Differential Activation of Protein Kinase B and p70S6K by Glucose and Insulin-like Growth Factor 1 in Pancreatic beta -Cells (INS-1)*

Lorna M. DicksonDagger , Melissa K. LingohrDagger , Jill McCuaigDagger , Sigrun R. HüglDagger §, Lynn SnowDagger , Barbara B. Kahn, Martin G. Myers Jr.||, and Christopher J. RhodesDagger **

From the Dagger  Pacific Northwest Research Institute and Department of Pharmacology, University of Washington, Seattle, Washington 98122, the  Division of Endocrinology and Metabolism, Department of Medicine, Beth Israel Deaconess Medical Center and Harvard Medical School, Boston, Massachusetts 02215, and the || Research Division, Joslin Diabetes Center and Program in Cell and Developmental Biology, Harvard Medical School, Boston, Massachusetts 02215

Received for publication, February 8, 2001


    ABSTRACT
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

It has been shown that IGF-1-induced pancreatic beta -cell proliferation is glucose-dependent; however, the mechanisms responsible for this glucose dependence are not known. Adenoviral mediated expression of constitutively active phosphatidylinositol 3-kinase (PI3K) in the pancreatic beta -cells, INS-1, suggested that PI3K was not necessary for glucose-induced beta -cell proliferation but was required for IGF-1-induced mitogenesis. Examination of the signaling components downstream of PI3K, 3-phosphoinositide-dependent kinase 1, protein kinase B (PKB), glycogen synthase kinase-3, and p70-kDa-S6-kinase (p70S6K), suggested that a major part of glucose-dependent beta -cell proliferation requires activation of mammalian target of rapamycin/p70S6K, independent of phosphoinositide-dependent kinase 1/PKB activation. Adenoviral expression of the kinase-dead form of PKB in INS-1 cells decreased IGF-1-induced beta -cell proliferation. However, a surprisingly similar decrease was also observed in adenoviral wild type and constitutively active PKB-infected cells. Upon analysis of extracellular signal-regulated protein kinase 1 and 2 (ERK1/ERK2), an increase in ERK1/ERK2 phosphorylation activation by glucose and IGF-1 was observed in kinase-dead PKB-infected cells, but this phosphorylation activation was inhibited in the constitutively active PKB-infected cells. Hence, there is a requirement for the activation of both ERK1/ERK2 and mammalian target of rapamycin/p70S6K signal transduction pathways for a full commitment to glucose-induced pancreatic beta -cell mitogenesis. However, for IGF-1-induced activation, these pathways must be carefully balanced, because chronic activation of one (PI3K/PKB) can lead to dampening of the other (ERK1/2), reducing the mitogenic response.


    INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
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DISCUSSION
REFERENCES

The molecular defects causing obesity-linked type 2 diabetes mellitus are not well defined. However, recently it has become clear that key factors involved in causing type 2 diabetes are both impaired beta -cell function (1) and a failure to increase beta -cell mass to compensate for peripheral insulin resistance (2, 3). It is therefore critical that strategies be developed to replenish the loss of beta -cells and/or to expand existing beta -cell mass to compensate for insulin resistance. Such an approach relies on defining the mechanisms involved in regulating beta -cell mitogenic signaling pathways in response to growth factors and nutrients.

Previous studies have shown that certain growth factors, such as growth hormone (GH)1 and insulin-like growth factor 1 (IGF-1), are important for stimulation of beta -cell proliferation (4, 5). In addition, these studies showed that GH and IGF-1 are dependent on glucose at concentrations in the physiologically relevant range of 6-18 mM to increase beta -cell mitogenesis. However, the basis of this glucose dependence of beta -cell proliferation remains unknown.

GH signals via the janus kinase-2/signal transducer and activator of transcription-5 pathway in INS-1 beta -cells. Although glucose has no independent effect on the activation of this pathway, it is nonetheless required for GH mitogenic action (4, 6). There appears to be no cross-talk of janus kinase-2 activation to insulin receptor substrate (IRS)-mediated signaling by GH. However, activation of phosphatidylinositol 3-kinase (PI3K) mediated by glucose is at least partially required for full GH-induced beta -cell proliferation.

IGF-1 has been shown to activate at least two major mitogenic signaling pathways, via PI3K and mitogen-activated protein kinase (7-10). The mitogenic stimulation of receptors, such as the IGF-1 receptor, results in the phosphorylation and activation of the IRS family of proteins and the SH2-containing protein (Shc). Shc then interacts with Shc homology 2 (SH2) domain-containing proteins, such as the growth factor receptor-bound protein-2, whereas IRS proteins interact with the regulatory subunit of PI3K, p85, as well as growth factor receptor-bound protein-2. The recruitment of growth factor receptor-bound protein-2 and its association to murine sons of sevenless-1 protein (a Ras guanine nucleotide exchange factor) activates Ras, resulting in Raf-1 activation, which phosphorylates the extracellular signal-regulated protein kinase (ERK) kinase, which in turn activates ERK1/ERK2 (8). Interaction of tyrosine-phosphorylated IRS with the p85 regulatory subunit of PI3K leads to the activation of the catalytic subunit, p110, which in turn phosphorylates phosphoinositides at the 3' position of the inositol ring, generating PIP3 (4, 6). This increase in phosphorylated phosphoinositides leads to the localization of protein kinase B (PKB) to the membrane through the interaction of PIP3 and PIP2 with the pleckstrin homology domain of PKB (11). Full activation of PKB appears to be dependent on the subsequent phosphorylation of two residues, Thr-308 in the activation loop of the kinase domain and Ser-473 in the carboxyl-terminal tail (12). The protein kinase shown to phosphorylate Thr-308 is 3-phosphoinositide-dependent kinase-1 (PDK1) (13, 14), whereas the kinase responsible for phosphorylation at the Ser-473 residue has not yet been identified. PKB regulates multiple biological processes, such as cell proliferation and apoptosis, suggesting that it may phosphorylate a number of target proteins (reviewed in Ref 15). Glycogen synthase kinase-3 alpha  and beta  (GSK3alpha /beta ) have been shown to be two such targets, and their phosphorylation on Ser-21 and Ser-9, respectively, negatively regulates GSK3alpha /beta activity (16). PKB has also been implicated in catalyzing phosphorylation activation of mammalian target of rapamycin (mTOR), which then mediates the phosphorylation of p70-kDa-S6-kinase (p70S6K) (17, 18). In beta -cells, glucose and IGF-1 activation of p70S6K via the IRS-mediated signal transduction pathway is dependent on PI3K. However, the important signaling components involved in the regulation of mitogenesis that are downstream of PI3K, such as PDK-1, PKB, mTOR, and GSK3alpha /beta , have not been characterized in beta -cells, even though it has been shown that p70S6K is activated by glucose and IGF-1 (4, 5). Therefore, in this study we set out to characterize the signaling elements downstream of PI3K that are regulated by glucose and IGF-1 and found that PKB and p70S6K are differentially activated. These data suggested that a major part of the glucose dependence of beta -cell proliferation is via a direct activation of mTOR/p70S6K, independent of PDK-1/PKB activation.

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INTRODUCTION
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Materials-- The PDK-1 kinase assay kit and PDK-1 antibody were from Upstate Biotechnology Inc. (Lake Placid, NY). The phospho-GSK3alpha /beta (Ser-21/9), total PKB, phosphoThr-308-PKB, phosphoSer-473-PKB antibodies, the GSK3 fusion protein, and the PKB kinase assay kit were from New England Biolabs Inc. (Beverly, MA). Anti-phospho-ERK1/ERK2 was obtained from Promega Corporation (Madison, WI), and the total ERK1/ERK2 antiserum was a gift from Dr. M. Cobb (University of Texas Southwestern Medical Center, Dallas, TX). The p70S6K antisera were generated as described (19). Monoclonal anti-c-Myc clone 9E10 was obtained from Sigma. The total GSK3alpha /beta antibody was from Santa Cruz Biotechnology, Inc. (Santa Cruz, CA). Anti-rabbit and anti-sheep IgG horseradish peroxidase conjugates were from JacksonImmuno Research (West Grove, PA), and the anti-mouse IgG horseradish peroxidase conjugate was from Upstate Biotechnology Inc. Wortmannin and rapamycin were from Calbiochem-Novabiochem. IGF-1 was purchased from Gro Pep Pty Ltd. (Adelaide, Australia). The pUSEamp expression vectors containing Myc-His-tagged mouse PKBalpha (wild type), myr-PKBalpha (constitutively active), and PKBalpha -K179M (kinase-dead) were from Upstate Biotechnology Inc. DNA purification kits and Superfect transfection reagents were purchased from Qiagen (Valencia, CA). Restriction enzymes were from New England Biolabs Inc. The bicinchoninic acid protein assay kit was purchased from Pierce. The [methyl-3H]thymidine and chemiluminescence reagent was from PerkinElmer Life Sciences. All other reagents were of analytical grade from either Sigma or Fisher.

Cell Culture-- The glucose-sensitive pancreatic beta -cell line INS-1 (20) was maintained in the complete medium RPMI 1640 (11.2 mM glucose) containing 10% (v/v) fetal calf serum, 50 µm beta -mercaptoethanol, 10 mM HEPES, 2 mM glutamine, 1 mM sodium pyruvate, 100 units/ml penicillin, 100 µg/ml streptomycin and incubated at 37 °C in 5% CO2 as described (20).

[3H]Thymidine Incorporation-- Thymidine incorporation was measured essentially as described, with minor changes. Briefly, INS-1 cells were cultured on 6-well plates to ~60% confluence and infected with adenovirus as described below. The cells were then counted and ~1 × 104 cells were added to each well of a 96-well plate. The cells were left to attach overnight and were then made quiescent by incubation in starvation medium for 24 h. The INS-1 cells were then incubated for 24 h in starvation medium with additional glucose ± 10 nM IGF-1 as described. During the final 4 h of this incubation 5 µCi/ml [3H]thymidine was added. The specific incorporation of [3H]thymidine into DNA was then measured by transferring the cell lysates to UniFilter-96 GF/C filter plates using the Packard cell harvester, and the radioactivity on the filters was counted with the Packard cell counter.

Stimulation and Lysis Conditions-- Cells were subcultured on either 6-well or 10-cm plates to ~60% confluence. The cells were then subjected to 24-h serum and glucose deprivation with starvation medium (RPMI 1640 medium containing 0.1% bovine serum albumin, 0.5 mM glucose, 100 units/ml penicillin, and 100 µg/ml streptomycin) or infected with adenovirus (see "Adenovirus Infection"), when appropriate, prior to the 24-h incubation with starvation medium. After the quiescent period the cells were pre-treated for 15 min with or without inhibitors as indicated, followed by incubation with fresh starvation medium with or without inhibitors with 0.5, 3, or 15 mM glucose with or without 10 nM IGF-1 for the times indicated. The medium was removed, the cells were washed once with ice-cold phosphate-buffered saline, and the phosphate-buffered saline was replaced with ice-cold cell lysis buffer consisting of 50 mM HEPES (pH 7.5), 1% (v/v) Nonidet P-40, 2 mM activated sodium orthovanadate, 100 mM sodium fluoride, 10 mM sodium pyrophosphate, 4 mM EDTA, 1 mM phenylmethylsulfonyl fluoride, 1 µg/ml leupeptin, and 1 µg/ml aprotonin. After sonication insoluble material was removed by centrifugation, and the samples were stored at -80 °C.

PDK-1 and PKB Kinase Assays-- Cells were stimulated as described (see "Stimulation and Lysis Conditions"). The PKB immunoprecipitation and kinase assay were carried out following the procedures described in the manual, whereas some changes were made to the PDK-1 kinase assay. Active PDK-1 was immunoprecipitated as described in the manual. Briefly, ~1 mg of cell lysate was pre-cleared with 50 µl of protein G-agarose. The beads were removed, the lysate was then added to the protein G-antibody complex, and the samples were left rotating for 2 h at 4 °C. After two washes with cell lysis buffer, followed by two washes with PDK-1 assay dilution buffer, the immunoprecipitates were resuspended in 30 µl of PDK-1 assay dilution buffer containing 10 µl (1 µg) of GSK3 fusion protein and 10 µl of Mg/ATP mixture. The assay was started by the addition of 10 µl (0.5 µg) of serum- and glucocorticoid-regulated protein kinase (SGK)-inactive recombinant protein. SGK is a member of the AGC subfamily of protein kinases whose kinase domain is most related to that of PKB. However, unlike PKB, SGK does not possess a pleckstrin homology domain enabling the assay to be carried out in the absence of PIP3. SGK is phosphorylated at the residue equivalent to Thr-308 of PKB, resulting in activation of this kinase (21). Having established conditions to ensure that the kinase activity was well within the linear portion of the reaction, samples were incubated for 7.5 min at 25 °C with continuous shaking. The reaction was terminated with 30 µl of 3× SDS gel loading buffer, and samples were analyzed by immunoblotting (see "Protein Immunoblot Procedures") with the phospho-GSK3alpha /beta (Ser-21/9) antibody.

Construction of Adenoviruses-- The PI3K adenoviruses, inter Src homology region 2 (AdV-iSH2), and the catalytic p110alpha subunit (AdV-p110) were constructed as described (22). The pUSEamp expression vectors containing Myc-His-tagged mouse PKBalpha (wild type), myr-PKBalpha (constitutively active), and PKBalpha -K179M (kinase-dead) were digested with the restriction enzymes HindIII and Pme1. Each of the cDNAs was inserted between the HindIII and SmaI sites of pBluescript, providing the necessary restriction sites for insertion into pAdTrack-CMV between KpnI and NotI. The PKB adenoviruses were generated and purified as described (23, 24).

Adenovirus Infection-- The appropriate titer for each adenovirus was determined by the addition of various dilutions of each adenovirus to cells subcultured in 6-well plates (9.5 cm2) to 60% confluence (~2 × 106 cells), giving a multiplicity of infection (m.o.i.) ranging from 50 to 2000 based on 0.5-2.0 × 106 plaque forming units/ml as measured by A260. The viral stock was replaced with complete medium after 2 h, and the cells were incubated at 37 °C in 5% CO2 for ~16 h. The cells were then treated as described.

Protein Immunoblot Procedures-- Cell lysates were normalized for total protein after levels were determined using the bicinchoninic acid protein assay kit. For immunoblot analysis 25-50 µg of protein was separated by SDS-polyacrylamide gel electrophoresis. After transfer to nitrocellulose, membranes were immersed in blocking buffer (10 mM Tris/HCl, pH 8.0, 150 mM NaCl, 0.1% Tween, and 5 or 10% (w/v) nonfat dry milk) and incubated with gentle agitation for 1 h. This was followed by incubation overnight at 4 °C with the appropriate primary antibody diluted in primary antibody dilution buffer (10 mM Tris/HCl, pH 8.0, 150 mM NaCl, 0.1% Tween, and 5% bovine serum albumin or 10% (w/v) nonfat dry milk). After a series of washes with blocking buffer without milk, the membranes were incubated for 1 h with gentle agitation with horseradish peroxidase-conjugated secondary antibody diluted in blocking buffer. Washes were repeated as before, and the positive signals were visualized with chemiluminescence reagent and x-ray film.

    RESULTS
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INTRODUCTION
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Constitutive Activation of PI3K in INS-1 Cells Only Increases IGF-1-induced beta -Cell Proliferation-- It has previously been shown that activation of PI3K is required for glucose and IGF-1-induced beta -cell proliferation (4, 5). As such, it was examined whether bypassing the requirement for PI3K activation by an adenoviral mediated constitutively active form of PI3K would unveil the extent of the requirement for this enzyme activity on glucose and IGF-1-induced beta -cell proliferation. Previous studies have shown that adenoviral expression of the iSH2 of the p85alpha subunit with the catalytic p110alpha subunit (p110) results in constitutive activation of PI3K (22). Because of the presence of a Myc tag on each of the subunits, INS-1 cells infected with recombinant adenovirus to express iSH2 (AdV-iSH2), p110 (AdV-p110), or iSH2 + p110 (AdV-p110 + AdV-iSH2) could be confirmed by subjecting the lysates to immunoblot analysis with the anti-Myc antibody (Fig. 1A). Bands at 35 and 115 kDa correspond to the predicted molecular mass of Myc-tagged iSH2 and p110, respectively, whereas the band at 40 kDa is nonspecific (as indicated by its presence in uninfected and AdV-beta -Gal-infected control cells). The beta -cell mitogenesis was determined in INS-1 cells infected with the control beta -Gal (AdV-beta Gal), AdV-iSH2, AdV-p110, or AdV-p110 + AdV-iSH2. The uninfected and AdV-beta Gal controls showed similar increases in [3H]thymidine incorporation in response to 3 or 15 mM glucose ± 10 nM IGF-1 (Fig. 1B), as observed previously (4, 5). For uninfected INS-1 cells at 15 mM glucose, beta -cell mitogenesis was increased 19-fold (p < 0.01), and in the additional presence of 10 nM IGF-1 was 48-fold (p < 0.005) above the 0.5 mM glucose control (Fig. 1B). In AdV-p110-infected INS-1 cells beta -cell mitogenesis in response to glucose and IGF-1 was not significantly different from the uninfected control. In addition, in AdV-iSH2-infected INS-1 cells glucose-induced beta -cell mitogenesis was similar to the uninfected control; however, that at 15 mM glucose + 10 nM IGF-1 was elevated to 68.2 ± 8.4-fold (n = 3) above 0.5 mM glucose (Fig. 1B; p < 0.02). In AdV-p110/AdV-iSH2-coinfected cells glucose-induced beta -cell mitogenesis was not significantly altered compared with that in uninfected or AdV-beta Gal controls in INS-1 cells (Fig. 1B). However, IGF-1-induced beta -cell mitogenesis in AdV-p110/AdV-iSH2 coinfected INS-1 cells was significantly increased 22.2 ± 0.5-fold (n = 3; p < 0.01) at basal 3 mM glucose and 126.5 ± 12.9-fold (n = 3; p < 0.01) at a stimulatory 15 mM glucose above 0.5 mM glucose control (Fig. 1B).


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Fig. 1.   [3H]Thymidine incorporation assays in INS-1 cells overexpressing PI3K. INS-1 cells were cultured on 6-well plates and infected with adenoviruses AdV-beta -Gal, AdV-p110, AdV-iSH2, AdV-p110 + AdV-iSH2 (using an equivalent m.o.i. in each well) or uninfected. A, cell lysates were prepared as described under "Experimental Procedures" and subjected to immunoblot (IB) analysis with the c-Myc antibody. B, [3H]thymidine incorporation assays were carried out as described under "Experimental Procedures" with 3 or 15 mM glucose ± 10 nM IGF-1 and 0.5 mM glucose as control.

Glucose and/or IGF-1 Does Not Affect PDK-1 Kinase Activity in INS-1 Cells-- PDK-1 has been suggested to lie downstream of PI3K in signal transduction pathways (15). It was determined whether PDK-1 plays a role in the mitogenic signal transduction in INS-1 cells in response to glucose ± IGF-1. PDK-1 activity was assessed in INS-1 cells incubated with 0.5, 3.0, or 15 mM glucose ± 10 nm IGF-1 for 2, 10, and 40 min. PDK-1 was found to be active at 0.5 mM glucose, but neither an increase in glucose nor the presence of IGF-1 had any significant effect on further increasing PDK-1 activity (Fig. 2B). Total levels of PDK-1 in each of the samples did not vary, indicating that equivalent amounts of PDK-1 were immunoprecipitated (Fig. 2A). Thus, it would appear that PDK-1 is present in INS-1 cells and is constitutively active.


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Fig. 2.   Analysis of PDK-1 kinase activity in INS-1 cells stimulated with glucose and/or IGF-1. Cell lysates were prepared from INS-1 cells subjected to 24-h serum and glucose deprivation (see "Experimental Procedures") prior to stimulation with 3 or 15 mM glucose ± 10 nM IGF-1 for the times indicated. PDK-1 was immunoprecipitated and assayed for kinase activity as described under "Experimental Procedures." As an indication of PDK-1 kinase activity, the phosphorylation of GSK3alpha /beta was measured by immunoblot (IB) using phospho-GSK3alpha /beta (Ser-21/9) antibody (A). For the controls, cells were stimulated with 15 mM glucose + 10 nM IGF-1, and either SGK was omitted from the assay or sheep IgG was used in place of the anti-PDK-1 kinase sheep polyclonal antibody. The total cell lysates were immunoblotted for PDK-1 (B). The results shown are representative of three independent experiments.

PKB Kinase Is Stimulated by IGF-1 but Not by Glucose in INS-1 Cells-- Activation of PI3K leads to downstream activation of PKB (25). It has been proposed that PKB translocation to the plasma membrane via its pleckstrin homology domain is increased via interaction with the PIP2 and PIP3 products synthesized by increased PI3K activity at the cell plasma membrane (11). PKB membrane localization appears to be sufficient to allow PDK-1-mediated phosphorylation of PKB at Thr-308 and partial activation, although full activation requires additional phosphorylation at Ser-473 by an as yet unidentified kinase (13, 14).

PKB Thr-308 and Ser-473 phosphorylation and consequential regulation of PKB activity was examined in INS-1 cells incubated at 0.5, 3.0, or 15 mM glucose ± 10 nM IGF-1 for 2, 5, 10, 20, and 40 min. PKB activity did not change significantly when cells were incubated at basal 3 mM glucose or stimulatory 15 mM glucose (Fig. 3A). In contrast, IGF-1 rapidly increased PKB activity, which reached a maximum after 5 min of IGF-1 treatment and was maintained over the 40-min period at a similar level whether at a basal 3 mM or stimulatory 15 mM glucose level (Fig. 3A). As such, IGF-1-induced activation of PKB activity did not appear to be glucose-dependent. The PKB phosphorylation state was determined in parallel, and negligible phosphorylation at Thr-308 or Ser-473 was observed in INS-1 cells incubated at 3 or 15 mM glucose, correlating with a lack of glucose-induced PKB activity (Fig. 3B). In contrast, IGF-1 induced a rapid and marked increase in PKB Thr-308 phosphorylation, which was maximal at 2 min and then trailed off but was still significantly above that at time zero by 40 min (Fig. 3B). IGF-1 also markedly increased phosphorylation of PKB at Ser-473 within 2 min, reaching a maximum between 10 and 20 min, which was maintained at 40 min (Fig. 3B). In general, the Thr-308/Ser-473 phosphorylation of PKB by IGF-1 correlated with IGF-1-induced PKB activity (Fig. 3A). Neither 3 or 15 mM glucose affected IGF-1-induced PKB Thr-308 or Ser-473 phosphorylation, also correlating with a lack of influence of glucose on IGF-1-induced PKB activity. The total amount of PKB did not significantly alter with glucose/IGF-1 treatment (Fig. 3B).


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Fig. 3.   The effects of glucose and IGF-1 on PKB activity in INS-1 cells. Cell lysates were prepared from INS-1 cells subjected to 24-h serum and glucose deprivation (see "Experimental Procedures") prior to stimulation with 3 or 15 mM glucose ± 10 nM IGF-1 for the times indicated and 0.5 mM glucose without IGF-1 as control. The level of GSK3alpha /beta phosphorylation was used to measure the PKB activity of each sample (as described under "Experimental Procedures"), and an immunoblot (IB) using phospho-GSK3alpha /beta (Ser-21/9) antibody is shown in A. Cell lysates were subjected to immunoblot analysis as described under "Experimental Procedures" using phospho-Thr-308-PKB, phospho-Ser-473-PKB, and total PKB antibodies (B). The results shown are representative of three independent experiments.

GSK3alpha /beta has been shown to be a phosphorylation substrate of PKB, where phosphorylation of GSK3alpha /beta by PKB inhibits GSK3alpha /beta activity (26). It was determined whether glucose and/or IGF-1 could influence endogenous GSK3alpha /beta phosphorylation in beta -cells (Fig. 4). INS-1 cells were treated at basal 3 mM glucose or stimulatory 15 mM glucose ± 10 nM IGF-1 for 2, 5, 10, 20, and 40 min and then subjected to immunoblot analysis with the phospho-GSK3alpha /beta antibody or total-GSK3alpha /beta antibody (Fig. 4). Neither 3 or 15 mM glucose had any significant effect on GSK3alpha /beta phosphorylation over the 40-min time course (Fig. 4), correlating with a lack of effect of glucose on PKB activity (Fig. 3A). In contrast, IGF-1 rapidly and markedly increased GSK3alpha /beta phosphorylation within 2 min that was sustained throughout the 40-min time course and was independent of the glucose activation (Fig. 4). This GSK3alpha /beta phosphorylation pattern correlated with IGF-1-induced PKB activity and phosphorylation (Fig. 3, A and B). The total amount of GSK3alpha /beta did not alter with glucose/IGF-1 treatment (Fig. 4).


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Fig. 4.   The effects of glucose and IGF-1 on GSK3alpha /beta phosphorylation in INS-1 cells. Cell lysates were prepared from INS-1 cells subjected to 24-h serum and glucose deprivation (see "Experimental Procedures") prior to stimulation with 3 or 15 mM glucose ± 10 nM IGF-1 for the times indicated and 0.5 mM glucose without IGF-1 as control. The level of GSK3alpha /beta phosphorylation was measured by subjecting cell lysates to immunoblot (IB) analysis as described under "Experimental Procedures" using phospho-GSK3alpha /beta (Ser-21/9) antibody (A). The total levels of GSK3alpha /beta were measured by immunoblot with the total GSK3alpha /beta antibody (B). The results shown are representative of three independent experiments.

Time-dependent Phosphorylation of p70S6K by Glucose and IGF-1-- Phosphorylation and activation of p70S6K has also been postulated to be downstream of PKB activation via activation of mTOR by PKB (17, 18). However, mTOR activation can also be mediated by nutrients such as branch chain amino acids (27-30). It was investigated whether p70S6K activation paralleled that of PKB in INS-1 cells. The activation of p70S6K protein is accompanied by phosphorylation at multiple Ser/Thr residues that retards its migration during SDS-polyacrylamide gel electrophoresis (4, 5, 31). The time-dependent activation of p70S6K was investigated in INS-1 cells incubated at 3 or 15 mM glucose ± 10 nM IGF-1 for 2, 5, 10, 20, and 40 min. The cell lysates were then subjected to immunoblot analysis with the p70S6K antibody. The results show that the phosphorylation of p70S6K was apparent after 10 min but only in the presence of 15 mM glucose + 10 nM IGF-1. Phosphorylation of p70S6K was not observed until after 20 min at 3 mM glucose + 10 nM IGF-1 or 15 mM glucose alone (Fig. 5). There was no apparent change in p70S6K phosphorylation at 3 mM glucose over the 40-min time period (Fig. 5). The greatest level of activation was observed after 40 min of stimulation in the presence of both 15 mM glucose and 10 nM IGF-1 (Fig. 5). It should be noted that although glucose activated p70S6K, it had no apparent effect on PKB activity (Fig. 5 versus Fig. 3). Moreover, IGF-1-induced activation of p70S6K was relatively slow compared with that of IGF-1-induced PKB activation and was enhanced by stimulatory glucose concentrations, unlike PKB activity, which was not influenced by glucose (Fig. 5 versus Fig. 3).


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Fig. 5.   The time-dependent phosphorylation of p70s6K in INS-1 cells by glucose and IGF-1. Cell lysates were prepared from INS-1 cells subjected to 24-h serum and glucose deprivation (see "Experimental Procedures") prior to stimulation with 3 or 15 mM glucose ± 10 nM IGF-1 for the times indicated and 0.5 mM glucose without IGF-1 as control. The cell lysates were immunoblotted (IB) with p70s6K antibody as described under "Experimental Procedures" with 10% milk in place of 5% milk and 5% bovine serum albumin for blocking and antibody dilution buffers. The results shown are representative of three independent experiments.

Glucose-stimulated p70S6K Phosphorylation Is Partially PI3K-independent-- It was investigated whether p70S6K phosphorylation activation by glucose and IGF-1 was dependent on upstream PI3K and/or mTOR activation by the use of two specific inhibitors, wortmannin and rapamycin. Wortmannin specifically inhibits PI3K (32), and rapamycin blocks mTOR activation by forming a complex with the immunophilin FKBP12 to generate a potent inhibitor of mTOR (33). INS-1 cells were pre-treated with or without inhibitors and stimulated with 3 or 15 mM glucose ± 10 nM IGF-1 for 40 min with or without inhibitor. To confirm that the wortmannin and rapamycin were specifically inhibiting their target, we analyzed their effects on phosphorylation of PKB (as a positive control) and ERK1/ERK2 (as a negative control) in the same INS-1 cells. In the absence of inhibitor (control) PKB was shown to be phosphorylated on Thr-308 and Ser-473 by IGF-1 but not glucose (Fig. 6A), as previously demonstrated (Fig. 3). The IGF-1-induced phosphorylation of PKB was completely inhibited by wortmannin (100 nM) but unaffected by rapamycin (25 mM), as compared with that of the control (Fig. 6A). PKB levels were equivalent in each sample, as indicated by total PKB immunoblot analysis (Fig. 6A). ERK1/ERK2 phosphorylation activation in INS-1 cells was detected by incubation with stimulatory 15 mM glucose and was increased further with additional IGF-1 (Fig. 6B), as previously observed (4, 5, 34). Phosphorylation of ERK1/ERK2 in response to 15 mM glucose ± 10 nM IGF-1 was not significantly affected by either wortmannin or rapamycin. ERK1/ERK2 levels were equivalent in each sample, as indicated by immunoblot analysis using a total ERK1/ERK2 antibody (Fig. 6B). In control cells, the phosphorylation activation of p70S6K was stimulated in samples treated with 15 mM glucose and by 10 nM IGF-1 at both 3 and 15 mM glucose (Fig. 6C). The greatest degree of phosphorylation was observed in cells treated with 15 mM glucose + 10 nM IGF-1 (Fig. 6C). In the presence of 100 nM wortmannin, the phosphorylation of p70S6K in cells treated with 15 mM glucose or 15 mM glucose + 10 nM IGF-1 was reduced but not completely blocked, whereas phosphorylation appeared to be completely inhibited in cells stimulated with 3 mM glucose + 10 nM IGF-1 (Fig. 6C). It appeared that IGF-1 no longer potentiated 15 mM glucose-induced p70S6K phosphorylation, because p70S6K phosphorylation by 15 mM glucose + 10 nM IGF-1 in the presence of wortmannin was equivalent to that by 15 mM glucose alone (Fig. 6C). In contrast, in the presence of rapamycin, the phosphorylation activation of p70S6K by glucose and IGF-1 was completely inhibited (Fig. 6C).


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Fig. 6.   The effect of PI3K and mTOR inhibition on various components of the signaling pathway in INS-1 cells. INS-1 cells subjected to 24-h serum and glucose deprivation were pre-treated for 15 min with 100 nM wortmannin or 25 nM rapamycin or without inhibitor. This was followed by stimulation with 3 or 15 mM glucose ± 10 nM IGF-1 in the presence of 100 nM wortmannin or 25 nM rapamycin or without inhibitor for 40 min and 0.5 mM glucose without IGF-1 or inhibitor as control. Cell lysates were subjected to immunoblot (IB) analysis as described under "Experimental Procedures" using phospho-Thr-308-PKB, phospho-Ser-473-PKB, and total-PKB antibodies (A); phospho-ERK 1/ERK2 and total ERK 1/ERK2 antibodies (B); and p70s6K antibody (C). The results shown are representative of three independent experiments.

Effect of PKB Overexpression on Mitogenesis in INS-1 Cells-- It was investigated whether increased PKB expression would influence glucose/IGF-1-induced beta -cell mitogenesis. Recombinant adenoviruses were generated to express three Myc/His-tagged constructs of PKB, consisting of a wild type (AdV-PKB-WT), a constitutively active (AdV-PKB-CA), and a kinase-dead form (AdV-PKB-KD), in INS-1 cells. The constitutively active PKB was created by fusing c-Src-derived residues, required for myristoylation, to PKB. This additional sequence directly targets PKB to the plasma membrane, leading to its constitutive activation (35). The kinase-dead form has a point mutation, K179M, removing the ATP-binding site, which results in a loss of kinase activity (36).

PKB overexpression was analyzed by titration of adenovirus infection in INS-1 cells with subsequent PKB immunoblot analysis (Fig. 7). A GFP-expressing adenovirus (AdV-GFP) was used as a control and illustrated the endogenous levels of PKB (Fig. 7). Immunoblot analysis of INS-1 cells infected with AdV-PKB-WT, AdV-PKB-CA, or AdV-PKB-KD indicated a higher molecular weight PKB protein, in addition to the endogenous PKB (Fig. 7). This was due to the additional Myc/His tags on the adenovirally introduced PKB and was confirmed by immunoblotting with a c-Myc antibody (data not shown). The highest levels of expression (that did not adversely affect INS-1 cells) were obtained at a m.o.i. of 10 × 102, and this was the amount of adenovirus used for all subsequent experiments.


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Fig. 7.   Overexpression of AdV-PKB wild type, activated, and kinase-dead forms in INS-1 cells. INS-1 cells were infected with the following adenoviruses: AdV-PKB wild type (AdV-WT), AdV-PKB constitutively active (AdV-CA), AdV-PKB kinase-dead (AdV-KD), and the control adenovirus-green fluorescent protein (AdV-GFP). A multiplicity of infection (MOI) from 0.5 to 20 × 102 was used as described under "Experimental Procedures." After the 16-h incubation in complete medium, cell lysates were subjected to immunoblot (IB) analysis as described under "Experimental Procedures" using the total PKB antibody.

INS-1 cells were infected with AdV-PKB-WT, AdV-PKB-CA, AdV-PKB-KD, or a control adenovirus expressing luciferase (AdV-Luc) and were assayed for glucose/IGF-1-induced [3H]thymidine incorporation in comparison with uninfected INS-1 cells (Fig. 8). The uninfected INS-1 cells showed 3.9 ± 0.1-fold (n = 3) higher levels of incorporation at 3 mM glucose compared with 12.6 ± 2.1-fold (n = 3) higher levels at 3 mM glucose + 10 nM IGF-1 above 0.5 mM glucose (p <=  0.05; Fig. 8). The 15 mM glucose-induced increase in INS-1 cell mitogenesis was 24.4 ± 1.3-fold (n = 3) above the 0.5 mM glucose background and 52.2 ± 6.4-fold (n = 3) higher in the added presence of IGF-1 (p <=  0.05; Fig. 8). These results are consistent with previous findings (4, 5). Control AdV-Luc-infected INS-1 cells were comparable with the uninfected cells in their proliferative response to glucose/IGF-1, indicating no adverse effects of the adenovirus vector per se (Fig. 8). AdV-PKB-WT, AdV-PKB-CA, and AdV-PKB-KD all increased basal 3 mM glucose 2-3-fold above uninfected control, but there was no significant effect with 10 nM IGF-1 at 3 mM glucose. In addition, although the PKB-AdVs did not significantly alter beta -cell mitogenesis at 15 mM glucose compared with the uninfected control, at 15 mM glucose + 10 nM IGF-1, the mitogenic response significantly decreased by 37.0, 53.8, and 41.4% for AdV-PKB-WT, AdV-PKB-CA, and AdV-PKB-KD respectively, compared with the uninfected control (p <=  0.05; Fig. 8).


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Fig. 8.   [3H]Thymidine incorporation assays in INS-1 cells overexpressing PKB wild type, activated, and kinase-dead forms. INS-1 cells were cultured on 6-well plates and infected with adenovirus-luciferase (AdV-Luc), AdV-PKB-WT, AdV-PKB-CA, or AdV-PKB-KD or uninfected, and [3H]thymidine incorporation assays were carried out as described under "Experimental Procedures" with 3 or 15 mM glucose ± 10 nM IGF-1 and 0.5 mM glucose as control.

Effect of PKB Overexpression on Glucose/IGF-1 Activation of PKB, GSK3alpha /beta , ERK1/ERK2, and p70S6K-- Our data indicated that PKB activation was involved in IGF-1-induced beta -cell proliferation but not necessarily that by glucose (Figs. 3-6). As such, one might have predicted that overexpression of AdV-PKB-KD would inhibit IGF-1-induced beta -cell mitogenesis at 15 mM glucose (as observed, Fig. 8), but it was surprising that overexpression of AdV-PKB-WT and especially AdV-PKB-CA also inhibited IGF-1-induced INS-1 cell proliferation at 15 mM glucose (Fig. 8). Hence, we investigated the activation of elements in the IGF-1 signal transduction pathway in PKB-overexpressing cells (Fig. 9). INS-1 cells were infected with AdV-PKB-WT, AdV-PKB-CA, AdV-PKB-KD, or AdV-GFP as a control adenovirus, made quiescent, and then incubated with 3 or 15 mM glucose ± 10 nM IGF-1 for 40 min. Immunoblot analysis with total PKB showed similar levels of adenoviral expressed PKB protein, which was much higher than the endogenous expressed PKB (Fig. 9A). In the AdV-GFP-infected cells, PKB phosphorylation was only detected on Thr-308 and Ser-473 residues when stimulated with 10 nM IGF-1 at 3 mM glucose or stimulatory 15 mM glucose (Fig. 9A), as previously seen (Fig. 3). In AdV-PKB-WT-infected cells, the level of Thr-308 and Ser-473 phosphorylation, although slightly lower for the endogenous PKB compared with the AdV-GFP-infected control cells, was much greater for the adenoviral wild type-expressed PKB (Fig. 9A). In the AdV-PKB-WT-infected cells there was increased basal phosphorylation, which was induced by IGF-1 on both Thr-308 and Ser-473 residues of PKB, independently of glucose, and this was in parallel with the endogenous PKB (Fig. 9A). In AdV-PKB-CA-infected INS-1 cells the level of phosphorylated adenovirally expressed PKB on both Thr-308 and Ser-473 residues was maximal under all conditions tested, as expected for the constitutively active variant of PKB, compared with wild type or kinase-dead PKB variants, and dampened the phosphorylation activation of endogenous PKB by IGF-1 (Fig. 9A). In AdV-PKB-KD-infected INS-1 cells, IGF-1-induced phosphorylation of Thr-308 and Ser-473 residues of endogenous PKB was similar to control AdV-GFP-infected beta -cells. However, the levels of phosphorylation on Ser-473 of the adenovirally expressed kinase-dead PKB were markedly reduced under all conditions tested (Fig. 9A). In contrast, Thr-308 phosphorylation of the adenoviral expressed kinase-dead PKB was increased under basal conditions and stimulated by IGF-1 in a glucose-independent manner (Fig. 9A).


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Fig. 9.   Effect of PKB overexpression of glucose/IGF-1-induced activation of PKB, GSK3alpha /beta , mitogen-activated protein kinase, and p70S6K. INS-1 cells were infected (as described under "Experimental Procedures") at an m.o.i. of 10 × 102 with the following adenoviruses: AdV-PKB-WT, AdV-PKB-CA, AdV-PKB-KD, and the control AdV-GFP. Following the 24-h serum and glucose deprivation described under "Experimental Procedures," the cells were stimulated with 3 or 15 mM glucose ± 10 nM IGF-1 for 40 min and 0.5 mM glucose without IGF-1 as control. Cell lysates were subjected to immunoblot (IB) analysis as described under "Experimental Procedures" using phospho-Thr-308-PKB, phospho-Ser-473-PKB, and total PKB antibodies (A), phospho-GSK3alpha /beta (Ser-21/9) and total GSK3alpha /beta antibodies (B), phospho-ERK 1/2 and total ERK 1/2 antibodies (C), or p70s6K antibody (D). The results shown are representative of three independent experiments.

GSK3alpha /beta is a downstream phosphorylation substrate of PKB, and as such its phosphorylation should parallel that of PKB Thr-308/Ser-473 phosphorylation activation (26). In AdV-GFP-infected control INS-1 cells endogenous GSK3alpha /beta phosphorylation was increased by IGF-1 in a glucose-independent manner (Fig. 9B) that paralleled PKB Thr-308/Ser-473 phosphorylation activation (Fig. 9A). In AdV-PKB-WT-infected cells basal phosphorylation of GSK3alpha /beta was raised and further increased in response to IGF-1 (Fig. 9B), in parallel with PKB phosphorylation (Fig. 9A). In AdV-PKB-CA-infected INS-1 cells GSK3alpha /beta phosphorylation was maximal, irrespective of the glucose/IGF-1 conditions (Fig. 9B), correlating with constitutive activation of PKB in these cells (Fig. 9A). In AdV-PKB-KD-infected INS-1 cells, phosphorylation of GSK3alpha /beta was comparable with that in AdV-GFP-infected cells and as such was likely to be due to endogenous PKB activity. This is consistent with previous results, which showed that the kinase-dead variant of PKB is not a dominant negative protein (15). Total levels of GSK3alpha /beta were equivalent in all samples analyzed (Fig. 9B).

ERK1/ERK2 phosphorylation activation was investigated in PKB-overexpressing INS-1 cells (Fig. 9C). In AdV-GFP-infected INS-1 cells, ERK1/ERK2 phosphorylation was increased by 15 mM glucose, compared with basal 3 mM glucose and further enhanced on addition of 10 nM IGF-1 (Fig. 9C). Surprisingly, 15 mM glucose ± 10 nM IGF-1-induced ERK1/ERK2 phosphorylation was partly inhibited in AdV-PKB-WT-infected INS-1 cells and abolished in AdV-PKB-CA-infected beta -cells. In contrast, ERK1/ERK2 phosphorylation activation by 15 mM glucose ± IGF-1 was not inhibited in AdV-PKB-KD-infected beta -cells but, if anything, was enhanced (Fig. 9C). Total ERK1/ERK2 levels were equivalent in all samples examined (Fig. 9C). The inhibition of glucose ± IGF-1 ERK1/ERK2 phosphorylation in the presence of constitutively active PKB strongly suggests that there is cross-talk between the PI3K/PKB and ERK1/ERK2 signaling pathways.

The phosphorylation state of p70S6K in response to 40 min of incubation with glucose and IGF-1 was examined in adenoviral mediated PKB-overexpressing INS-1 cells (Fig. 9D). Phosphorylation of p70S6K was not detected in the AdV-GFP-infected control cells at basal 3 mM glucose, slightly increased at 3 mM glucose + 10 nM IGF-1 or 15 mM glucose alone, and further enhanced after treatment with 15 mM glucose + 10 nM IGF-1 (Fig. 9D), similar to observations in uninfected INS-1 cells (Fig. 6C). Similar patterns of p70S6K phosphorylation were observed in AdV-PKB-WT- and AdV-PKB-KD-infected INS-1 cells (Fig. 9D). In AdV-PKB-CA-infected INS-1 cells, phosphorylation of p70S6K at basal 3 mM glucose was increased, but at stimulatory 15 mM glucose or in the added presence of IGF-1, p70S6K phosphorylation was not significantly different from that in AdV-GFP-infected control beta -cells (Fig. 9D). These results suggested that constitutive activation of PKB did not overly affect glucose/IGF-1-induced phosphorylation activation of p70S6K.

    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Previous studies have not only shown that PI3K is important for glucose-dependent beta -cell mitogenesis (4, 5) but that glucose induces the activity of PI3K (37). Hence, to gain more insight into the mechanisms involved in glucose-dependent IGF-1 beta -cell mitogenesis, we studied the effects of overexpressing constitutively active PI3K by infecting INS-1 cells with AdV-p110 and AdV-iSH2. However, because AdV-p110- and AdV-iSH2-infected INS-1 cells only showed IGF-1-enhanced beta -cell mitogenesis (Fig. 1B), it suggested that the glucose-dependent signaling events must lie elsewhere. This led us to focus on events downstream of PI3K.

Two such components downstream of PI3K are PDK-1 and PKB (15). The proposed model for PKB activation describes a complex process with a number of steps, one of which involves the protein PDK-1 (15). The first step is translocation of PKB from the cytosol to the plasma membrane, which is induced by increased levels of PIP3, synthesized at the plasma membrane by PI3K. The interaction of PIP3/PIP2 with the pleckstrin homology domain of PKB causes a conformational change allowing phosphorylation at Thr-308 and Ser-473, which appear to be important steps for full activation of PKB. PDK-1 has been shown to phosphorylate PKB at Thr-308; however, the kinase that phosphorylates PKB at Ser-473 has not yet been identified. We first analyzed the activity of PDK-1 in response to glucose and IGF-1. PDK-1 activity did not respond to glucose or IGF-1 in INS-1 cells (Fig. 2B). Hence, it appeared that PDK-1 exists in an active state under basal conditions in pancreatic beta -cells and does not appear to be stimulated in response to glucose or IGF-1. This is consistent with reports in other cells that showed that PDK-1 is constitutively active in vivo (38, 39). In addition, the expression of AdV-PKB-CA, which is constitutively active because of a membrane-targeting motif attached to the amino terminus, in INS-1 cells is sufficient to localize PKB to the membrane, resulting in phosphorylation of the Thr-308 and Ser-473 residues in unstimulated cells (Fig. 9A). These results suggest that there is a significant amount of active PDK-1 present at the membrane of unstimulated cells. Therefore, although PDK-1 is an important component of the PI3K pathway, it does not appear to be a key regulatory component of the glucose or IGF-1 mitogenic response in pancreatic beta -cells.

Similar studies were carried out to determine whether PKB activity was induced by glucose. However, only IGF-1 stimulated the activation of PKB, whereas glucose had no significant effect (Fig. 3). This lack of response to glucose is consistent with the data obtained from INS-1 cells infected with the constitutively active PI3K in which mitogenesis was only enhanced by IGF-1 and not glucose alone (Fig. 1B). Interestingly, the results from the time course of IGF-1-enhanced PKB phosphorylation show that phosphorylation of PKB at Ser-473 increases at a slower rate compared with PKB Thr-308 phosphorylation (Fig. 3B). In addition, the time course of PKB phosphorylated at Thr-308 shows a mobility shift to a slower migrating species that mirrors the increase in PKB phosphorylated at Ser-473 (Fig. 3B). Hence, the slower migrating species could be PKB phosphorylated at both Thr-308 and Ser-473. As such, these results suggested that phosphorylation of PKB at Thr-308 was first, followed by phosphorylation at Ser-473. Intriguingly, the PKB kinase-dead variant, although inactive (as confirmed by lack of GSK3alpha /beta phosphorylation), was still phosphorylated at Thr-308 in a manner regulated by IGF-1. However, lack of phosphorylation at Ser-473 of the kinase-dead PKB suggested that Ser-473 phosphorylation of PKB might well be an autophosphorylation event. If so, the slight amount of IGF-1-induced kinase-dead PKB Ser-473 phosphorylation observed was probably due to endogenous PKB activity (Fig. 9A). These data are consistent with a recent report suggesting that Thr-308 is phosphorylated first, followed by autophosphorylation of the Ser-473 residue of PKB (40).

A known substrate of PKB is GSK3alpha /beta , a protein kinase implicated in several biological and metabolic processes (26). GSK3alpha /beta phosphorylation by PKB leads to down-regulation of its activity. However, only IGF-1 stimulated GSK3alpha /beta phosphorylation, whereas glucose had no effect (Figs. 4 and 9B). This lack of response to glucose and the stimulation of GSK3alpha /beta phosphorylation by IGF-1 correlated with the activation of PKB (Fig. 4). Hence, these results suggest that GSK3alpha /beta is activated by IGF-1 in a glucose-independent manner. However, it is not clear what lies downstream of IGF-1-mediated GSK3alpha /beta inhibition in beta -cells and if it relates to the control of beta -cell mitogenesis. Hence the potential biological role of GSK3alpha /beta in beta -cells awaits future experimental investigation.

Additional proteins that are important in mitogenic signaling are mTOR and p70S6K. These enzymes are activated, in part, by a PI3K-dependent pathway and are critical for cell proliferation (18, 41-43). Although a role for mTOR in mitogenesis has been implicated, little is known about the molecular mechanisms involved in regulating the activation of this large molecular mass protein. The mitogenic activation of p70S6K is also complex due to a requirement for hierarchical phosphorylation at multiple sites (31, 44). However, there is substantial evidence that mTOR mediates the phosphorylation of p70S6K, because rapamycin, which interacts with and inhibits mTOR, blocks the activation of p70S6K in response to mitogenic stimuli (45). A number of reports exist that strongly suggest that p70S6K is downstream of PKB via the activation of mTOR (17, 18). However, the phosphorylation activation of p70S6K in pancreatic beta -cells did not correlate with the activation of PKB. In this regard, the activation of p70S6K was much slower compared with PKB activation (Fig. 5 versus Fig. 3), and whereas glucose stimulated p70S6K activation (Figs. 5 and 9), glucose had no effect on upstream control of PKB activity (Fig. 3). In addition, p70S6K phosphorylation activation by glucose was not inhibited by the PI3K-specific inhibitor, wortmannin, in contrast to an apparent complete inhibition of IGF-1-induced p70S6K and PKB phosphorylation activation by wortmannin (Fig. 6). In addition, overexpression of AdV-PKB-KD did not appear to change the activation of p70S6K in response to IGF-1 and/or glucose compared with the AdV-PKB-WT (Fig. 9D), even though complete phosphorylation activation of AdV-PKB-KD did not occur (Fig. 9A). However, the mTOR-specific inhibitor, rapamycin, completely abolished p70S6K activation phosphorylation by IGF-1 and glucose (Fig. 6D). Hence, taken together, these results strongly support a model in which p70S6K activation by glucose is via mTOR, bypassing a requirement for PKB activation in beta -cells. This is consistent with other reports that have shown p70S6K activation via mTOR, independent of PKB, by other nutrient sources such as branched chain amino acids (27, 28, 30). In addition, studies in yeast suggest that mTOR is involved in regulating cellular responses to nutrient availability (46). In contrast, IGF-1 activated the PI3K/PKB/mTOR signaling pathway. Therefore the mitogenic stimulation by glucose is, at least in part, PKB-independent, and mTOR may mediate the glucose-dependent aspect of the stimulated phosphorylation of p70S6K. Hence, mTOR may be one major component regulating glucose-dependent beta -cell mitogenesis in addition to the glucose activation of ERK1/ERK2 (34). Although it is clear that glucose metabolism is required, the secondary signals that activate kinases to induce the activation of signaling proteins, such as mTOR and ERK1/ERK2, have yet to be identified. One possible candidate is Ca2+, because the inhibition of glucose-induced Ca2+ levels in beta -cells prevents the phosphorylation of ERK1/ERK2, suggesting that ERK1/ERK2 phosphorylation is in part regulated by a Ca2+-dependent protein kinase (34).

It was not too surprising that the kinase-dead form of PKB, which does not appear to act as a dominant negative protein, had little effect on beta -cell mitogenesis, due to compensation by endogenous PKB (Fig. 8). However, it was unexpected that overexpression of the wild type or constitutively active forms of PKB did not increase beta -cell mitogenesis. The phosphorylation activation of p70S6K by glucose and IGF-1 was not enhanced by overexpression of the wild type or constitutively active forms of PKB (Fig. 9D), reaffirming the importance of glucose activation bypassing PKB and acting directly through mTOR activation (as discussed above). Surprisingly, the constitutively active PKB inhibited the IGF-1 and/or glucose phosphorylation activation of ERK1/ERK2 (Fig. 9C). One possible mechanism by which this may occur is through inhibition of Raf1 activity, because studies have shown that this enzyme is negatively regulated by PKB phosphorylation (47, 48). Hence, these PKB inhibitory effects on the ERK1/ERK2 pathway probably contribute to the decrease in beta -cell mitogenesis observed in IGF-1-treated cells expressing the constitutively active or wild type forms of PKB. Interestingly, the ERK1/ERK2 phosphorylation levels in IGF-1- and/or glucose-stimulated INS-1 cells expressing the kinase-dead form of PKB were slightly higher compared with those in control-infected cells (Fig. 9C). Therefore, although PKB activity is diminished in AdV-PKB-KD-expressing INS-1 cells, the ERK1/ERK2 signaling pathway appears to be more active. These observations of adenovirus-mediated PKB overexpression in beta -cells strongly suggest that there is a requirement for both the PI3K and ERK1/ERK2 signaling pathways for glucose-dependent IGF-1-induced beta -cell mitogenesis. Moreover, the data imply that there is a tightly controlled balance between PKB and ERK1/ERK2 signaling pathway elements, both kinetically and of their expression levels; otherwise, negative cross-talk between the pathways would likely dampen signal transduction. It should also be considered that other targets downstream of PKB, such as BAD, caspase-9, and forkhead transcription factors (reviewed in Ref. 49), which affect the mitogenesis and/or survival of beta -cells, may contribute to control of beta -cell mass and warrant further investigation. These elements downstream of PKB may be important factors that play a major role in the pathogenesis of type 2 diabetes if adversely regulated by prolonged hyperglycemia and/or hyperlipidemia, which in turn could contribute to the failure of beta -cell expansion. Alternatively, if PKB downstream elements can be carefully controlled pharmacologically, this may provide a means of preserving or even enhancing beta -cell mass as a potential therapy for both type 1 and 2 diabetes (2).

    ACKNOWLEDGEMENT

We are grateful to Cynthia Jacobs in the preparation of this manuscript.

    FOOTNOTES

* This work was supported by National Institutes of Health Grants DK 55267 (to C. J. R.) and RO1 43051 (to B. B. K.) and by the Juvenile Diabetes Foundation International (to C. J. R.).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.

§ Current address: Medizinische Klinik I, Universität Regensburg, F. J. Strauss-Allee, 93042 Regensburg, Germany.

** To whom correspondence and reprint requests should be addressed: Pacific Northwest Research Inst., 720 Broadway, Seattle, WA 98122. Tel.: 206-860-6777; Fax: 206-726-1202; E-mail: cjr@pnri.org.

Published, JBC Papers in Press, March 27, 2001, DOI 10.1074/jbc.M101257200

    ABBREVIATIONS

The abbreviations used are: GH, growth hormone; IGF-1, insulin-like growth factor 1; IRS, insulin receptor substrate; PI3K, phosphatidylinositol 3-kinase; SH2, Shc homology 2; ERK, extracellular signal-regulated protein kinase; PIP3, phosphatidylinositol 3,4,5-trisphosphate; PKB, protein kinase B; PIP2, phosphatidylinositol 3,4-diphosphate; PDK-1, 3-phosphoinositide-dependent kinase 1; GSK3, glycogen synthase kinase-3; mTOR, mammalian target of rapamycin; p70S6K, p70-kDa-S6-kinase; SGK, serum- and glucorticoid-regulated protein kinase; iSH2, inter SH2 of p85alpha ; m.o.i., multiplicity of infection; AdV, adenovirus; WT, wild type; CA, constitutively active; KD, kinase-dead; GFP, green fluorescent protein; Luc, luciferase.

    REFERENCES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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