expression was strongly inhibited by p21 S17N-Ras expression. EGF increased prolactin-CAT expression 7-fold in control GH4 cells, whereas in p21 S17N-Ras cotransfected cells EGF did not significantly increase prolactin-CAT expression.


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Fig. 6.   The effect of inhibition of Ras signaling on prolactin-CAT expression and MAP kinase activation. GH4 cells were cotransfected with 15 µg of Prl-(-173/+75)-CAT and with 5 µg of an expression vector for the human insulin receptor, pRT3HIR2 without (left) or with 10 µg (center) of Raf-C4, or with 10 µg (right) of p21S17N-Ras. The cultures were then incubated in hormone-depleted medium for 24 h. The medium was exchanged, and hormones were added for an additional 24 h. The cells were harvested, and CAT enzyme activity was determined. The average percentage of acetylation/10 µg of protein in control and insulin-treated cultures was determined, and the insulin incubations were compared with control levels to determine the -fold stimulation by insulin (Fold-Control). The results are from three separate experiments done in duplicate. Basal prolactin-CAT levels were not affected by cotransfection of either Raf-C4 or p21S17N-Ras. Basal levels of prolactin-CAT expression varied in these experiments from a low of 0.67 to 7.8% acetylation/10 µg of protein, but basal prolactin-CAT levels were 88 ± 12% of control levels in cells transfected with 10 µg of Raf-C4 and 114 ± 15% of control in cells transfected with 10 µg of p21S17N-Ras. Parallel cultures were used to determine hormone-responsive MAP kinase activity in GH4 cells expressing inhibitors of prolactin-CAT expression. GH4 cells were transfected with Raf-C4, p21S17N-Ras, or RPTPalpha or were mock-transfected as a control. After 24 h, 1 µg/ml of insulin or 20 ng/ml EGF was added to some of the cultures. The cells were incubated with hormones for 5 min (B) or 2 h (C) and then quickly chilled on ice and washed with normal saline at 4 °C. 100 µg of cell lysate was precipitated with anti-HA antibody and assayed for MAP kinase activity as described under "Experimental Procedures." The phosphorylation of myelin basic protein from the different treatments was quantitated with a Molecular Dynamics PhosphorImager using ImageQuant NT software. The results of four separate experiments were averaged to provide these data.

Dominant negative Raf-C4 resulted in the almost complete inhibition of both insulin- and EGF-increased prolactin gene expression (Fig. 6A). Insulin-increased prolactin-CAT expression is reduced from 10- to 3-fold, and the EGF effect is lowered from 7- to 2.5-fold in cells expressing Raf-C4. The effect of cAMP is not diminished in these experiments. Raf-C4 acts by binding to GTPases such as Ras and competing with functional substrate. However, Raf-C4 binds to numerous non-Ras GTPases. These results imply that the effect of insulin to increase prolactin-CAT expression is Ras-independent but that it is dependent on a Ras-related GTPase. The effect of cAMP on prolactin gene expression is independent of Ras, and this agrees with previous studies that suggest that the effect of cAMP is mediated through cAMP-dependent protein kinase A (32, 33).

Effect of Insulin on MAP Kinase Activity in GH4 Cells Expressing Inhibitors-- Insulin increases MAP kinase activity in a Ras/Raf-dependent manner in several cell lines. MAP kinase activity in cells treated for 6 min with insulin or EGF or left untreated as controls was determined (Fig. 6B). Insulin increased MAP kinase activity 10-fold in control cells. This is not affected by cotransfection with dominant negative Ras. However, MAP kinase activity was increased only 4-fold in insulin-treated cells that were cotransfected with Raf-C4. Thus, dominant negative Raf reduces the effect of insulin by 60%. Cotransfection with RPTPalpha reduces the effect of insulin approximately 75%. The effect of EGF is reduced 40% by dominant negative Raf and 33% by dominant negative Ras, but it is not affected by overexpression of RPTPalpha .

The effect of inhibitors on insulin- and EGF-increased MAP kinase activity paralleled effects of the same inhibitors to reduce insulin- and EGF-increased prolactin-CAT expression. However, the magnitude of the changes in early stimulation of MAP kinase was not as great as the inhibition of prolactin-CAT expression. Several studies have indicated that differentiation-enhancing effects of growth factors correlate with the prolonged phase of MAP kinase activation and not with the acute, transient effects (34). Therefore, the effect of insulin or EGF to increase MAP kinase activity was determined after 2 h in control GH4 cells and in GH4 cells co-transfected with dominant negative p21 Ras, Raf-C4, or RPTPalpha (Fig. 6C). Insulin treatment resulted in a 3.5-fold increase in MAP kinase activity in control cells. This is not significantly different from the 3.1-fold stimulation seen in EGF-treated cultures. Expression of dominant negative Raf prevented both of these effects. MAP kinase activity in cultures expressing dominant negative Ras was increased 2-fold by insulin but was not increased by EGF. MAP kinase activity was not increased by insulin in cells co-transfected with RPTPalpha . EGF-increased MAP kinase activity was increased in RPTPalpha -co-transfected cells to 2.8-fold control. Thus, insulin- and EGF-increased steady-state activation of MAP kinase and increased prolactin-CAT expression exhibit identical responses to p21S17N Ras, to Raf-C4, and to RPTPalpha .

Inhibition of MEK with PD098059-- These experiments suggested that a Ras-independent activation of MAP kinase by insulin might mediate the increase in prolactin gene expression in insulin-treated cells. The experiment shown in Fig. 7 eliminates this possibility. Incubation of GH4 cells with the inhibitor of MEK, PD098059, for 2 h before the addition of hormones eliminates the ability of insulin and cAMP to activate MAP kinase and reduces the activation of MAP kinase by EGF from 80- to 30-fold (Fig. 7A). Prolactin-CAT expression in response to these hormones is not significantly affected by PD098059 under the same conditions (Fig. 7B). Thus, insulin increased prolactin-CAT expression is MAP kinase-independent. Numerous other negative results support this conclusion. First, Raf kinase assays performed in control GH4 cells, A23 (RPTPalpha -expressing) cells, and in K5 (RPTPkappa -expressing) cells show the same level of insulin and EGF activation of both c-Raf-1 and B-Raf kinase (data not shown). Second, a dominant negative MEK and dominant negative MAP kinase do not inhibit prolactin gene transcription (data not shown). Third, constitutively active MEK does not activate prolactin gene transcription (data not shown). Fourth, a MAP kinase phosphatase does not block the action of insulin, and phosphatase-inactive MAP kinase phosphatase does not increase prolactin gene expression (data not shown).


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Fig. 7.   Inhibition of MEK with PD098059. GH4 cells were cotransfected with 15 µg of Prl-(-173/+75)-CAT, 1 µg of HA-MAP kinase, and 5 µg of an expression vector for the human insulin receptor, pRT3HIR2. The cultures were then incubated in hormone-depleted medium for 24 h. The cells were refed after 24 h, and 40 µM PD098059 was added to half of the cultures. Two hours after the addition of the inhibitor, 1 µg/ml insulin, 40 ng/ml EGF, or 0.5 mM 8-CPT-cAMP was added to selected wells. A, the cells were harvested 24 h after the addition of hormones. The average percentage of acetylation/10 µg of protein in control and insulin-treated cultures was determined, and the insulin incubations were compared with control levels to determine the -fold stimulation by insulin (Fold-Control). The results are from three separate experiments done in duplicate. B, the cells were incubated with hormones for 6 min and then quickly chilled on ice, washed, and frozen. 100 µg of cell lysate was precipitated with anti-HA antibody and assayed for MAP kinase activity as described under "Experimental Procedures." The phosphorylation of myelin basic protein from the different treatments was quantitated with a Molecular Dynamics PhosphorImager using ImageQuant NT software. The results of three separate experiments were averaged to provide these data.

Effect of Inhibition of PI 3-Kinase and p70S6 Kinase on Prolactin-CAT Expression-- LY294002 and wortmannin inhibit PI 3-kinase activity and insulin-stimulated glucose transport in 3T3-L1 adipocytes. Therefore, LY 294002 was used at a concentration of 50 µM and wortmannin was used at a concentration of 20 µM to determine the effect of insulin, EGF, and cAMP in cells where PI 3-kinase was inhibited. Insulin increases prolactin-CAT expression 11-fold over untreated cells with or without LY294002. However, LY294002 alone causes an increase in prolactin-CAT expression over untreated cells. Thus, it is difficult to determine if the effect of LY294002 is inhibition of the insulin response or whether LY294002 and insulin are both affecting the same pathway to increase prolactin-CAT expression. The effect of EGF is doubled by LY294002 from 6- to 14-fold, and the effect of cAMP is tripled from 7- to over 20-fold the levels seen in untreated cells in the same experiment. In cells treated with 20 µM wortmannin, insulin increased prolactin-CAT expression was only 25% (2.5-fold) of the insulin stimulation seen in control cells (11-fold; Fig. 8). Both EGF- and cAMP-increased prolactin-CAT expression were increased by wortmannin treatment (Fig. 8). Thus, the effects of EGF and cAMP are independent of PI 3-kinase, while insulin-increased prolactin-CAT expression may be PI 3-kinase-dependent.


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Fig. 8.   Insulin-increased prolactin-CAT expression in cells treated with PI 3-kinase and p70S6 kinase inhibitors. GH4 cells were cotransfected with 10 µg of Prl-(-173/+75)-CAT, 2 µg of RSV-beta -galactosidase, and 5 µg of an expression vector for the human insulin receptor, pRT3HIR2. The cultures were then incubated in hormone-depleted medium for 24 h. The cells were refed after 24 h, and 50 µM LY294002, 1 µM rapamycin, or 20 µM wortmannin was added to the indicated cultures. Two hours after the addition of the inhibitor, 1 µg/ml insulin, 40 ng/ml EGF, or 0.5 mM 8-CPT-cAMP was added to selected wells. The cells were harvested 24 h after the addition of hormones. The average percentage of acetylation/10 µg of protein in control and insulin-treated cultures was determined, and the insulin incubations were compared with control levels to determine the -fold stimulation by insulin (Fold-Control). The results are from three separate experiments done in duplicate.

Another potential insulin signaling pathway is mediated by p70S6 kinase that is activated by phosphorylation through TOR (target of rapamycin). To examine the possibility that insulin-increased prolactin-CAT expression was p70S6 kinase-mediated, GH4 cells were treated with rapamycin. The insulin-increased prolactin-CAT expression in untreated cultures was 14-fold control levels. This was not significantly affected by rapamycin, 11.7-fold (Fig. 8). However, both EGF- and cAMP-increased prolactin-CAT expression were inhibited approximately 75% by rapamycin falling from 8- to 2-fold.

    DISCUSSION
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Abstract
Introduction
Procedures
Results
Discussion
References

Stimulation of prolactin gene transcription is a well established and physiologically relevant response to insulin (32, 35). We have used the responsiveness of the prolactin promoter to insulin and other factors as a defined assay to study the effect of PTPases on insulin signaling. The data presented document strikingly specific effects of RPTPalpha on insulin-dependent gene transcription. First, overexpression of RPTPalpha inhibits the insulin-mediated increase in prolactin promoter activity. These results are observed both in transiently and stably transfected cells. Second, the overexpression of RPTPalpha does not reduce either EGF- or cAMP-increased prolactin promoter activity, but, in transient expression experiments, RPTPalpha expression augmented the increase in prolactin-CAT expression due to EGF and cAMP. This demonstrates that the effect of RPTPalpha overexpression does not involve a general inhibition of growth factor or second messenger responses. Finally, none of the other phosphatases tested inhibited insulin-increased transcription from the prolactin promoter.

Others have reported studies on the important role of the LAR PTPase as a potential negative regulator of insulin signaling (36). By contrast, we did not observe any effect of LAR expression on the regulation of the prolactin promoter by insulin in GH4 cells (Fig. 2B). Thus, our data may seem to conflict with the reports on the control of insulin signaling by LAR. However, (a) distinct PTPases may regulate different insulin signaling pathways, (b) distinct PTPases may contribute to regulation of insulin signaling in different cell types, (c) more than one PTPase may act together within the same cell, or (d) different PTPases may control insulin signaling with varying degrees of specificity (see below).

Recently, Moller et al. (37) showed that substratum detachment of insulin-treated, insulin receptor-expressing BHK cells was reduced in cells that also expressed either RPTPalpha or RPTPepsilon . This was interpreted as evidence that expression of either RPTPalpha or RPTPepsilon blocked insulin signaling. However, these data might reflect an effect of RPTPalpha or RPTPepsilon expression on cell adhesion unrelated to a physiological insulin response, since the effect of other factors was not tested. In our assay system, the expression of RPTPalpha has no effect on basal or on EGF- or cAMP-increased prolactin-CAT transcription. This makes it clear that the effect of RPTPalpha on prolactin promoter activity is probably mediated through a direct effect on the insulin signaling pathway. This is further supported by the RPTPalpha inhibition of MAP kinase activation by insulin.

The insulin signaling pathway to gene expression is not currently defined. However, a number of signaling molecules have been identified that may also participate in signaling to gene transcription. Therefore, experiments were performed to determine whether expression of RPTPalpha alters the response of these molecules to insulin.

Phosphorylation of the insulin receptor was substantially the same in control GH4 cells and in GH4 cells expressing RPTPalpha , either transiently (Fig. 4A) or stably (Fig. 4B). Previously published studies (37) suggested that insulin receptor was hypophosphorylated in RPTPalpha -overexpressing cells. However, in that study, both the insulin receptor and RPTPalpha were highly overexpressed using the 293 expression system. It is possible that, under such conditions, less specific events contribute to the phenomena observed. This is suggested by the fact that transient insulin receptor expression induced ligand-independent phosphorylation of the receptor and that PTPase co-expression also reduced these levels of basal phosphorylation of the receptor. Nonspecificity is also suggested by the fact that, in the latter study, similar degrees of insulin receptor dephosphorylation were induced by CD45 and RPTPalpha , yet only the RPTPalpha protein abolished the antiadhesive effect of insulin (37).

Data from in vivo studies suggest that precise control of phosphorylation of the insulin receptor regulatory region is important (38). Since there are multiple sites of insulin receptor phosphorylation, it remains possible that critical tyrosines on the insulin receptor are specifically targeted by RPTPalpha , whose dephosphorylation might have gone undetected in the experiment shown in Fig. 4, A and B. However, it is unlikely that RPTPalpha blocks insulin action through selective dephosphorylation of insulin receptor tyrosines, since the kinase activity of the insulin receptor was not significantly changed by the expression of RPTPalpha (Fig. 4C). Likewise, no effect of RPTPalpha was seen when insulin-increased phosphorylation of IRS-1 and Shc was examined. However, these studies cannot eliminate an effect on specific phosphorylation sites of these molecules. Further, it is also possible that Shc and IRS-1 are not in the insulin signaling pathway to prolactin. Recently, a new insulin signaling intermediary, IRS-2, was found in IRS-1 knockout mice (39). Thus, it remains possible that this or another, as yet unknown, intermediary mediates insulin signaling to prolactin gene expression.

The process that RPTPalpha influences probably occurs in association with or close to the cell membrane. The small GTPases such as Ras, Rac, and Rap are membrane-anchored and might be targets for inactivation by RPTPalpha , or RPTPalpha might block activation of an insulin-responsive GTPase. This could then result in inactivation of downstream effectors such as Raf/MEK/MAP kinase, PI 3-kinase, or p70S6 kinase. Therefore, experiments were done to determine if any of these signaling pathways were essential for the response to insulin and were altered in RPTPalpha overexpressing cells.

The experiments using dominant negative Ras and Raf indicate that EGF-increased prolactin-CAT expression is Ras-mediated, while insulin-increased prolactin-CAT expression is dependent on a Ras-like GTPase (Fig. 6). The activity of MAP kinase in hormone-treated GH4 cells expressing these inhibitors paralleled the inhibition of insulin- and EGF-increased prolactin-CAT activity. This suggested that insulin and EGF might increase prolactin-CAT expression in a MAP kinase-dependent manner. However, experiments with PD098059 (Fig. 7) demonstrate that MAP kinase does not mediate the increase in prolactin-CAT expression in insulin-treated cells, and numerous other experiments supported this conclusion.

Ras was also shown to activate PI 3-kinase (40) and, indirectly, p70S6 kinase (41). The experiments with rapamycin (Fig. 8), an inhibitor of p70S6 kinase phosphorylation (42), demonstrate that insulin-increased prolactin-CAT expression is not mediated by p70S6 kinase. However, wortmannin, an irreversible inhibitor of PI 3-kinase, blocked insulin-increased prolactin-CAT expression without affecting basal levels of prolactin-CAT gene transcription or its increase by EGF or cAMP. This could suggest that insulin mediates its effect by activating PI 3-kinase. However, the concentration of wortmannin needed to inhibit insulin-increased prolactin-CAT expression is 100-1000-fold higher than that reported to be necessary for PI 3-kinase inhibition, and lower concentrations of wortmannin do not inhibit insulin-increased prolactin-CAT expression (data not shown). This makes it unlikely that the wortmannin inhibition of insulin-increased prolactin-CAT expression is due to inhibition of PI 3-kinase. The failure of LY294002, a reversible inhibitor of PI 3-kinase (13), to reduce insulin-increased prolactin-CAT expression and other experiments with constitutively activated p110 or with p85 (data not shown) supports this conclusion. Recently, wortmannin was shown to inhibit phosphatidyl 4-kinase (43) at concentrations 100-1000-fold higher than necessary to inhibit PI 3-kinase. Experiments are presently focusing on whether insulin increases inositol -4-PO4 and/or inositol-3-PO4 in RPTPalpha -expressing cell lines.

The identification of PTPases that inactivate insulin signaling will provide important insights into regulation of insulin action and may provide clues for new treatment modalities. PTPases that are potential regulators of insulin responsiveness would be expected to be (a) specific to insulin responses and (b) widely distributed and expressed in insulin-responsive tissues. Experiments in vivo and in vitro have implicated numerous protein tyrosine phosphatases in the control of insulin signaling. These include, in addition to RPTPalpha , the membrane-spanning PTPases, LAR and CD45, and the cytosolic PTPases, PTP1B, and SHP2 (23, 24, 36, 44-46). However, many of these do not have the characteristics expected of a phosphatase that specifically down-regulates the insulin response pathway. LAR is widely expressed and has been shown to dephosphorylate the insulin receptor in vitro (24), and LAR expression blocks insulin signaling (36). However, these effects are not specific for the insulin receptor (24) and the insulin signaling pathway (47). The transmembrane PTPase CD45 (leukocyte common antigen) was shown to block phosphorylation of the platelet-derived growth factor receptor and the insulin growth factor-1 receptor and to block their downstream effects (23), and it is able to dephosphorylate both the insulin and EGF receptors in vitro (44). But this enzyme is not specific and is confined to cells of hematopoietic origin. PTP1B was shown to dephosphorylate the insulin receptor (24) in vitro, and microinjected PTP1B blocks insulin-induced oocyte maturation (48). However, the effect of PTP1B was not specific, since it also blocked maturation induced by progesterone and maturation-promoting factor. SHP2 is ubiquitously expressed and dephosphorylates IRS-1, if not the insulin receptor (45), but SHP2 positively regulates effects of insulin (46). By contrast, the data presented here suggest RPTPalpha may serve as a negative regulator for at least some insulin signaling pathways. It specifically blocks the insulin signaling pathway leading to prolactin gene expression but does not inhibit the effects of EGF or cAMP. Further, it is the only PTPase from among those that were tested that blocks the insulin response pathway. Finally, it is widely expressed including in adipose and muscle cells (49).2

    ACKNOWLEDGEMENTS

We thank L. Feig, V. Narrayanan, T. Payne, U. Rapp, J. Schlessinger, E. Skolnik, K. Siddle, N. Tonks, M. White, and J. Whittaker for plasmids and antibodies used in these studies.

    FOOTNOTES

* This work was supported by National Institutes of Health Grants DK43365 (to F. M. S.) and R29CA68365 (to J. S.) and grants from the Juvenile Diabetes Foundation International (to F. M. S.) and from Sugen Inc. (to J. S.).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

par To whom correspondence should be addressed: Dept. of Medicine, TH 450, NYU Medical Center, 550 First Ave., New York, NY 10016. Tel.: 212-263-7927; Fax: 212-263-7701.

1 The abbreviations used are: CAT, chloramphenicol acetyltransferase; EGF, epidermal growth factor; MAP, mitogen-activated protein; DMEM, Dulbecco's modified Eagle's medium; RPTP, receptor-like protein-tyrosine phosphatase; 8-CPT-cAMP, 8-(chlorophenylthio)-3',5'-cyclic AMP; PI 3-kinase, phosphatidylinositol 3-kinase; IRS, insulin receptor substrate; MEK, MAP kinase kinase; PTPase, protein-tyrosine phosphatase; HA, hemagglutinin; RSV, Rous sarcoma virus; Prl, prolactin.

2 J. Sap, unpublished observations.

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Abstract
Introduction
Procedures
Results
Discussion
References

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