Glucose Regulates EF-2 Phosphorylation and Protein Translation by a Protein Phosphatase-2A-dependent Mechanism in INS-1-derived 832/13 Cells*

Limei YanDagger , Angus C. Nairn§, H. Clive Palfrey, and Matthew J. BradyDagger ||

From the Departments of Dagger  Medicine and  Neurobiology, Pharmacology and Physiology, University of Chicago, Chicago, Illinois 60637 and § Department of Psychiatry, Yale University School of Medicine, New Haven, Connecticut 06508

Received for publication, February 3, 2003, and in revised form, March 17, 2003

    ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The role of elongation factor (EF)-2 phosphorylation in the regulation of pancreatic beta -cell protein synthesis by glucose was investigated in the INS-1-derived cell line 832/13. Incubation of cells in media containing 1 mM glucose resulted in a progressive increase in EF-2 phosphorylation that was maximal by 1-2 h. Readdition of 10 mM glucose promoted a rapid dephosphorylation of EF-2 that was complete in 10 min and maintained over the ensuing 2 h. Similar results were obtained using primary rat islets or Min-6 insulinoma cells. The glucose effect in 832/13 cells was replicated by addition of pyruvate or alpha -ketocaproate, but not 2-deoxyglucose, suggesting that mitochondrial metabolism was required. Accordingly, glucose-mediated dephosphorylation of EF-2 was completely blocked by the mitochondrial respiratory antagonists antimycin A and oligomycin. The hyperglycemic effect was not mimicked by incubation of cells in 100 nM insulin, 30 mM potassium chloride, or 0.25 mM diazoxide, indicating that insulin secretion and/or depolarization of beta  cells was not required. The locus of the high glucose effect appeared to be protein phosphatase-2A, the principal phosphatase acting on EF-2. Protein phosphatase-2A activity was stimulated by glucose addition to 832/13 cells, but neither protein phosphatase-1 nor calmodulin kinase III (EF-2 kinase) activity was affected under these conditions. The slower rephosphorylation of EF-2 during the transition from high to low glucose may involve effects on EF-2 kinase activity. Addition of 5-aminoimidazole-4-carboxamide 1-beta -D-ribofuranoside in high glucose led to a marked stimulation of EF-2 phosphorylation, consistent with the possibility that increased AMP kinase activity in low glucose stimulates EF-2 kinase. In parallel with the effects on EF-2 dephosphorylation, addition of high glucose to 832/13 cells markedly increased the incorporation of [35S]methionine into total protein. Taken together, these results suggest that modulation of extracellular glucose impacts protein translation rate in beta  cells at least in part through regulation of the elongation step, via phosphorylation/dephosphorylation of EF-2.

    INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Glucose exerts many effects on pancreatic islets in addition to the familiar enhancement of insulin secretion. Several studies have shown that hyperglycemia results in both transcriptional and translational activation in beta  cells or their derivative cell lines (e.g. Refs. 1-5). For example, proinsulin production is controlled by glucose at both levels, and acetyl-CoA carboxylase gene transcription is activated. Measures of total protein synthesis using [35S]methionine labeling and two-dimensional SDS-PAGE reveal substantial increases in many proteins after glucose stimulation of isolated islets, particularly the components of secretory granules (6, 7). Mechanistic studies of the glucose effect on protein synthesis have been ambiguous. Early studies in isolated islets suggested that the initiation step was primarily affected (1), but subsequent studies proposed that both initiation and elongation were involved (2). However, attempts to identify the specific initiation and/or elongation factors that might contribute to changes in translational control have been inconclusive. The situation is complicated by the fact that glucose causes insulin secretion, and insulin itself can exert profound effects on protein synthesis in responsive cells, including beta  cells themselves. Thus, some of the effects of glucose on translation in beta  cells may well be mediated in an autocrine manner (8).

Regulation at the level of initiation is often dependent on the phosphorylation of the limiting accessory factors eIF-2B and eIF4E-BP (4E-BP, Phas-1) (for review, see Ref. 9). Whereas insulin is known to alter the activity of 4E-BP via the phosphatidylinositol 3-kinase-Akt-mTOR1 pathway in many target cells, glucose appears not to directly affect this system in beta  cells (10) but can induce 4E-BP phosphorylation via the autocrine pathway, provided that amino acids are present (8). Glucose does appear to increase the activity of eIF-2B, but not by altering the phosphorylation state of the eIF-2alpha factor commonly found to be involved in translational initiation control (10). Protein translation can also be regulated at the level of elongation, principally by secondary modification of both elongation factors 1 and 2. EF-1 is a substrate for several protein kinases, and its activity can be modulated by insulin in target cells (11). Phosphorylation of EF-2 by the enzyme Ca2+/CaM-dependent protein kinase III (EF-2 kinase), primarily at Thr-56, blocks the ability of this factor to participate in protein synthesis (12, 13). EF-2 phosphorylation state has subsequently been shown to vary in a wide variety of cell types in response to diverse stimuli (for review, see Ref. 14). Frequently, these stimuli elevate intracellular Ca2+, thereby activating the kinase and increasing phospho-EF-2 (EF-2P) levels. However, other mechanisms of altering EF-2P levels may be even more important, including phosphorylation and activation or inactivation of EF-2 kinase by calcium-independent kinases, as well as effects on the dephosphorylating arm of the cycle.

In this study we examined the effects of glucose on the EF-2 phosphorylation system in beta  cells or cell lines derived from beta  cells. For the most part, we used the INS-1-derived 832/13 cell line that shows robust insulin secretory responses to glucose and appears to mimic beta -cell behavior in several ways (15). We found that glucose addition to cells maintained in low glucose medium induced a marked and rapid dephosphorylation of EF-2 that was accompanied by a significant increase in overall protein synthesis. The effect on EF-2 phosphorylation seemed to be principally mediated by stimulation of protein phosphatase-2A (PP2A) activity rather than by inhibition of the kinase reaction. Together, our data suggest that promotion of protein synthesis by glucose involves modification of the elongation step of protein translation.

    EXPERIMENTAL PROCEDURES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Materials-- Cell culture reagents were supplied by Mediatech, Inc., except for cysteine/methionine-free media, which was from Invitrogen. All chemicals were purchased from Sigma, with the exception of AICAR (Toronto Research Chemicals) and rapamycin, PD98059, and wortmannin (Calbiochem). Tran35S-label (1000 Ci/mmol) and [gamma -32P]ATP (4500 Ci/mmol) were obtained from ICN. Anti-EF-2 and anti-phospho-EF-2 antibodies were generated as described previously (16); the phospho-acetyl-CoA carboxylase antibody was from Upstate Cell Signaling Solutions. Horseradish peroxidase-conjugated goat anti-rabbit and goat anti-mouse IgG was from Bio-Rad, whereas ECL reagent was obtained from Amersham Biosciences.

Cell Culture and Experimental Treatment-- The INS-1-derived cell lines 832/1 and 832/13 were generously provided by Dr. C. Newgard (Duke University) and cultured as described previously (15). Multiwell cultures (75-90% confluent) were rinsed twice with phosphate-buffered saline and incubated for 2 h in Krebs-Ringer buffer supplemented with 25 mM Hepes (pH 7.4) and 0.5% bovine serum albumin (KRBH) and either 1 or 10 mM glucose. Sample wells were then switched to KRBH containing the same or different glucose concentrations for various periods as indicated in the figures. Cells were then rapidly washed three times on ice with phosphate-buffered saline, scraped into lysis buffer (50 mM Hepes (pH 7.4), 150 mM NaCl, 10 mM NaF, 10 mM EDTA, 10% glycerol, 0.5% Triton X-100, and protease inhibitors), and centrifuged at 14, 000 × g for 10 min at 4 °C. Supernatants were removed, and equal amounts of lysate protein were analyzed by SDS-PAGE and immunoblotting. Rat islets were prepared as described previously (17), and treated samples were kindly provided by Drs. J. Corbett and P. Hansen (St. Louis University).

Enzyme Assays-- Ca2+/CaM-dependent EF-2 kinase activity was measured as described previously (18), using purified rat liver EF-2 as substrate. Reactions contained 5 µg of lysate protein, 3 µg of EF-2, and 25 µM [gamma -32P]ATP. Reactions were terminated by the addition of SDS sample buffer and boiling; 32P-EF-2 was resolved by SDS-PAGE, identified by autoradiography, and counted by liquid scintillation. Protein phosphatase assays were performed as described previously (19). After treatment, cells were collected in phosphatase homogenization buffer (50 mM Hepes (pH 7.4), 2 mM EDTA, 2 mg/ml glycogen, 0.2% beta -mercaptoethanol, 0.5% Triton X-100, and protease inhibitors). Samples were then centrifuged at 14,000 × g for 10 min at 4 °C, and ~5 µg of supernatant protein was used for assays. [32P]Phosphorylase was used as substrate and prepared as described previously (19), with the modification that recombinant phosphorylase kinase catalytic subunit was used. Phosphatase activity inhibited by addition of 3 nM okadaic acid is defined as PP2A, whereas phosphatase activity lost between 3 and 500 nM okadaic acid is defined as protein phosphatase-1. Addition of 500 nM okadaic acid completely inhibited all cellular phosphatase activity measured under these conditions.

[35S]Methionine/Cysteine Incorporation into Total Protein-- 832/13 cells were plated in 12-well dishes and serum-starved as described above. Cells were pretreated in triplicate for 10 min as indicated, and then 10 µCi of Tran35S-label was added to all wells. After a 10-min incubation at room temperature, the dishes were washed thrice with ice-cold 10% trichloroacetic acid; precipitated proteins were then dissolved in 0.5 ml of 0.1 N NaOH and transferred to scintillation vials. The samples were neutralized by addition 10 µl of 10% acetic acid, and 35S incorporation into proteins was measured by scintillation counting. In parallel, a replicate well for each condition was washed three times with phosphate-buffered saline, and protein lysates were analyzed by SDS-PAGE and autoradiography.

    RESULTS
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Glucose Increases Protein Translation in 832/13 Cells-- Shifts in extracellular glucose markedly affect insulin secretion and protein biosynthesis in beta -cell lines and primary islets (1-5). To confirm that glucose levels also regulate protein synthesis in the INS-1-derived 832/13 cells, we preincubated cells for 2 h in 1 mM glucose and then added back either glucose (3 or 10 mM), pyruvate (5 mM), or insulin (100 nM) for 10 min and measured incorporation of [35S]methionine into total cellular protein. Addition of glucose caused a ~4-fold increase in total incorporation (Fig. 1A), and analysis of labeled proteins by SDS-PAGE showed that this effect involved numerous species (Fig. 1B). The effect was reproduced by pyruvate, but insulin in the presence of 1 mM glucose had little effect on labeling. These results are comparable with those found previously with isolated islets (7) and demonstrate that the 832/13 cell line exhibits typical glucose responsiveness with respect to protein translation.


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Fig. 1.   Stimulation of protein synthesis in INS-1-derived 832/13 cells by glucose. 832/13 cells were maintained in KRBH/10 mM glucose (con) or glucose-restricted in KRBH/1 mM glucose for 2 h. Replicate wells kept in low glucose were stimulated with glucose (3 or 10 mM), 5 mM pyruvate, or 100 nM insulin (in 1 mM glucose) for 10 min, and then all samples were pulse-labeled in [35S]methionine-containing medium for an additional 10 min. Samples were collected for measurement of total protein synthesis by trichloroacetic acid precipitation (A) or for analysis of synthesized proteins by SDS-7.5% PAGE and autoradiography (B). Results in A are a summary of three experiments, each point performed in duplicate (data are means ± S.D.). B, lane 1, 1 mM glucose; lane 2, 3 mM glucose; lane 3, 10 mM glucose; lane 4, 5 mM pyruvate; lane 5, 100 nM insulin. Autoradiograph in B is representative of three independent experiments.

Extracellular Glucose Levels Regulate EF-2 Phosphorylation in beta -Cell Lines and Primary Islets-- Because EF-2 phosphorylation state has been correlated with protein synthetic capacity in several studies (for review, see Ref. 14), we investigated whether ambient glucose affected EF-2P levels in the 832/13 cell line, as well as in Min-6 insulinoma cells and isolated pancreatic islets. Cells were preincubated for 2 h in buffer containing either 1 or 10 mM glucose, and lysates were prepared and analyzed by immunoblot using a phospho-specific EF-2 antibody (raised against a peptide containing phospho-Thr-56; Ref. 16). Cultures maintained in low glucose exhibited relatively high levels of EF-2P, whereas those maintained in high glucose had low levels of EF-2P (Fig. 2A). When samples were shifted from low to high glucose, EF-2P declined within 10 min to the level found in cells maintained in high glucose throughout (Fig. 2, A and B). In contrast, there was no change in total EF-2 protein with any treatment (Fig. 2, A and B). Importantly, the glucose-dependent phosphorylation/dephosphorylation of EF-2 was also manifest in Min-6 cells and primary rat islets (Fig. 2A), indicating that this effect may be physiologically relevant in beta  cells from a variety of sources. However, in high glucose, EF-2P levels were elevated in the islets as compared with the cell lines, perhaps reflecting the presence of non-regulated EF-2P in alpha  and delta  cells in the islet preparations. To investigate the reversibility of the phenomenon, we verified that after a 2-h incubation in high glucose, samples returned to low glucose exhibited a rephosphorylation of EF-2, albeit with slower kinetics as described below.


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Fig. 2.   Glucose levels regulate the state of EF-2 phosphorylation in INS-1-derived 832/13 and pancreatic beta  cells. A, 832/13 cells (left panel), Min-6 cells (center panel), or freshly isolated rat pancreatic islets (right panel) were preincubated in KRBH containing 10 mM glucose (hi) or 1 mM glucose (lo) for 2 h. Some of the cells in KRBH/1 mM glucose were then switched back to KRBH/10 mM glucose for 10 min (lo right-arrow hi). Extracts were made, and equal amounts of lysate protein were separated by SDS-7.5%PAGE, transferred to nitrocellulose, and incubated in rabbit polyclonal anti-EF-2P IgG (0.5 µg/ml), followed by secondary antibody and development using ECL. After exposure, blots were stripped and reprobed with anti-EF-2 IgG as a loading control (bottom panels; signals varied <10% by densitometric analysis). B, 832/13 cells were preincubated for 2 h in KRBH containing 10 mM (hi) or 1 mM glucose; 10 mM glucose was added to individual wells for the indicated times (lo right-arrow hi). Fluorograms are representative of three to five independent experiments. Note that EF-2P levels were somewhat elevated in islets cultured in high glucose, probably due to the presence of alpha  and delta  cells in addition to beta  cells.

Mitochondrial Metabolism of Glucose Is Required for Reduction in EF-2P Levels-- To determine whether the hyperglycemic effect on EF-2 phosphorylation was mediated by breakdown and mitochondrial utilization of the sugar, we tested the effects of non-metabolizable glucose analogs, as well as permeant compounds that can bypass glucose catabolism. Addition of 2-deoxyglucose to cells maintained in low glucose had no effect on EF-2P level, indicating that metabolism beyond the glucokinase step is required (Fig. 3A). By contrast, addition of 5 mM of either pyruvate or alpha -ketocaproic acid, both of which can enter mitochondria and be directly metabolized to produce ATP, could substitute for glucose in mediating EF-2 dephosphorylation (Fig. 3B). Further evidence for mitochondrial involvement came from the use of respiratory chain inhibitors such as antimycin A or oligomycin, either of which blocked the effect of glucose on EF-2 dephosphorylation (Fig. 3C). These data indicate that production of ATP or some catabolite derived from glucose may be an important intermediary in promoting EF-2 dephosphorylation.


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Fig. 3.   Glucose metabolism is required for EF-2 dephosphorylation in 832/13 cells. A, 832/13 cells were glucose-restricted for 2 h (lo), and then 10 mM glucose (hi) or 2-deoxyglucose (lo + 2-DOG; 10 mM) was added for 10 min. B, replicate wells were pretreated as described in A, and then 10 mM glucose (hi), 5 mM pyruvate, or 5 mM alpha -ketocaproate was added for 10 min. C, cells were glucose-deprived for 2 h (lo) and stimulated with 10 mM glucose for 10 min (lo right-arrow hi). The indicated samples were preincubated with the mitochondrial inhibitors antimycin A or oligomycin (both 1 µM) for 10 min before changing glucose levels. All autoradiographs are representative of three to four experiments.

Glucose-stimulated EF-2 Dephosphorylation Is Not Mediated by Insulin Secretion or by Insulin-activated Signaling Pathways-- INS-1 cells and islet beta  cells themselves have insulin receptors, and it is likely that some effects of glucose are mediated by released insulin, acting in an autocrine or paracrine manner (20). Moreover, insulin treatment of some other cell types has been reported to reduce EF-2P levels via inactivation of EF-2 kinase (e.g. see Ref. 21). To investigate the potential role of insulin release/signaling on EF-2P levels, 832/13 cells were preincubated for 2 h in buffer containing 1 mM glucose. Insulin-dependent effects on EF-2P were estimated by direct addition of 100 nM insulin or by depolarizing the cells with either 30 mM KCl or the ATP-sensitive potassium channel blocker tolbutamide. Exogenous insulin did lead to a small decrease in EF-2P levels at 10 min (Fig. 4A) but was unable to mimic the glucose effect, even after 2 h (data not shown). Additionally, stimulation of endogenous insulin release from 832/13 cells by addition of 100 µM tolbutamide or 30 mM KCl had no effect on EF-2P levels (Fig. 4B; data not shown). EF-2 dephosphorylation resulting from glucose addition was also unaffected by inclusion of 0.25 mM diazoxide, an inhibitor of insulin exocytosis (data not shown). Finally, the glucose effect was evinced in 832/1 cells (Fig. 4B), INS-1-derived cells that exhibit meager glucose-stimulated insulin secretion (15).


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Fig. 4.   The glucose effect on EF-2P does not involve insulin-dependent signal transduction pathways. A, 832/13 cells were maintained in KRBH/1 mM glucose (lo) for 2 h to elevate EF-2P. Half the samples were preincubated for 15 min with 100 nM wortmannin; 10 mM glucose (hi) or 100 nM insulin (lo + Ins) was then added for 10 min. EF-2P levels were analyzed by immunoblotting; loading controls using total EF-2 immunoblotting showed <10% variation between lanes (data not shown). B, left panel, cells were glucose-deprived for 2 h (lo) and then pretreated for 15 min without or with 10 µM tolbutamide (T). 10 mM glucose (hi) was then added to half the wells for 10 min before preparation of cell lysates. Right panel, a variant INS-1-derived cell line (832/1), selected for poor insulin secretory responses to glucose, was treated as described in the Fig. 2 legend. Note that an increase in glucose also lowers EF-2P in these cells. C, inhibitors of the Ras-mitogen-activated protein kinase and phosphatidylinositol 3-kinase-mTOR pathways do not block glucose-induced dephosphorylation of EF-2P. After 2 h of glucose restriction, 832/13 cells were maintained in either 1 mM glucose (lo; lanes 1-5) or 10 mM glucose (hi; lanes 1'-5') for 10 min. Lanes 1, control; lanes 2, PD98059 (20 µM); lanes 3, rapamycin (100 nM); lanes 4, wortmannin (200 nM); lanes 5, PD98059 + wortmannin. All drugs were preincubated with cells for 15 min before shift to high glucose. EF-2P levels were analyzed by immunoblotting. Bottom panel, reprobe of blot with EF-2 IgG as loading control. All results are representative of three independent experiments.

To investigate potential signaling pathways mediating the regulation of EF-2P levels by glucose, a variety of well-characterized kinase inhibitors were used. 832/13 cells were glucose-restricted for 2 h in KRBH containing 1 mM glucose and preincubated for 15 min with the indicated compounds, and then 10 mM glucose was added for a final 10-min period. Pretreatment of 832/13 cells with 100 nM of the phosphatidylinositol 3-kinase inhibitor wortmannin had no effect on the glucose-dependent dephosphorylation of EF-2, whereas the modest insulin effect on EF-2P levels was completely blocked by the drug (Fig. 4A). Neither the mitogen-activated protein kinase/extracellular signal-regulated kinase kinase inhibitor PD98059 (20 µM) nor the mTOR inhibitor rapamycin (100 nM), alone, in combination, or together with wortmannin, had any effect on the glucose-mediated reduction in EF-2P levels (Fig. 4C; data not shown). The efficacy of these compounds on their respective signaling pathways was confirmed in parallel experiments using insulin-stimulated 3T3-L1 adipocytes (data not shown). Cumulatively, these results indicate that the regulation of EF-2P levels by extracellular glucose occurs independently of insulin secretion/signaling and activation of several well-characterized kinase signaling cascades.

Stimulation of Protein Phosphatase-2A Plays a Major Role in the High Glucose Effect on EF-2 Dephosphorylation-- The regulation of EF-2P levels by extracellular glucose must involve alteration of kinase and/or phosphatase activities. EF-2 kinase is the major and perhaps only kinase that phosphorylates EF-2, whereas PP2A is the most active cellular phosphatase acting on EF-2P (12, 14, 18, 22). Direct assays of kinase activity in lysates derived from cells shifted from low to high glucose revealed no significant difference in either basal or Ca2+/CaM-stimulated activity (using activity in 1 mM glucose as 100%, cells maintained in 10 mM glucose had 113% of this activity, whereas cells shifted for 10 min from 1 to 10 mM glucose had 97% of this activity), suggesting that this enzyme is not the primary target of the hyperglycemic effect. In parallel, both protein phosphatase-1 and PP2A activities were measured in cellular lysates using [32P]phosphorylase as substrate. Extracts from cells incubated with 10 mM glucose contained a high level of PP2A activity (Fig. 5A). Reducing extracellular glucose to 1 mM for 2 h reduced PP2A activity by ~2-fold. Conversely, raising extracellular glucose from 1 to 10 mM caused a substantial activation of PP2A activity within 10 min; by contrast, protein phosphatase-1 activity measured in the same lysate remained constant during these transitions (Fig. 5A). If stimulation of PP2A is involved in the effect of high glucose, then the response should be sensitive to permeant inhibitors of this enzyme. Accordingly, preincubation of 832/13 cells with calyculin A (50 nM), an inhibitor of both protein phosphatase-1 and PP2A but not of protein phosphatase-2B or protein phosphatase-2C, markedly impaired EF-2 dephosphorylation in response to glucose addition (Fig. 5, B and C). Taken together, these data suggest that the hyperglycemic reduction in EF-2 phosphorylation state appears to be mediated primarily by an increase in PP2A rather than a decrease in EF-2 kinase activity.


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Fig. 5.   Glucose-induced dephosphorylation of EF-2 is mediated by PP2A. A, lysates were prepared from 832/13 cells that were treated as described in the Fig. 2 legend. Cells were collected in phosphatase homogenization buffer, and protein phosphatase-1 and PP2A activities against [32P]phosphorylase were determined as detailed under "Experimental Procedures." Results represent mean ± S.D. of three independent experiments, each performed in duplicate. *, p < 0.01; NS, p > 0.3 by Student's t test. B, phosphatase inhibition reduces the glucose effect on EF-2P. Replicate wells of 832/13 cells were maintained in KRBH with 1 mM (lo) or 10 mM (hi) glucose for 2 h. Some samples were then preincubated for 10 min with 50 nM calyculin A before the addition of 10 mM glucose (lo right-arrow hi) for the indicated times. Lysates were analyzed by sequential anti-EF-2P and anti-EF-2 immunoblotting and quantitated by densitometry (C). Results are representative of three independent experiments. Note in B that calyculin A treatment of cells in high glucose does not increase EF-2P significantly within 10 min; other experiments show that this is also true at 1 h (data not shown).

Phosphorylation of EF-2 in Low Glucose May Involve AMP Kinase-- When cells were shifted from high to low glucose media, there was a relatively slow reappearance of EF-2P (Fig. 6A). The marked kinetic difference between dephosphorylation in high glucose and rephosphorylation in low glucose suggested that the two processes might be mediated by distinct mechanisms. Indeed, whereas calyculin A attenuated the dephosphorylation of EF-2 on glucose addition, the phosphatase inhibitor did not substantially raise the already low EF-2P levels of 832/13 cells maintained in high glucose (e.g. see Fig. 5B; data not shown). Thus, a simple reversal of PP2A stimulation cannot account for the effect of glucose restriction. This result implies that stimulation of EF-2 kinase, rather than a decrease in PP2A activity with no change in EF-2 kinase, is somehow involved in the phosphorylation phenomenon. It seemed highly unlikely that such a stimulation could occur via changes in intracellular Ca2+ because low glucose hyperpolarizes beta  cells, resulting in the closure of plasma membrane Ca2+ channels and a consequent lowering of cytoplasmic [Ca]. Additionally, a 15-min treatment with 10 µM forskolin caused only a slight increase in EF-2 phosphorylation, suggesting that changes in cAMP levels were not involved in the phosphorylation response to low glucose (Fig. 6B).


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Fig. 6.   Phosphorylation of EF-2 in low glucose: possible role of AMP kinase. A, 832/13 cells were transferred from 10 mM to 1 mM glucose-containing KRBH for the indicated times, and EF-2 phosphorylation was determined by immunoblotting (inset). The graph shows densitometric quantitation of EF-2P immunoblots, indicating a half-time to maximum phosphorylation of ~20 min. B, 832/13 cells were incubated in KRBH plus 10 mM (hi) without AICAR (con) or in the presence of 1 mM AICAR (+AICAR) for the indicated times. A replicate well was incubated in KRBH with 1 mM glucose (lo) for 2 h. Lysates were analyzed by anti-EF-2P immunoblotting. A 15-min exposure to 10 µM forskolin (forsk) caused only a slight increase in EF-2P. C, acetyl-CoA carboxylase phosphorylation. As control, cells were incubated in KRBH and 1 mM (lo) or 10 mM (hi) glucose for 2 h. Additionally, cells were incubated in 1 mM glucose (hi right-arrow lo), or 1 mM AICAR was added to the high glucose media (+AICAR), for the indicated times. Lysates were analyzed by anti-phospho-acetyl-CoA carboxylase (ACC-P) immunoblotting. All results are representative of three to four independent experiments.

Shifts in extracellular glucose have been reported to alter the ATP/AMP ratio in beta  cells, and it has been proposed that AMP kinase might act as a sensor to transmit signals from metabolism to various effector pathways (23). Accordingly, we tested whether AICAR, a nucleotide analog activator of AMP kinase (24), would affect EF-2 phosphorylation in 832/13 cells. AICAR treatment of cells maintained in high glucose led to an increase in EF-2P that peaked at 30 min (Fig. 6B). The effects of the nucleotide were not additive with glucose restriction (data not shown), suggesting that AMP kinase may play a role in the calcium-independent activation of EF-2 kinase in glucose-restricted cells. This conclusion was bolstered by the observations that glucose restriction increased the phosphorylation of the AMP kinase substrate acetyl-CoA carboxylase (25), with a time course similar to that of EF-2 (Fig. 6, compare C with A), and that AICAR stimulation of EF-2 and acetyl-CoA carboxylase phosphorylation was also temporally correlated (Fig. 6, compare C with B).

    DISCUSSION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The acceleration of protein synthesis by glucose in pancreatic beta  cells was established many years ago, yet the mechanisms underlying the increase in translational capacity are still obscure. Initiation is the rate-limiting step in translation under many circumstances, thus it had been anticipated that glucose stimulation would primarily impact this step. One report does claim an effect of glucose stimulation on eIF-2B activity, but the mechanism is unknown (10). We show here that, as in islets themselves, the 832/13 beta -cell line exhibits a robust increase in overall protein synthetic rates in response to glucose. Our data strongly suggest that glucose-induced EF-2 dephosphorylation plays a major role in this response. A potential route by which this might take place is by an autocrine/paracrine mechanism whereby secreted insulin activates beta -cell insulin receptors. Insulin is known to affect beta -cell function, as strikingly shown in the differential effects of glucose or insulin on insulin gene transcription in control versus beta -cell-specific, insulin receptor-deficient (beta IRKO) mice (20). However, the mechanism of glucose action on EF-2 dephosphorylation in the present study is definitively not via secreted insulin and is not mediated by either the phosphatidylinositol 3-kinase-mTOR pathway or Ras-mitogen-activated protein kinase, both of which are downstream of the activated insulin receptor. Neither insulin itself nor stimuli that evoke a glucose-independent secretion of insulin had a profound effect on EF-2 phosphorylation state. Conversely, glucose-stimulated dephosphorylation of EF-2 was unaffected by inhibition of cellular depolarization and insulin secretion. Nevertheless, as with the insulin secretory response, catabolism of glucose was required, and it appears likely that a mitochondrial metabolite might be pivotal to the signaling pathway required for the effect on EF-2 phosphorylation state.

The failure to find an obvious effect of glucose addition on EF-2 kinase activity raised the possibility that the high glucose control of EF-2P resided primarily on the phosphatase arm of the cycle. Hyperglycemic conditions evoked an activation of protein phosphatase activity in 831/13 cells, confirming a previous preliminary report in islets (26). Differential measurement of protein phosphatase activities revealed that PP2A was the likely locus of the effect in 832/13 cells. With respect to EF-2 dephosphorylation, this makes sense because PP2A is the most potent phosphatase acting on EF-2P (12, 22). Dephosphorylation of EF-2P upon glucose addition was attenuated by calyculin A, supporting the notion that control is exercised at the phosphatase level in the glucose signaling pathway. PP2A is a key member of the serine/threonine-protein phosphatase family and is responsible for a substantial fraction of the dephosphorylating activity present in all mammalian cells. In this group of enzymes, a conserved catalytic subunit (C) is linked to variable anchoring (A) and regulatory subunits (B) to form a variety of heterotrimeric enzymes, although AC dimers may also exist in cells (27). A novel regulatory mechanism involving the TAP42/alpha 4 protein may also play an important role in PP2A specificity. TAP42 is a yeast protein implicated in the TOR pathway, and its mammalian equivalent (alpha 4) has been found in association with the PP2A catalytic subunit in vivo. Indeed, overexpression of alpha 4 has been reported to affect EF-2P levels in COS-7 cells without influencing other phosphoproteins relevant to protein synthesis (28). It is possible that the effects of glucose in beta  cells will be mediated by some factor that modulates the association of PP2Ac with a specific regulatory subunit. Molecular identification of PP2A subspecies in beta  cells is clearly warranted and will be required before the details of the glucose signaling pathway can be elucidated. Our data are not consistent with a recent report claiming that glucose might exert some of its effects in beta  cells through the inhibition of protein phosphatase activity (29). In that study, several metabolites of glucose such as phosphoenolpyruvate were found to inhibit total protein serine/threonine phosphatase activity in beta -cell extracts. However, very high concentrations of these intermediates were used, and no attempt was made either to discriminate between different phosphatases or to show that enzyme activity was modulated in intact cells. Glucose has also been reported to increase protein phosphatase-2B (calcineurin) activity in islets through a calcium-dependent mechanism, and this may be involved in transcriptional and secretory control in beta  cells (30). Protein phosphatase-2B is unlikely to be involved in EF-2P dephosphorylation because depolarization had no effect on EF-2P state, and protein phosphatase-2B has minimal activity against EF-2P in vitro.

EF-2 kinase is a member of an atypical family of protein kinases that differ in the primary structure of the catalytic domain from the "conventional" protein kinases, such as protein kinase A or CaM kinase I (31, 32). The enzyme is conserved from Caenorhabditis elegans to man and presumably plays a critical role in cell behavior because it is expressed in most tissues of the body. The purified enzyme is activated by Ca2+/CaM, but other calcium-independent mechanisms of activation as well as inhibition of activity have been demonstrated. For example, as pointed out above, insulin appears to inhibit the enzyme in some cells, leading to a decrease in EF-2P (21). The mechanism of this effect is still poorly defined but may involve mTOR-dependent phosphorylation of EF-2 kinase because it is reportedly blocked by rapamycin (33). In the present study, we did find a small effect of exogenous insulin on EF-2P levels, consistent with an inhibition of EF-2 kinase, and this was blocked by wortmannin and rapamycin. In addition, the stress-activated pathway initiated by treatments such as protein synthesis inhibitors or ligands such as tumor necrosis factor alpha  can also significantly inhibit EF-2 kinase in epithelial cells (34). This effect is mediated by direct phosphorylation of the enzyme on serine residues by stress-activated protein kinase/p38delta (35). Our results suggest that glucose addition does not lead to an acute inhibition of EF-2 kinase activity that would contribute significantly to the dephosphorylation of EF-2. Nevertheless, it seems likely that the increase in phosphorylation of EF-2 during glucose restriction involves stimulatory effects on kinase activity, rather than just a reversal of PP2A stimulation, because inhibition of PP2A activity by calyculin A in high glucose did not substantially raise EF-2P levels. An attractive possibility is that AMP kinase is responsible for the indirect stimulation of EF-2 kinase under hypoglycemic conditions. Although further work is needed on this question, the fact that AICAR treatment resulted in elevated EF-2P levels in cells maintained in high glucose suggests that a connection between AMP kinase and EF-2 phosphorylation exists. Indeed, low glucose levels do increase AMP kinase in islets (23), and EF-2 phosphorylation levels are sensitive to AMP kinase activation in other cell types (36). Although it is too early to rule out an effect of AMP kinase on EF-2 phosphorylation by a more circuitous route in beta  cells (e.g. via inhibition of PP2A), an AMP kinase stimulation of EF-2 kinase and a consequent increase in EF-2P have been proposed to account for the rapid, reversible shut-off in protein synthesis found in hepatocytes under hypoxic conditions (36). Evidently, the complex regulation of EF-2 phosphorylation at both the kinase and phosphatase levels expands the options available in beta  cells for modulating protein synthetic capacity in response to a variety of inputs (see Fig. 7 for summary).


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Fig. 7.   Model of translational regulation in beta  cells. Extracellular glucose impacts protein synthesis by a variety of mechanisms (dashed lines indicate undefined mechanisms, whereas solid lines represent established pathways). Increased glucose uptake and metabolism alter translational initiation through modulation of eIF-2B activity (10). As shown here, extracellular glucose levels also regulate protein translation rate through the bidirectional modulation of EF-2 phosphorylation. Elevation of metabolites in high glucose causes the PP2A-mediated dephosphorylation of EF-2, contributing to increased protein translation rate. Conversely, reduced metabolites in low glucose favor EF-2 phosphorylation, potentially through an AMP kinase (AMPk)-EF-2 kinase (EF-2k) link, which contributes to the suppression of protein synthesis. Additionally, glucose stimulates insulin secretion and autocrine signaling to protein synthesis through the phosphatidylinositol 3-kinase-Akt-mTOR pathway (8).


    ACKNOWLEDGEMENTS

We thank Dr. C. Newgard for providing the INS-1-derived 832/1 and 832/13 cells and Drs. P. Hansen and J. Corbett for providing the rat islet samples.

    FOOTNOTES

* This work was supported by a Career Development Award (to M. J. B.) and a Research Award (to H. C. P.) from the American Diabetes Association.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.

|| To whom correspondence should be addressed: Dept. of Medicine, University of Chicago, MC1027, 5841 S. Maryland Ave., Chicago, IL 60637. Tel.: 773-702-2346; Fax: 773-834-0486; E-mail: mbrady@medicine.bsd.uchicago.edu.

Published, JBC Papers in Press, March 18, 2003, DOI 10.1074/jbc.M301116200

    ABBREVIATIONS

The abbreviations used are: mTOR, mammalian target of rapamycin; CaM, calmodulin; EF, elongation factor; EF-2P, phospho-elongation factor 2; PP2A, protein phosphatase-2A; KRBH, Krebs-Ringer buffer supplemented with 25 mM Hepes and 0.5% bovine serum albumin; AICAR, 5-aminoimidazole-4-carboxamide 1-beta -D-ribofuranoside.

    REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

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