1 School of Biochemistry and Genetics, Medical School, University of Newcastle, Newcastle upon Tyne, U.K.
2 Target Cell Biology, Novo Nordisk, Bagsvaerd, Denmark
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ABSTRACT |
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DMEM, Dulbeccos modified Eagles medium; FCS, fetal calf serum; Glu, glucose free; G6P, glucose-6-phosphate; GS, glycogen synthase; GSK, GS kinase; PBS, phosphate-buffered saline; PP, protein phosphatase
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INTRODUCTION |
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Glycogen synthesis can also be stimulated in an insulin-independent manner (after exercise), a process associated with glycogen depletion (10). Furthermore, as early as 1965, a reciprocal relationship between glycogen content and glycogen synthase activity was reported in muscle (11).
Previously, we have used human muscle cells in culture to study the control of glycogen synthesis by insulin and growth factors (12,13). In the current study, we examined the effects of glycogen depletion on the rate of glycogen synthesis and the activity of GS in human myoblasts. The effect of subsequent glucose readdition was also studied, and the mechanism leading to stimulation by glucose of GS was analyzed and compared with that for insulin.
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RESEARCH DESIGN AND METHODS |
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Cell culture.
Human myoblasts were grown from needle biopsy samples taken from the gastrocnemius muscle of healthy subjects with no family history of type 2 diabetes and with normal glucose tolerance and normal insulin sensitivity, as assessed using the short insulin tolerance test (13). Myoblasts were maintained in growth medium consisting of Hams F-10 nutrient mixture containing 20% fetal calf serum (FCS), 1% chick embryo extract, 100 U/ml penicillin, and 100 µg/ml streptomycin. All experiments were performed using cells between the 5th and 15th passage at a confluence >80%. Before hormone treatment, cells were incubated for at least 2 h in serum-free medium.
Cellular glycogen content determination.
Total cellular glycogen content was assessed by modification of a previous method (15). After treatment, cells were washed rapidly in ice-cold phosphate-buffered saline (PBS) and scraped into 100 µl of 0.2 mol/l sodium acetate, pH 4.8. Extracts were briefly sonicated using a Soniprep 150, before the addition of 250 mU amyloglucosidase per sample. Samples were incubated for 2 h at 40°C and vortexed regularly to avoid sedimentation. The sample (10 µl) was incubated with an assay cocktail (0.1 mol/l Tris-HCl [pH 8.0], 0.3 mmol/l ATP, 6 mmol/l MgCl2, 5 mmol/l dithiothreitol, 60 µmol/l NADP+, 2.5 U/ml hexokinase, and 1 µg/ml G6P-dehydrogenase) for 30 min at room temperature. Changes in fluorescence, as a result of NADPH production, were determined using an excitation wavelength of 355 nm and an emission wavelength of 460 nm. Reaction blanks were determined as the fluorescence of samples before enzymatic treatment with amyloglucosidase.
Measurement of glycogen synthesis.
Glycogen synthesis was determined as 14C-glucose incorporation into glycogen over a 1-h period, as previously described (13). Results were expressed as picomoles of glucose incorporated into glycogen per minute per milligram of cell protein.
Estimation of glucose uptake.
Glucose uptake was determined as the rate of 2-deoxy-D-[6-3H]glucose uptake, using a modification of a previous method (16). Cells were maintained in the absence of serum for 2 h before the replacement of media with glucose-free (Glu) Dulbeccos modified Eagles medium (DMEM) for 15 min at 37°C. The rate of 2-deoxy-D-[6-3H]glucose uptake was determined during a 5-min incubation with 10 µmol/l 2-deoxy-D-[6-3H]glucose (specific activity 400 dpm/pmol). Reaction blanks were determined as the rate of 2-deoxy-D-[6-3H]glucose uptake in the presence of 0.1 mmol/l cytochalasin B.
After incubation, cells were washed with ice-cold PBS several times and solubilized in 0.05% SDS for 30 min at room temperature. Protein content of samples was assayed using Coomassie protein assay reagent, and uptake of 2-deoxy-D-[6-3H]glucose was determined by liquid scintillation counting.
Assay of glycogen synthase.
Following the indicated treatments, cells were rapidly washed three times with ice-cold PBS and collected, by scraping, into GS extraction buffer (10 mmol/l Tris-HCl [pH 7.8], 150 mmol/l KF, 15 mmol/l EDTA, 60 mmol/l sucrose, 1 mmol/l 2-mercaptoethanol, 10 µg/ml leupeptin, 1 mmol/l benzamidine, and 1 mmol/l phenylmethylsulfonyl fluoride). Cells were then disrupted by briefly sonicating using a Soniprep 150. Glycogen synthase activity was determined in whole lysates as the incorporation of 3H-glucose from uridine-5'-diphosphate [U-3H] glucose into glycogen, as previously described (17). Samples were incubated with reaction cocktail (50 mmol/l Tris-HCl [pH 7.8], 20 mmol/l EDTA, 25 mmol/l KF, 1% glycogen, and 0.4 mmol/l UDP-[3H]glucose [specific activity 3,000 dpm/nmol]), containing either 0.1 mmol/l (active) or 10 mmol/l (total) glucose-6-phosphate for 30 min at 30°C. Results were expressed as fractional activities (active/total). This assay has been optimized to detect the activity changes resulting from dephosphorylation of glycogen synthase (17).
Determination of GSK-3 activity.
Following treatment, cells were washed three times with ice-cold PBS and excess liquid was removed. Cells were then scraped into kinase extraction buffer (100 mmol/l Tris-HCl [pH 7.4] containing 100 mmol/l KCl, 2 mmol/l EDTA, 25 mmol/l KF, 0.1% [vol/vol] Triton X-100, 1 mmol/l benzamidine, 0.1 mmol/l Na3VO4, 1 µg/ml pepstatin, 1 µg/ml antipain, and 1 µg/ml leupeptin), transferred to 1.5 ml Eppendorf tubes, and immediately frozen in liquid nitrogen. GSK-3 activity was determined by a modification of the method reported by Ryves et al. (18), in the presence or absence of 50 mmol/l LiCl (an allosteric inhibitor of GSK-3). Samples (15 µg) were incubated with reaction mixture (50 mmol/l Tris-HCl [pH 7.5] containing 0.1 mmol/l EGTA, 100 mmol/l Mg-Acetate, 5 µmol/l protein kinase inhibitor, 100 µmol/l [-32P]ATP [
600 cpm/pmol], and 0.2 mg/ml phospho-eIF2B peptide substrate) (14) for 15 min at 30°C. After incubation, samples containing the radiolabelled peptide product were spotted onto 3 cm2 Whatman P81 phosphocellulose paper squares. After washing in 175 mmol/l phosphoric acid with four changes, the papers were dried, and phosphate incorporation was determined by liquid scintillation counting. Phosphate incorporation into peptide substrate in the presence of lithium was equivalent to that observed using control dephosphopeptide. GSK-3 activity was regarded as the difference between values in the absence and presence of lithium. Enzyme activity was defined as that which catalyzes the incorporation of 1 nmol of phosphate into peptide substrate in 1 min.
Western blotting.
Samples were fractionated on 10% gels by SDS-PAGE. After separation, proteins were transferred onto polyvinylidine fluoride membrane and probed with antiGSK-3 and GSK-3ß phosphospecific antibodies (1:1,000). Anti-rabbit peroxidase conjugate (1:2,000) was used as secondary antibody, and immunoreactive proteins were determined using enhanced chemiluminescence. Membranes were stained with protein-reactive copper stain (0.05% [wt/vol] copper phthalocyanine 3,4',4',4'-tetrasulphonic acid in 12 mmol/l HCl) to allow molecular weight estimation of immunoreactive proteins, as compared with those of proteins of known molecular weight.
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RESULTS |
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Time and concentration dependence of GS activation by glucose in glycogen-depleted myoblasts.
Myoblasts were incubated in DMEM Glu- for 5 h before treatment with glucose-containing media for increasing periods of time. Glucose treatment (6.1 mmol/l) caused a rapid time-dependent increase in the fractional activity of GS, with stimulation being observed within 2 min and reaching a maximum fractional activity of 0.3 after 1015 min (Fig. 2A). After 30 min of glucose re-administration, the fractional activity of GS started to decrease, reaching
0.1 after 4 h, but remaining constant thereafter up to 8 h (Fig. 2B). During the same period, the glycogen content of the cells increased, reaching a value
80% of that in control cells. The stimulation of GS was dependent on the concentration of glucose added, with significant stimulatory effects being observed in response to 1.5 mmol/l (Fig. 2C).
Combined effect of insulin and glucose on GS activity and glycogen synthesis in glycogen-depleted myoblasts.
The combined effects of glucose readdition and insulin on cells cultured in the absence of glucose was then examined. Treatment of cells with 100 nmol/l insulin for 15 min after preincubation in glucose-containing media for 5 h led to an 1.6-fold increase in the fractional activity of GS from 0.040 ± 0.010 to 0.071 ± 0.020 (Fig. 3A). Similarly, GS activity was increased by insulin
1.7-fold from 0.214 ± 0.021 to 0.337 ± 0.037 in myoblasts that had been glucose-depleted for 5 h and that had glucose re-administered during the 15 min of insulin treatment; this finding indicates that the effects of glucose and insulin are additive and act by different mechanisms. In the absence of readministration of glucose, stimulatory effects of insulin on GS activity were minimal after glycogen depletion (data not shown).
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Effect of glucose deprivation on 2-deoxyglucose uptake in human myoblasts.
An increase in the rate of 2-deoxyglucose uptake was observed in myoblasts deprived of glucose for increasing time, reaching 1.7-fold after 5 h (Fig. 4A). The most significant increase in the rate of 2-deoxyglucose uptake was observed after the first 2 h in DMEM Glu-: 35.45 ± 1.99 pmol · min1 · mg 1 in cells maintained in the presence of glucose and 49.58 ± 3.93 pmol · min1 · mg 1 in cells deprived of glucose for 2 h.
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Mechanisms involved in activation of GS by glucose.
To investigate the mechanisms by which glucose activates GS, selective inhibitors of signaling pathways known to be stimulated by insulin were used (Fig. 5). DMEM Glu- supplemented with 5.5 mmol/l glucose was added for 15 min to myoblasts previously depleted of glucose for 5 h, resulting in an 4.2-fold increase in GS activity ratio. Preincubation of cells with rapamycin, which selectively inhibits the activation of p70s6k, failed to inhibit this stimulatory effect of glucose on GS activation. Treatment of glycogen-depleted myoblasts with either the MEK inhibitor, PD098059, or the PI 3-kinase inhibitor wortmannin partly reduced the activity state of GS obtained in response to glucose readministration. However, this is essentially attributable to these inhibitors reducing the basal activity state of GS, as previously observed (13). Therefore, these findings indicate that the mechanisms involved in the activation of GS by glucose are independent of the activity of PI 3-kinase, the classical mitogen-activated protein kinase pathway, and the rapamycin-sensitive pathway leading to activation of p70s6k. Furthermore, during glucose readministration, there was no observable decrease in the activity of GSK-3 and no detectable phosphorylation of that protein, as detected by phosphospecific antiGSK-3 antibodies (Fig. 6). No changes in the activity of protein kinase B were detected (not shown). Thus, the mechanism underlying the effects of glucose/glycogen are apparently distinct from those utilized by insulin.
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The activity of endogenous PPs against GS was then measured in extracts from control and glycogen-depleted cells. Because it has been demonstrated that GS becomes a better substrate for PPs in the presence of G6P (21), this was carried out over a range of G6P concentrations. No differences were found in the rate of activation of GS by endogenous phosphatases in extracts prepared from control and glycogen-depleted cells. For example, at a physiological concentration of 0.25 mmol/l G6P in the extract, the effect of endogenous phosphatases on GS activity in extracts of cells preincubated in the presence of glucose led to an increase of 3.44 ± 0.29 pmol · min1 · mg 1 GS activity in 30 min, compared with an increase of 3.85 ± 0.60 pmol · min1 · mg1 in 30 min in cells preincubated in the absence of glucose for 5 h. Therefore, glycogen depletion does not appear to stimulate phosphatase activity against GS, at least when measured subsequently in cell extracts.
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DISCUSSION |
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The activation of GS is observed by the use of an assay optimized to detect activity changes resulting from phosphorylation/dephosphorylation of the enzyme in hepatocytes (17). This is expressed as a fractional activity, i.e., activity in the presence of 0.1 mmol/l G6P as a fraction of the activity in 10 mmol/l G6P. Similar methodologies have been applied to studies of GS activity in muscle, where activity has been reported as a fractional velocity or as A0.5, the G6P concentration required for half maximal activity (22).
The molecular mechanism responsible for this stimulatory effect of glucose is a primary concern. The alterations in the fractional activity of GS are almost certainly because of a change in the phosphorylation state of the enzyme, as the removal of small activatory/inhibitory molecules from cell extracts failed to alter the elevated GS activity. Inhibition of GSK-3 is thought to be the key event in the activation of muscle GS by insulin; however, selective inhibitors of the known insulin-stimulated pathways leading potentially to GSK-3 inhibition failed to prevent the activation of GS during the refeeding of glucose to glycogen-depleted cells (Fig. 5). Furthermore, no inhibition or phosphorylation of GSK-3 was observed in response to glucose (Fig. 6). However, the involvement of GSK-3 inhibition in this process cannot be completely ruled out, as GSK-3 could be inhibited by an alternative, yet unidentified, mechanism not involving phosphorylation of the single serine residue recognized by the phosphospecific antibodies and not being retained when the enzyme is assayed in cellular extracts. In that regard, allosteric regulation of GSK-3 by glycogen or small metabolites must be considered. A recent study performed in rat skeletal muscle demonstrated an exercise-induced increase in GS activity accompanied by inactivation of GSK-3 (23). However, in this model, GSK-3 inactivation was not associated with phosphorylation of the serine 9/21 (/ß) residues, and it was suggested that glycogen content might regulate GSK-3 activity through direct allosteric activation of the kinase by the glycogen particle, although no evidence was offered to support this hypothesis.
The activity of GS is dependent on the relative contribution of GSK-3 and PP1 in determining the phosphorylation state of the enzyme. Phosphorylation of the glycogen-binding subunit of PP1 has been postulated as a mechanism for activation of that enzyme in response to insulin; however, a growing body of evidence suggests that this is not the case (rev. in [1]). After exercise in human muscle, no increase in total or glycogen-associated PP activity was observed; however, the rate of reactivation of GS by endogenous phosphatases was increased, suggesting that GS became a better substrate for PP1 after exercise (24). In the present work, no increase in the phosphatase activity directed toward GS was observed after the glycogen depletion of human myoblasts. However, it is possible that PPs, principally PP1, can alter GS activity in vivo, independent of changes in the intrinsic activity of the phosphatase detected in in vitro assays. For example, effects of changes in intracellular G6P concentration to enhance the ability of PP1 to dephosphorylate GS (21), or the effect of overexpression of a glycogen-binding subunit of PP1 in CHO cells, which results in an increase in basal and insulin-stimulated glycogen synthesis (25), would not be detected as a change in phosphatase activity in cell extracts.
Work in rat adipocytes has previously shown that glucose can activate GS in the absence of insulin (26), an effect attributed to increased glucose transport leading to accumulation of G6P, which can then increase PP activity toward GS. The extent to which such a mechanism contributes to the observations in muscle reported in this study remains to be established, although studies in mouse diaphragm have demonstrated a modest stimulatory effect of glucose on GS activity (27). The model from rat adipocytes does not account for the effect of glycogen stores on the activation, and a recent study in human myotubes has indicated that glycogen repletion, after glucose administration to cells that have been depleted of glycogen by overexpression of glycogen phosphorylase, is not dependent on increases in intracellular G6P concentration (28).
However, metabolic flux through G6P has been suggested as the hub of coordinate regulation of muscle glycogen synthesis (29); changes in GS activity are a consequence of alterations in intracellular G6P concentration, a result of increased glucose uptake and hexokinase activity. G6P is an allosteric activator of GS, but also serves to make GS a better substrate for dephosphorylation by PPs (21). Low glycogen content in vivo could increase glucose uptake and hexokinase activity, resulting in an increase in intracellular G6P concentration and consequently in an increase in GS activity, although no obvious mechanism for this is known.
A further consideration is whether glycogen depletion followed by glucose refeeding alters the distribution of GS and its regulatory proteins within the myoblast. PP1, GSK-3, and GS are all capable of redistributing within the cell in response to metabolic and hormonal stimuli (5,30,31). If glucose (or one of its metabolites) caused either increased interaction of GS and PP1 or decreased interaction of GS and GSK-3 in glycogen-depleted cells, this could explain the activation of GS in response to this nutrient.
An exercise-induced increase in glycogen resynthesis after glycogen depletion can only occur if adequate substrate is available. Indeed, after glucose deprivation of cultured human muscle cells, there was a twofold increase in the subsequent rate of 2-deoxyglucose uptake. Increased glucose transporter numbers at the plasma membrane has been suggested as the mechanism for increased glucose uptake postexercise, and in rat skeletal muscle, a 1.8-fold increase in glucose transporters found at the plasma membrane was observed after exercise (32). The relationship between glycogen and membrane permeability to glucose is apparently reciprocal, with increasing glycogen content postexercise leading to a decrease in glucose uptake (33).
In summary, the work reported here has highlighted the important role of glucose in stimulating glycogen synthesis in muscle after glycogen depletion. Recent elegant work using 31P nuclear magnetic resonance to study glycogen metabolism in human muscle in vivo is yielding important information on the effects of glycogen on glycogen synthesis (34). However, work with human muscle cells in culture has the benefit of providing a means of independently varying glycogen content, extracellular glucose concentration, and insulin levels. The data reported here are consistent with work in human muscle in vivo showing activation of GS after exercise-mediated glycogen depletion (22), leading to glycogen repletion in an insulin-independent phase (10). The molecular mechanism leading to the activation of GS by glucose after glycogen depletion is as yet undefined, but is apparently distinct from the upstream signaling mechanisms used in the actions of insulin on this parameter. Recent evidence suggests that AMP-activated protein kinase may play a role in insulin-independent exercise-stimulated glucose uptake (35). The possibility that it is also involved in the stimulation of glycogen synthesis after glycogen depletion is an attractive one, although no evidence is currently available to support this. Clearly, how the two different signaling pathways interact has implications for the overall control of glycogen synthesis in control subjects and patients with type 2 diabetes.
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ACKNOWLEDGMENTS |
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We thank Dr. Mark Walker and Prof. Doug Turnbull for obtaining the initial muscle biopsies and Dorothy Fittes for technical assistance with the cell culture.
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FOOTNOTES |
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Received for publication 7 June 2000 and accepted in revised form 20 December 2000.
R.H. has received funds from Novo Nordisk. J.G.M. is employed by and holds stock in Novo Nordisk. S.J.Y. holds stock in Xcellsyz, has received honoraria from Novo Nordisk and Glaxo Wellcome, and has received funds from Novo Nordisk and SmithKline Beecham.
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REFERENCES |
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