1 Department of Endocrinology, Hvidovre Hospital and Clinical Trial Unit, University of Copenhagen, Copenhagen, Denmark
2 Department of Clinical Physiology, Karolinska Hospital, Karolinska Institutet, Stockholm, Sweden
3 Steno Diabetes Center, Gentofte, Denmark
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ABSTRACT |
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INTRODUCTION |
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In patients with type 2 diabetes, defects in insulin-stimulated glucose metabolism in skeletal muscle have been attributed to impaired glucose transport (7,8), glycogen synthesis (9), and glycogen synthase activation (10). These defects may result from impaired insulin signal transduction (11). The molecular signaling mechanisms by which insulin regulates glucose uptake and storage is initiated by the binding of insulin to its specific cell-surface receptor, which results in receptor autophosphorylation and activation of insulin receptor tyrosine kinase (IRTK). IRTK phosphorylates tyrosine residues on insulin receptor substrates (IRS-14). IRS-1 seems to be the major postreceptor component of the signaling machinery involved in mediating GLUT4 translocation, glucose transport, and glucose metabolism in human skeletal muscle (12). Furthermore, in insulin-resistant rodent skeletal muscle, the decrease in total phosphotyrosine-associated phosphoinositide 3-kinase (PI 3-kinase) activity closely parallels the reduction in IRS-1associated PI 3-kinase activity (13). Binding of IRS-1 to the regulatory subunit of PI 3-kinase results in activation of the kinase and initiation of a phosphorylation cascade involving phosphoinositide-dependent protein kinase-1 and the downstream kinase Akt (also known as protein kinase B) (14,15). Among other insulin-mediated effects, Akt phosphorylates and inactivates glycogen synthase kinase-3, resulting in a greater degree of dephosphorylation and thereby activation of glycogen synthase (16). Impaired insulin action on glycogen synthase in skeletal muscle represents a major defect that correlates with insulin resistance in the pathway of nonoxidative glucose metabolism in patients with type 2 diabetes (12,17) and their nondiabetic first-degree relatives (4,18). Thus, impaired insulin action on Akt in skeletal muscle from prediabetic and diabetic individuals may contribute to the pathophysiology of type 2 diabetes.
Insulin receptor binding and IRTK activity have been reported to be either normal (19) or decreased (17) in muscle biopsies from patients with type 2 diabetes. Despite the inconsistent findings for immediate insulin signaling events at the level of the receptor, insulin action on PI 3-kinase in skeletal muscle from patients with overt type 2 diabetes is impaired (11,12,20,21). Moreover, we recently reported decreased Akt activity in isolated skeletal muscle from patients with type 2 diabetes in response to supraphysiological insulin concentrations (22). In contrast, Akt activity is normal in muscle biopsies obtained from patients with type 2 diabetes during a euglycemic-hyperinsulinemic clamp, whereby insulin levels were maintained at a high physiological level (12,21). Therefore, the role of Akt in the development of insulin resistance in type 2 diabetes is unclear.
One explanation for the conflicting results on IRTK activity may be the presence of hyperglycemia and its dual effects on glucose metabolism in patients with overt type 2 diabetes. Hyperglycemia (or "glucose toxicity") may be a major cause of insulin resistance and defective signal transduction in skeletal muscle from patients with type 2 diabetes (23). Hyperglycemia also has a compensatory effect on insulin action on signal transduction and downstream metabolic responses in skeletal muscle, allowing for normal insulin-stimulated glucose uptake and muscle glycogen synthase activation when patients with type 2 diabetes are studied during their ambient hyperglycemic state (24,25). One way to avoid the influence of hyperglycemia on glucose uptake and metabolism is to study nondiabetic first-degree relatives of patients with type 2 diabetes with a known high risk for the development of overt type 2 diabetes (4,18,26,27). Importantly, this approach may also reveal a potential primary defect(s) at the level of signal transduction in people who are at high risk for the development of type 2 diabetes.
The aim of the present study was to determine whether impaired insulin signal transduction at the level of IRS-1, PI 3-kinase, and/or Akt is associated with defects in glucose uptake and metabolism (oxidative and/or nonoxidative) in prediabetic individuals. To ensure an a priori high risk for the later progression to overt type 2 diabetes, we studied first-degree relatives of patients with type 2 diabetes with impaired glucose tolerance but normal HbA1c levels.
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RESEARCH DESIGN AND METHODS |
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Protocol for in vivo studies.
All studies commenced at 0800 h after a 10-h overnight fast. A polyethylene catheter was inserted into an antecubital vein for infusion of test substances. Another polyethylene catheter was inserted into a contralateral wrist vein for blood sampling. This hand was kept in a heated plexiglas box throughout the test to obtain arterialized venous blood (29). Basal samples for insulin, C-peptide, free fatty acid (FFA), and glucose determination were obtained. Each study was initiated with a basal period (-160 min), at which time the tracer bolus was given. Indirect calorimetry was performed during the predefined basal steady state period (-70 to -40 min) for basal glucose oxidation measurements. Thereafter, a basal (noninsulin-stimulated) muscle biopsy was obtained (-40 to -30 min). From -30 to 0 min, an intravenous glucose tolerance test (IVGTT) was performed to characterize the first-phase insulin response.
Euglycemic-hyperinsulinemic clamp.
Squared priming was performed (09 min) with a stepwise decline in the insulin (Actrapid; Novo Nordisk, Bagsvaerd, Denmark) infusion rate every third minute, thereby reducing the insulin infusion rate from 10080 to 6040 mU · m-2 · min-1. Thereafter, the insulin infusion rate was fixed at 40 mU · m-2 · min-1 from 9 to 120 min. Plasma glucose concentration was maintained constant at euglycemia, using a variable glucose infusion (180 g/l) (30). Plasma glucose concentration was monitored every 5 min using an automated glucose oxidase method (Glucose Analyzer 2; Beckman Instruments, Fullerton, CA). Indirect calorimetry was performed during the insulin-stimulated steady-state period (90120 min) to measure insulin-stimulated glucose oxidation.
Tritiated glucose.
At 160 min before the start of insulin (-160 min), an adjusted primed (11 µCi · [fasting plasma glucose concentration/5 mmol/l]) continuous (0.11 µCi/min) infusion of 3-[3H]glucose (New England Nuclear, Boston, MA) was initiated to ensure isotope equilibrium (31). The tracer infusion was continued throughout the 120-min period of insulin infusion. To obtain constant specific activity (SA) during insulin infusion, we added tritiated glucose to the infused glucose solution (54 µCi/500 ml in an 18% glucose solution) (32). Blood samples were drawn in fluoride-treated tubes at the beginning and end of the 30-min basal steady-state period and every 10 min thereafter during the 30-min insulin-stimulated steady-state period for determination of 3-[3H]glucose activity. Plasma 3-[3H]glucose was measured every 30 min during the rest of the study. Plasma 3-[3H]glucose concentration was determined from radioactivity in the evaporated (to avoid 3-[3H]water) 0.5-ml plasma samples (31).
Indirect calorimetry.
A ventilated canopy was placed over the participants head (Deltatrac; Datex, Helsinki, Finland), and continuous gas exchange was determined. Inspired and expired air was analyzed for oxygen content using a paramagnetic differential oxygen sensor and for carbon dioxide tension using an infrared carbon dioxide sensor. Oxygen consumption and carbon dioxide production were recorded and calculated each minute. After an equilibrium period of 10 min, the average gas exchange during the two 30-min steady-state periods (basal and insulin-stimulated) (-70 to -40 min and 90120 min) were used to calculate rates of glucose oxidation as previously described (33,34).
Muscle biopsy.
Muscle biopsies were obtained under local anesthesia, from m. vastus lateralis using a modified Bergströms needle (including suction), at -40 (basal) and 120 min (insulin-stimulated). Biopsies were frozen in liquid nitrogen and stored at -80°C for later analysis for signaling transduction studies. Previous in vitro and in vivo studies showed that insulin-mediated signal transduction in human muscle is sustained between 15 min and 3 h (12,21).
IVGTT.
An IVGTT was performed from -30 min to 0 min. A bolus of 300 mg glucose/kg body mass (18% glucose) was infused over 1 min. Blood samples were collected at -10, -5, 0, 2, 4, 6, 8, 10, 15, and 30 min. All samples were analyzed for plasma glucose, insulin, and C-peptide.
Blood chemistry.
Plasma glucose was determined using an automated glucose oxidase method (Glucose Analyzer 2; Beckman Instruments). Tritiated glucose was measured as described by Hother-Nielsen and Beck-Nielsen (31). Plasma insulin and C-peptide concentration were determined using the 1234 AutoDELFIA immunoassay system (Wallac Oy, Turku, Finland). Plasma FFA were quantified using an enzymatic colorimetric method (Wako Chemicals, Neuss, Germany).
Materials and antibodies.
PI was from Avanti Polar Lipids (Alabaster, AL). The aluminum-backed Silica Gel 60 thin-layer chromatography plates were from EM Separations (Gibbstown, NJ). Protein A-Sepharose was purchased from Pharmacia (Uppsala, Sweden). All other chemicals were purchased from Sigma (St. Louis, MO) or Merck (Rahway, NJ). Antiphosphotyrosine and p85 antibodies were from Transduction Laboratories (Lexington, KY). IRS-1 polyclonal antibody was from Dr. Ton Maassen (Leiden University, Leiden, the Netherlands). Polyclonal antibodies to detect Akt phosphorylation or Akt protein were from New England Biolabs (Beverly, MA). These antibodies were produced by immunizing rabbits with a KLH-coupled synthetic phosphopeptide (Akt phosphorylation) or synthetic peptide (Akt protein expression) corresponding to residues 466479 of mouse Akt.
Tissue processing.
Muscle biopsies were homogenized in ice-cold homogenizing buffer (50 mmol/l Hepes [pH 7.6], 150 mmol/l NaCl, 1% Triton-X 100, 1 mmol/l Na3VO4, 10 mmol/l NaF, 30 mmol/l Na4P2O7, 10% (vol/vol) glycerol, 1 mmol/l benzamidine, 1 mmol/l dithiothreitol [DTT], 10 µg/ml leupeptin, 1 mmol/l phenylmethylsulfonyl fluoride, and 1 µmol/l microcystin) using a glass-on-glass rotating homogenizer and subjected to centrifugation (12,000 g for 10 min at 4°C). Protein was determined in the supernatant using a commercial kit (Bio-Rad, Richmond, CA).
IRS-1 tyrosine phosphorylation.
From the remaining homogenate described above, an aliquot of the supernatant (800 µg) was immunoprecipitated with antiIRS-1 coupled to protein A-Sepharose. Immunoprecipitates were washed four times in ice-cold homogenizing buffer, resuspended in Laemmli sample buffer with 100 mmol/l DTT, and heated (95°C) for 4 min. Proteins were separated by SDS-PAGE, transferred to polyvinylidene difluoride (PVDF) membranes incubated with antiphosphotyrosine antibodies, washed, and incubated with appropriate secondary antibodies. The reactions were visualized by enhanced chemiluminescence (ECL; Amersham, Arlington Heights, IL) and quantified by densitometry. Results are presented as arbitrary densitometric units.
PI 3-kinase activity.
Muscle specimens were homogenized as described above, and an aliquot of the supernatant (800 µg) was immunoprecipitated overnight (4°C) with antiphosphotyrosine or antiIRS-1 antibody coupled to protein A-Sepharose. PI 3-kinase activity was assessed directly on the protein A-Sepharose beads as previously reported (35). Reaction products were resolved by thin-layer chromatography and quantified using a PhosphorImager (Bio-Rad). Results are presented as arbitrary phosphoimager units.
Akt phosphorylation.
Aliquots of muscle homogenate (40 µg) were solubilized in Laemmli sample buffer with 100 mmol/l DTT and heated (95°C) for 6 min. Proteins were separated by SDS-PAGE, transferred to PVDF membranes, and immunoblotted as described above, using a phospho-specific antibody that recognizes Akt when phosphorylated at Ser 473 (New England Biolabs). Phosphorylated Akt was visualized by ECL and quantified by densitometric scanning.
Protein expression.
For protein expression of IRS-1, p85 subunit of PI 3-kinase, and Akt, an aliquot (40 µg) of supernatant was resuspended in sample buffer and heated (95°C) for 6 min. Proteins were separated by SDS-PAGE, transferred to PVDF membranes, and blocked as described above. Membranes were incubated with the appropriate primary antibodies as indicated above, washed, and incubated with appropriate secondary antibodies as recommended by the supplier (Amersham). Proteins were visualized by ECL and quantified by densitometry.
Calculations.
Hepatic glucose production (HGP) and glucose disposal rate (Rd) were calculated during the steady-state periods using Steeles nonsteady-state equation (36). During the insulin-stimulated steady-state period, Rd and HGP were calculated at 10-min intervals. In the calculations, the distribution volume of glucose was taken as 200 ml/kg body wt and the pool fraction of 0.65 (36). HGP during the basal steady-state period was equal to the rate of appearance of 3-[3H]glucose (Ra), whereas HGP during the clamp steady-state period was calculated as the difference between Ra and the glucose infusion rate. Nonoxidative glucose metabolism was calculated by subtracting the glucose oxidation rate (determined by indirect calorimetry) from Rd. Glucose metabolism data were expressed as mg · kg FFM-1 · min-1. The acute insulin response to intravenous glucose was calculated as the incremental area under the plasma insulin concentration curve (AUC) from 0 to 10 min (AUC10 min insulin).
Statistical analysis.
The results are represented as means ± SE. Differences between groups were compared by Mann-Whitney rank-sum test. Paired comparisons were performed using Wilcoxon matched-pairs signed rank test. Correlation analyses were performed using Spearman correlation analysis. Significance was accepted at P < 0.05.
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RESULTS |
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Glucose metabolism.
SA for tritiated glucose was similar between the IGT relatives and control subjects under basal (210 ± 14 vs. 205 ± 8 cpm, respectively) and insulin-stimulated (246 ± 12 vs. 229 ± 10 cpm, respectively) steady-state periods. Basal and insulin suppressed rates of HGP were similar in the IGT relatives and control subjects (Table 1).
Insulin increased the Rd in control subjects 3.8-fold (basal versus insulin-stimulated, 2.30 ± 0.24 vs. 8.79 ± 0.67 mg · kg FFM-1 · min-1; P = 0.004) and 1.7-fold in IGT relatives (3.02 ± 0.21 vs. 5.03 ± 0.42; P = 0.008). The mean basal Rd were similar between the IGT relatives and control subjects, whereas the insulin-stimulated Rd was lower in IGT relatives compared with control subjects (P = 0.002; Fig. 1). The insulin-stimulated increase in Rd over basal levels was significantly lower in IGT relatives (2.01 ± 0.45 vs. 6.39 ± 0.84; P = 0.002). Basal glucose metabolism was similar between IGT relatives and control subjects, with similar rates of basal oxidative (IGT relatives versus control subjects, 1.88 ± 0.20 and 1.61 ± 0.16, respectively) and nonoxidative (IGT relatives versus control subjects, 1.14 ± 0.27 and 0.69 ± 0.24, respectively) components of glucose metabolism. During insulin stimulation, oxidative (2.76 ± 0.22 vs. 3.48 ± 0.13, respectively; P = 0.02) and nonoxidative (2.27 ± 0.55 vs. 5.31 ± 0.68, respectively; P = 0.01) glucose metabolism was lower in IGT relatives versus control subjects (Fig. 1). Furthermore, the insulin-stimulated increase over basal glucose metabolism was lower in IGT relatives versus control subjects for oxidative (0.89 ± 0.17 vs. 1.85 ± 0.11, respectively; P < 0.0001) and nonoxidative (1.13 ± 0.40 vs. 4.53 ± 0.80, respectively; P = 0.006) components of glucose metabolism.
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IRS-1 tyrosine phosphorylation.
Physiological hyperinsulinemia increased IRS-1 tyrosine phosphorylation in skeletal muscle from control subjects 3.9-fold (basal versus insulin-stimulated, 80.2 ± 18.4 vs. 314.8 ± 57.6 arbitrary units; P = 0.008; Fig. 2A). Conversely, insulin infusion did not significantly alter IRS-1 tyrosine phosphorylation in skeletal muscle from IGT relatives (201.0 ± 108.1 vs. 190.9 ± 35.1 arbitrary units; NS). Basal IRS-1 tyrosine phosphorylation tended to be higher in IGT relatives, although this difference was not significant (P = 0.82). Insulin-stimulated IRS-1 tyrosine phosphorylation was slightly lower in IGT relatives compared with control subjects, although this difference did not reach statistical significance. The insulin-stimulated increase in IRS-1 tyrosine phosphorylation over basal was greater in control subjects versus IGT relatives (234.6 ± 59.4 vs. -10.0 ± 81.4 arbitrary units, respectively; P = 0.046). IRS-1 protein expression was similar between IGT relatives and control subjects (1.1 ± 0.3 vs. 1.2 ± 0.3 arbitrary units; NS).
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IRS-1associated PI 3-kinase activity.
In a subset of IGT first-degree relatives of patients with type 2 diabetes (n = 6) and control subjects (n = 6), sufficient material was available to assess IRS-1associated PI 3-kinase in basal and in vivo insulin-stimulated muscle (Fig. 2C). Physiological hyperinsulinemia increased IRS-1associated PI 3-kinase activity 3.5-fold in control subjects (basal versus insulin-stimulated, 32.2 ± 1.6 vs. 111.3 ± 27.9 arbitrary units; P = 0.03). In contrast, insulin did not increase IRS-1associated PI 3-kinase activity in skeletal muscle from IGT relatives (78.1 ± 10.3 vs. 108.7 ± 21.2 arbitrary units, for basal and insulin-stimulated conditions, respectively; NS), a finding consistent with data for phosphotyrosine-associated PI 3-kinase activity. When comparing responses for IRS-1associated PI 3-kinase activity between IGT relatives and control subjects, basal activity was greater in IGT relatives (P = 0.002), and insulin-stimulated activity was similar. Consistent with data for phosphotyrosine-associated PI 3-kinase activity, the insulin-stimulated increase in IRS-1associated PI 3-kinase activity over basal was greater in control subjects compared with IGT relatives (79.1 ± 28.7 vs. 30. 6 ± 22.7 arbitrary units, respectively), although because of the large degree of variability within the groups, this difference was not significant (P = 0.43).
Akt phosphorylation.
The serine/threonine kinase Akt (PKB/Rac) is a downstream target of PI 3-kinase (37,38,39). In vivo basal and insulin-stimulated Akt phosphorylation was assessed in skeletal muscle from IGT relatives and control subjects (Fig. 2D). Insulin increased serine phosphorylation of Akt 16.8-fold in control subjects (basal versus insulin-stimulated, 18 ± 6 vs. 303 ± 85 arbitrary units; P = 0.004) and 6.7-fold in IGT relatives (20 ± 5 vs. 137 ± 38 arbitrary units; P = 0.008). In contrast to our results for IRS-1 and PI 3-kinase, basal serine phosphorylation of Akt was similar between IGT relatives and control subjects, and insulin-stimulated Akt serine phosphorylation tended to be lower in IGT relatives (P = 0.11). The insulin-stimulated increase in Akt serine phosphorylation over basal was lower in the IGT relatives versus control subjects (116 ± 34 vs. 285 ± 85 arbitrary units; P = 0.11). Akt protein expression was similar between IGT relatives and control subjects (2.1 ± 0.9 vs. 2.9 ± 0.6 arbitrary units, respectively).
Correlation analysis.
The incremental increase in IRS-1 tyrosine phosphorylation, PI 3-kinase activity, and Akt serine phosphorylation during in vivo insulin infusion was weakly correlated to the increase in glucose disposal, as measured in the total study population (n = 1517; IRS-1 tyrosine phosphorylation: r = 0.52 and P = 0.04; PI 3-kinase activity: r = 0.42 and P = 0.09; and Akt serine phosphorylation: r = 0.43 and P = 0.08). The incremental increase in IRS-1associated PI 3-kinase activity did not correlate with the increase in glucose disposal (r = -0.02 and P = 0.93). When the two groups were considered separately, insulin-stimulated glucose disposal was not significantly correlated to phosphorylation/activity of any the components of the insulin signal transduction cascade measured, including IRS-1 tyrosine phosphorylation, PI 3-kinase activity, and Akt serine phosphorylation.
Because elevated basal IRS-1 tyrosine phosphorylation and PI 3-kinase activity was noted in the IGT relatives, correlation analysis was performed between these parameters and plasma insulin and glucose levels. Basal levels of phosphotyrosine-associated PI 3-kinase activity, IRS-1associated PI 3-kinase activity, and Akt phosphorylation were independently correlated with basal insulin levels in all participants (phosphotyrosine-associated PI 3-kinase activity: r = 0.59 and P = 0.012; IRS-1associated PI 3-kinase activity: r = 0.72 and P = 0.008; Akt phosphorylation: r = 0.63 and P = 0.007). When parameters were correlated for the individual study groups, basal insulin level was also correlated with PI 3-kinase activity and Akt serine phosphorylation (PI 3-kinase activity: r = 0.83 and P = 0.008; Akt serine phosphorylation: r = 0.81 and P = 0.01) in control subjects but not in IGT relatives (Figs. 3B and D). IRS-1 tyrosine phosphorylation and insulin level were not correlated under basal conditions (Fig. 3A). Furthermore, when comparisons were made for all participants or for the individual study groups, basal phosphorylation/activation of the insulin signaling intermediates was not correlated with basal plasma glucose level (data not shown).
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DISCUSSION |
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We observed impairments in both oxidative and nonoxidative components of insulin-stimulated glucose metabolism in the IGT relatives. Thus, our findings are consistent with the hypothesis that defects in both glucose transport and glycogen synthesis contribute to whole-body insulin resistance in skeletal muscle from IGT relatives. Peripheral insulin resistance in first-degree relatives of patients with type 2 diabetes and in people with IGT is primarily due to a quantitatively major defect in the pathway of nonoxidative glucose metabolism (40), which is tightly correlated with a defect in insulin activation of muscle glycogen synthesis and muscle glycogen synthase enzyme activity (4,18). The extent to which defective muscle glycogen synthesis in IGT relatives is explained by decreased glucose transport (41) or defective glycogen synthase enzyme activity is a topic of current debate (4,18), and the relative importance of each pathway may depend on the study design, the analytical methods used (42,43), and the individuals investigated.
The extent to which muscle insulin resistance in first-degree relatives represents a primary underlying genetic defect responsible for the risk of developing type 2 diabetes is unknown. One hypothesis is that a primary ß-cell abnormality, associated with early insulin hypersecretion, causes insulin resistance as a result of hyperinsulinemia (44). Alternatively other endocrine or paracrine substances, such as FFA and TNF- (45), may induce insulin resistance. We have reported normal insulin-stimulated glucose uptake and metabolism in isolated muscle strips from patients with type 2 diabetes during in vitro incubation under euglycemic conditions, in the absence of endocrine and paracrine substances (9). This finding supports the hypothesis that in some patients with type 2 diabetes, muscle insulin resistance is secondary to an altered metabolic milieu. Similarly, a recent report provided evidence that proximal insulin-signaling parameters elicit a normal response in cultured myotubes prepared from muscle biopsies from insulin-resistant nondiabetic individuals (42).
Insulin increased IRS-1 tyrosine phosphorylation and PI 3-kinase activity in skeletal muscle from control subjects, consistent with our earlier report (11). Conversely, in skeletal muscle from IGT relatives, insulin infusion did not alter either IRS-1 tyrosine phosphorylation or PI 3-kinase activity, a finding similar to our earlier report in patients with insulin-resistant type 2 diabetes (11). Protein expression of IRS-1, the p85 subunit of PI 3-kinase, and Akt was similar between IGT relatives and control subjects. Given the degree of whole-body insulin resistance in the IGT participants, impaired insulin action at these early components of the insulin signaling machinery in skeletal muscle may precede the development of overt type 2 diabetes. In contrast to our findings for IRS-1 and PI 3-kinase, insulin increased serine phosphorylation of Akt in both control subjects and IGT relatives. Discordance between in vivo insulin action on PI 3-kinase and Akt has previously been noted in skeletal muscle from patients with type 2 diabetes (21). However, in the former study, the absolute level of insulin-stimulated PI 3-kinase activity was depressed in skeletal muscle from patients with diabetes, whereas the absolute level of insulin-stimulated Akt activity was normal, potentially denoting an important difference between these studies.
In the present study, insulin-stimulated phosphorylation/activity of IRS-1, PI 3-kinase, and Akt was not significantly decreased in an absolute sense in skeletal muscle from IGT relatives compared with control subjects. Rather, the elevated basal phosphorylation/activity of these signal transduction parameters may possibly mask or inhibit any further increase in signal transduction in response to insulin in skeletal muscle from the IGT relatives. However, the precise molecular mechanism that accounts for the lack of insulin response is unknown. It is interesting that the finding of elevated basal signal transduction at the level of these proximal parameters in skeletal muscle from insulin-resistant IGT relatives is consistent with a recent report of a significantly greater basal IRS-1 tyrosine phosphorylation (1.7-fold) in skeletal muscle from insulin-resistant patients with type 2 diabetes, compared with lean control subjects (20). Furthermore, insulin did not elicit a further increase in IRS-1 phosphorylation in skeletal muscle from patients with type 2 diabetes (20), a finding comparable with that noted for IGT relatives. Elevated basal phosphorylation/activity of the signaling intermediates is also consistent with increased basal glucose transport in cultured muscle cells from insulin-resistant nondiabetic first-degree relatives of patients with type 2 diabetes (43).
The molecular mechanism for the observed increased basal tyrosine phosphorylation of IRS-1 in IGT relatives and patients with type 2 diabetes is elusive but may involve modulation at the level of the insulin receptor in response to high levels of insulin or glucose. Although the IGT relatives were not hyperglycemic, intermittent periods of postprandial hyperglycemia as a result of glucose intolerance may modulate insulin receptor and IRS-1 tyrosine phosphorylation in skeletal muscle. In various cultured cell systems, high extracellular glucose concentrations inhibit insulin action (46,47), presumably by inducing serine phosphorylation of the insulin receptor through a PKC-mediated mechanism (47). Glucose-induced serine phosphorylation of the insulin receptor is associated with decreased IRS-1 tyrosine-phosphorylation and attenuation of more distal signaling events, such as activation of PI 3-kinase (47) and Akt (47,48).
Hyperinsulinemia may be a likely candidate to account for increased basal signal transduction in skeletal muscle from the IGT relatives. The high basal IRS-1 tyrosine phosphorylation and PI 3-kinase activity in the IGT relatives may have prevented a further insulin-induced increase in signal transduction. Consistent with this, hyperinsulinemia may promote a constitutive activation of insulin signal transduction in skeletal muscle, which may induce a refractory state of the signaling intermediates when acutely stimulated by insulin during the in vivo experiments. This hypothetical phenomenon may underlie and be phenotypically recognized as insulin resistance in vivo. To test this possibility, we performed correlation analysis between basal insulin levels and basal IRS-1 tyrosine phosphorylation, PI 3-kinase activity, and Akt phosphorylation. The positive association noted between fasting plasma insulin and PI 3-kinase activity, as well as with Akt phosphorylation, for the entire study group, as well as in the control subjects, supports the hypothesis that hyperinsulinemia may partly account for the elevated signal transduction parameters in the IGT relatives in the "basal" state. However, the lack of a direct association between fasting plasma insulin levels and signal transduction parameters in the IGT relatives may to some extent challenge this hypothesis. Alternatively, other proximal, distal, or even parallel defects of insulin signal transduction parameters may play a greater role for the development of in vivo insulin resistance.
Insulin-stimulated serine phosphorylation of Akt was 55% lower in IGT relatives compared with control subjects; however, this difference was not statistically significant (P = 0.12). Nevertheless, the tendency toward decreased insulin-induced serine phosphorylation of Akt (insulin-stimulated minus basal) was consistent with our finding of decreased IRS-1 tyrosine phosphorylation and PI 3-kinase activity in the IGT relatives. Therefore, we cannot exclude that decreased insulin action on Akt as well as on IRS-1 and PI 3-kinase are all likely to represent physiologically relevant defects of some importance for insulin resistance in the IGT relatives. Because these signal transducers constitute early components of the insulin signaling cascade, these defects are likely to contribute to impaired glucose transport and glycogen synthase activation. However, given the relative impairment of these signal transduction parameters, our data suggest the presence of a more proximal postreceptor defect. Although the extent to which muscle insulin resistance in patients with overt type 2 diabetes may be explained by defects of insulin receptor binding or tyrosine kinase activity is controversial (17,18), the only available data in nondiabetic first-degree relatives of patients with type 2 diabetes demonstrates defects in muscle insulin receptor binding and IRTK activity (49).
In conclusion, we have demonstrated that a high physiological insulin infusion does not increase IRS-1 tyrosine phosphorylation and PI 3-kinase activity in skeletal muscle from glucose-intolerant first-degree relatives of patients with type 2 diabetes. This impaired insulin response may partly be explained by elevated basal activation states of these molecules. Thus, when phosphorylation/activity of these signaling intermediates are expressed as increment over basal, defective insulin action on IRS-1, PI 3-kinase, and Akt was noted in IGT relatives. Therefore, insulin signaling defects may partly contribute to impaired insulin action on glucose transport and glycogen synthesis in skeletal muscle in glucose-intolerant relatives of patients with type 2 diabetes, and these signaling defects are present before the development of overt diabetes. However, because the absolute magnitude of insulin action on signal transduction events was not decreased in IGT relatives, other signaling parameters or downstream defects (impaired glucose transport) may play a greater role in the development of skeletal muscle insulin resistance.
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ACKNOWLEDGMENTS |
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We thank all of the individuals who participated in the study for their cooperation and Susanne Reimer and Sussi Polmann, Hvidovre Hospital, for technical assistance.
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FOOTNOTES |
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Received for publication 2 November 2000 and accepted in revised form 5 September 2001.
H.S. and X.M.S. contributed equally to this study.
AUC, area under the curve; DTT, dithiothreitol; ECL, enhanced chemiluminescence; FFA, free fatty acid; FFM, fat-free body mass; IGT, impaired glucose tolerance; IGT relatives, glucose-intolerant first-degree relatives of type 2 diabetic patients; IRS, insulin receptor substrate; IRTK, insulin receptor tyrosine kinase; IVGTT, intravenous glucose tolerance test; HGP, hepatic glucose production; OGTT, oral glucose tolerance test; PI 3-kinase, phosphoinositide 3-kinase; PVDF, polyvinylidene difluoride; SA, specific activity; Rd, glucose disposal rate.
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REFERENCES |
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