1Department of Medicine, Mount Sinai Hospital, 2Department of Physiology and 3Banting and Best Diabetes Centre, University of Toronto, Ontario, Canada M5G 1X5
Submitted 12 August 2002 ; accepted in final form 23 May 2003
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ABSTRACT |
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euglycemic clamp; insulin resistance; protein carbonyls; protein kinase C; antioxidants
Oxidative stress, which is present in diabetic subjects (6, 24, 82) and has been suggested to contribute to the complications of diabetes associated with chronic hyperglycemia (6, 24), has recently been suggested to induce insulin resistance (64, 66). There is evidence to support a link between elevated plasma glucose and oxidative stress. Experimental induction of hyperglycemia resulted in elevated markers of oxidative stress (16, 36). In type 2 diabetic subjects, plasma malondialdehyde and oxidized LDL were increased, whereas total plasma antioxidant capacity was decreased during postprandial hyperglycemia (16 mM for 2 h) after a carbohydrate meal (17, 18).
There is also evidence that oxidative stress can cause insulin resistance. Low levels of reactive oxygen species (ROS), such as hydrogen peroxide (H2O2), can be produced in the presence of hyperglycemia (28, 33, 37). In vitro studies using a variety of cell lines have demonstrated that micromolar concentrations of H2O2 can inhibit insulin signaling and glucose transport (10, 29, 76, 85). In human subjects, the efficacy of using antioxidant supplementation to improve insulin sensitivity remains unclear. Several studies of small numbers of diabetic subjects have shown that intravenous vitamin C (61), oral vitamin E (62, 63), or lipoic acid (34, 35) administration could improve insulin-mediated glucose utilization. However, in all these studies, the antioxidants were able to effect only a partial improvement of insulin sensitivity.
The etiology of the insulin resistance in type 2 diabetes is multifactorial. Thus, whether antioxidants improve insulin sensitivity by correcting the hyperglycemia-induced component of insulin resistance has not been addressed. Recently, the antioxidant N-acetylcysteine (NAC) has been shown to exert a protective effect on the -cell of diabetic db/db mice (40), Zucker diabetic fatty rats (81), and alloxan-induced diabetic CD1 mice (32). In these studies, NAC supplementation prevented hyperglycemia or improved glucose intolerance associated with the preservation of glucose-induced insulin secretion. Insulin sensitivity was measured in only one study, in the db/db mouse (40), and was assessed only with an insulin tolerance test, an insensitive method. The lack of effect of NAC on insulin resistance in the db/db mouse model of diabetes may be due to the complex etiology of the insulin resistance and associated abnormalities, e.g., leptin resistance and dyslipidemia (42).
The objective of this study was to ascertain whether oxidative stress participated in the pathogenesis of the insulin resistance induced by hyperglycemia in nondiabetic rats. To accomplish this, a previously established model of hyperglycemia-induced insulin resistance, namely, the rat infused with glucose for 6 h, was used (54). Insulin action was measured using the hyperinsulinemic-euglycemic glucose clamp technique, an established sensitive method to measure insulin sensitivity in vivo. Coinfusion of two different antioxidants, NAC and taurine, with glucose was tested to determine whether hyperglycemia-induced insulin resistance could be prevented. At the same time, soleus muscle protein carbonyl content and circulating levels of malondialdehyde and 4-hydroxynonenal, markers of oxidative stress, were measured in the absence and presence of high glucose with and without antioxidant coinfusion.
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MATERIALS AND METHODS |
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Surgery. Rats were anesthetized with ketamine HCl (85 mg/kg), xylazine (1 mg/kg), and acepromazine maleate (1 mg/kg). Indwelling catheters were inserted into the right internal jugular vein and left carotid artery, tunneled subcutaneously to the back of the neck, and exteriorized. Polyethylene catheters (PE-50; Cay Adams, Boston, MA) extended 0.5 cm with a segment of Silastic tubing (0.02 in. ID; Dow Corning, Midland, MI) were used for vascular catheterization. Catheters were filled with heparinized saline and flushed every second day to ensure patency. The jugular catheter was used for infusions and the carotid catheter was used for blood sampling. Rats were allowed to recover for 35 days before the experiment.
Preclamp infusions. All studies were performed in awake, unstressed rats fasted overnight. The animals were infused for 6 h with 1) saline (30 µl/min) (n = 5), 2) a variable infusion of 50% dextrose to maintain plasma glucose concentrations at 15 mM (n = 6), 3) 50% dextrose, as above, + NAC (0.35 mg · kg1 · min1; n = 5), or 4) saline + NAC (n = 5). NAC is often used for the treatment of acetaminophen overdose, and the standard dose used in those instances is not known to cause significant adverse effects (5, 70, 77). The rate of infusion of NAC in our experiment was just slightly higher than that used for the treatment of acetaminophen overdose in humans, although the total dose delivered over the 8-h experiment was approximately one-half. Because side effects of NAC are known to be dose dependent (5), and in preliminary studies identical results were obtained in the experiments to be described with or without an initial bolus dose, it was decided to forego the initial bolus dose (150 mg/kg). Blood samples were taken at 0, 2, 4, and 6 h for determination of plasma insulin and C-peptide levels.
A similar protocol was used in a second set of experiments, which tested the efficacy of the antioxidant taurine (2-amino ethanesulfonic acid) (1, 30). Taurine, similar to NAC, has been used intravenously in animal models to reduce lung injury (22), as well as in human subjects to decrease reperfusion lipid peroxidation-associated injury during myocardial revascularization (53). Thus rats were infused for 6 h with 1) saline, 2) glucose to maintain a concentration of 15 mM, as above, 3) 50% dextrose + taurine (0.35 mg · kg1 · min1; n = 5), and 4) saline + taurine (n = 6).
After the 6-h infusion period, a subset of animals that did not undergo the euglycemic clamp were used to obtain soleus muscle samples for analysis of oxidative protein damage and for evidence of translocation of PKC isoenzymes. Animals were placed under surgical anesthesia with a titrated dose of pentobarbital sodium. Soleus muscle was removed and flash-frozen with aluminum clamps cooled in liquid nitrogen. Muscle samples were stored at 70°C until further analysis.
Hyperinsulinemic euglycemic clamp. Insulin sensitivity was assessed using a 2-h hyperinsulinemic euglycemic clamp immediately after the 6-h infusion period during which infusion of NAC was continued. Regular porcine insulin (180 mU/kg bolus and 18 mU · kg1 · min1) was infused at 6 h (time 0) to maximally stimulate glucose uptake and to suppress endogenous glucose production. Clamp experiments were performed in combination with [3-3H]glucose infusion (40 µCi bolus and 0.4 µCi/min) for determination of glucose production. Blood samples (30 µl) were collected every 5 min during the 2-h clamp for the immediate determination of plasma glucose. A 50% dextrose solution was infused at a variable rate to maintain euglycemia. Additional blood samples (100 µl) were taken at 90, 100, 110, and 120 min for determination of [3H]glucose specific activity and at 60 and 120 min for plasma insulin levels. To avoid changes due to volume depletion, red blood cells were collected and reinfused in equal volumes of normal saline.
Assays. Plasma glucose was measured by the glucose oxidase method by use of a Beckman Glucose Analyzer II (Beckman Instruments, Fullerton, CA). Insulin was measured by radioimmunoassay with a kit (Linco) for rat insulin with 100% cross-reactivity with porcine insulin. Plasma [3-3H]glucose radioactivity was measured in duplicate after deproteinization using Ba(OH)2 and ZnSO4 and evaporation to dryness. An aliquot of the tracer infusate was also run with the plasma sample.
Determination of protein oxidation. Muscle tissue was homogenized at 4°C in buffer A (50 mM Tris, pH 7.5, 1 mM EDTA, 1 mM EGTA, 0.5 mM sodium orthovanadate, 0.1% 2-mercaptoethanol, 1% Triton X-100, 50 mM NaF, 5 mM sodium pyrophosphate, 10 mM sodium glycerophosphate, 0.1 mM PMSF, and 1 µg/ml each of aprotinin, pepstatin, and leupeptin), and cell debris was removed by centrifugation. Protein concentrations were determined using a standardized assay kit (Bio-Rad) with bovine serum albumin as the standard (14). Oxidative protein damage, assessed by the formation of carbonyl groups, was measured essentially as described by Levine et al. (46). One milligram of protein was precipitated by addition of 20% TCA and centrifuged (8,500 g) for 3 min, and the supernatant was discarded.
Protein pellets were washed with PBS (phosphate-buffered saline) and incubated with and without 2,4-dinitrophenylhydrazine (DNPH), 10 mM in 2 M HCl, and were allowed to stand at room temperature for 1 h, with vortexing every 15 min. After incubation, protein was reprecipitated using 20% TCA, and the pellet was obtained by centrifugation. The pellets were washed 3 times with ethanol-ethyl acetate (1:1) to remove free DNPH; the samples were allowed to stand for 10 min each time before the supernatant was discarded. The pellet was then dissolved in guanidine solution (6 M with 20 mM potassium phosphate, adjusted to pH 2.3 with trifluoroacetic acid) for 1 h at 37°C. Insoluble material was removed by centrifugation. Carbonyl content was calculated from the sample absorbance at 365 nm after subtraction of HCl-treated blanks by use of a molar absorption coefficient of 22,000 M/cm.
Malondialdehyde and 4-hydroxynonenal analysis. Samples were analyzed for malondialdehyde (MDA) and 4-hydroxynonenal (4-HNE) by a modification of a previously described method (49). Briefly, plasma aldehydes and 100 pmol of benzaldehyde-ring-D5 (internal standard) were derivatized by pentafluorobenzyl hydroxylamine hydrochloride (PFBHA · HCl) to form the aldehydes-PFBHA derivative. Plasma protein was precipitated by methanol, and aldehydes were separated by hexane extraction. The hydroxyl group of 4-HNE was further derivatized by 50 µl of N,O-bis(trimethylsilyl)-trifluoroacetamide (BSTFA) + 1% trimethylchlorosilane (TMCS) at 60°C for 15 min. Finally, 50 µl of hexane were added to each sample, and 1 µl was analyzed by gas chromatography-mass spectrometry (GC-MS).
The Hewlett-Packard 5973N MSD GC-MS was equiped with an HP-5 ms capillary column (30 m length, 0.25 mm ID, 0.25 µm film thickness), and the mass spectrometry was performed in negative-ion chemical ionization with methane as the reagent gas.
Determination of membrane PKC. Activation of PKCs is associated with translocation of the enzyme from the cytoplasm to cell membranes, and usually, but not always, with a corresponding decrease in cytosolic content of the enzyme (9, 44, 58). Therefore, activation of novel PKCs was assessed by quantification of the enzyme content in the membrane fractions of soleus muscle samples.
Samples were homogenized in 4 volumes of STE buffer [320 mM sucrose, 10 mM Tris · HCl (pH 7.4), 1 mM EGTA, 5 mM NaN3, 10 mM -mercaptoethanol, 40 µM leupeptin, 1 mM PMSF, 50 mM NaF, and 15 µg/ml aprotinin] and then centrifuged at 1,000 g for 10 min. The supernatant was then centrifuged at 100,000 g for 60 min. The pellet was resuspended in STE buffer containing 1% Triton X-100. Protein concentration was determined by the Lowry method, with bovine serum albumin as a standard.
The solubilized membrane fractions were added to 1 volume of 10% SDS, 13% glycerol, 300 mM Tris · HCl, 130 mM dithiothreitol, and 0.2% bromophenol blue (pH 6.8) and boiled for 5 min. Twenty micrograms of protein were separated by SDS-PAGE and transferred electrophoretically to a nitrocellulose membrane (Schleicher and Schuell). The membranes were blocked with 5% nonfat milk in TBST buffer [150 mM NaCl, 10 mM Tris · HCl (pH 7.4), and 0.1% Tween-20] for 1 h. Affinity-purified isoform-specific polyclonal anti-PKC antibodies (Sigma) were diluted 1:1,000 in the blocking buffer, and membranes were incubated for 12 h at 4°C. The membranes were washed and incubated with horseradish-peroxidase-linked goat anti-rabbit IgG (Amersham, Baie d'Urfe, QC, Canada), diluted in 5% nonfat milk, for 1 h at room temperature. Membranes were again washed and then detected by an enhanced chemiluminescence method (Zymed Laboratories, San Fransisco, CA) with exposure to Hyperfilm.
Insulin degradation. The reduced form of NAC contains an active sulfhydryl group that can bind to free S-H, forming a disulfide bond, or compete for and disrupt disulfide bonds, thus acting as a reducing agent (52). Because the structure of the intact insulin molecule is dependent on the presence of 3 disulfide bonds, the effect of NAC on immunoreactive insulin was determined. Insulin, 100 nmol, was added to DMEM in the presence of 010 mM NAC and incubated for 06 h at 37°C. Aliquots of medium were taken at 1-h intervals and frozen at 70°C, and insulin concentration was determined by RIA (Linco). For the in vivo infusion studies, 1 ml of whole blood was obtained from rats by following the protocols described above after 36 h of infusion with and without NAC (before the clamp). Insulin (100 nmol) was added to the blood samples, which were then incubated for 4 h at 37°C. Aliquots were taken at 0, 15, 30, 60, 120, and 240 min and centrifuged, and serum was frozen at 70°C for later determination of insulin by RIA, as described above.
Statistical analysis and calculations. Hepatic glucose production and glucose disappearance rates were calculated using steady-state equations (79). All values are expressed as means ± SE. Statistical significance was determined by analysis of variance (ANOVA) for repeated measurements followed by Tukey's t-tests. Differences were considered significant at P < 0.05.
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RESULTS |
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During the 6-h infusion period, plasma glucose was elevated to 15 mM in both the HG and HG + NAC groups (P < 0.001 vs. saline and NAC only groups), and there were no significant differences between these two groups (Fig. 1). Additionally, the total amount of glucose delivered during the infusion period to maintain the 15 mM concentration was essentially identical between the HG and HG + NAC groups (13,294 ± 935 and 13,277 ± 766 mg/kg, respectively).
Plasma insulin was measured every 2 h during the infusion period, and as expected, it remained constant in the saline and NAC only groups (119 ± 27 and 111 ± 18 pM). In response to the glucose infusion, plasma insulin levels were increased in the HG group (1,357 ± 188 pM; P < 0.001 vs. all other groups) and HG + NAC group (695 ± 106 pM; P < 0.001 vs. all other groups). There was a difference noted between the HG and HG + NAC groups for plasma insulin (P < 0.001; Fig. 2). C-peptide levels after 6 h of infusion were 226 ± 51, 2,550 ± 135, 1,670 ± 523, and 336 ± 163 pmol/l for the saline, HG, HG + NAC, and NAC only groups. C-peptide levels for the HG and HG + NAC groups were significantly greater than for control (P < 0.01) and different from each other (P < 0.05). Infusion of NAC alone did not alter C-peptide (P = NS).
During the hyperinsulinemic-euglycemic clamp, steady-state plasma glucose and insulin values were similar in all four groups (Figs. 1 and 2). Glucose infusion rate (GINF) for the HG group (31.1 ± 0.6 mg · kg1 · min1) was 20% lower than that of the saline group (37.8 ± 2.8 mg · kg1 · min1, P < 0.05). This decrease in GINF was completely prevented by coinfusion of NAC (41.8 ± 3.0 mg · kg1 · min1). GINF in the NAC only group (42.9 ± 4.5 mg · kg1 · min1) was not different from saline. The rate of disappearance (Rd) of glucose is equal to the GINF plus endogenous glucose production (EGP) and, during hyperinsulinemic clamp conditions, reflects primarily glucose utilization by muscle (19). Six hours of glucose infusion (HG) induced a significant decrease in Rd (32.4 ± 1.9 mg · kg1 · min1) compared with saline (41.2 ± 1.7 mg · kg1· min1) and NAC only (42.3 ± 3.8 mg · kg1 · min1; P < 0.05, HG vs. all other groups). Coinfusion of NAC with glucose completely prevented this decrease (45.9 ± 3.5 mg · kg1 · min1; Fig. 3). There were no significant differences in EGP (endogenous Ra) (mg · kg1 · min1: saline = 1.6 ± 0.8; HG = 0.6 ± 1.4; HG + NAC = 2.9 ± 0.6; NAC only = 2.2 ± 1.8, P = NS; Fig. 3B). EGP was almost completely suppressed in each group because of the high insulin levels present during the clamp.
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The efficacy of the antioxidant NAC to inhibit the hyperglycemia-induced insulin resistance suggested a potential role for oxidative stress in mediating the action of high glucose. To determine whether high glucose combined with the stimulated endogenous hyperinsulinemia caused oxidative stress in the major insulin target tissue, skeletal muscle, protein oxidation as assessed by DNPH binding to carbonyl groups in soleus muscle was measured. The presence of protein carbonyl groups has been demonstrated to reflect elevated levels of ROS (8, 71). Protein carbonyls were raised 5-fold (P < 0.001) after 6 h of glucose infusion compared with the saline-infused group. This increase was completely prevented by coinfusion of NAC in the HG + NAC group (Fig. 4).
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Although these data suggested an essential role for oxidative stress in hyperglycemia-induced insulin resistance, NAC may have had other actions. It is a known precursor of glutathione (GSH), and GSH may act as a cofactor in a number of enzyme reactions. Most relevant to hyperglycemia is the glyoxalase pathway, which is responsible for metabolism of reactive triose phosphate-derived 3-carbon intermediates such as methylglyoxal (6). Because methylglyoxal has been implicated in the formation of advanced glycation end products and diabetes complications (7, 84), the reduction of this dicarbonyl intermediate by NAC could not be excluded as an alternate possibility. We therefore utilized a second antioxidant, taurine, to determine whether hyperglycemia-induced insulin resistance was prevented. Taurine was chosen not only because it has been used as an antioxidant in a variety of settings (see review in Ref. 30), but also because, whereas NAC can be utilized to generate GSH as well as taurine, the reverse pathway, i.e., taurine to cysteine, does not occur. We found that coinfusion of taurine with glucose also prevented the HG-induced decrease in glucose infusion and glucose utilization rates (Table 1). It should be noted that fasting glucose and insulin concentrations in the HG + taurine and saline + taurine groups were comparable to those of all other groups (not shown). In addition, the plasma insulin values during the 6-h infusion of HG + taurine (1,014 ± 14 pmol/l) and C-peptide (3,171 ± 314 pmol/l) were not different from those during HG, and values for taurine alone (insulin, 107 ± 13 pmol/l; C-peptide, 349 ± 56 pmol/l) were similar to saline and NAC. Finally, the total amount of glucose infused in the HG + taurine group (13,952 ± 1,092 mg/kg) was similar to HG and HG + NAC (see above).
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To determine that HG infusion did promote oxidative stress and that taurine infusion, under these conditions, acted as an antioxidant, the lipid oxidative stress markers MDA and 4-HNE (28, 49) were assayed. Both were significantly elevated by 6 h of HG infusion and were normalized (MDA) or markedly reduced (4-HNE) by coinfusion of taurine (Table 2).
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Exposure to high glucose has been found to elevate diacylglycerol (DAG) and activate one or more DAG-sensitive isoforms of PKC (44). Furthermore, activation of PKCs by phorbol myristate acetate, or PMA, has been associated with insulin resistance (9, 12, 41, 55, 68). In a previous study, infusion of glucose for 24 h resulted in translocation of the novel PKC-
(45) and, similarly, infusions of Intralipid/heparin to raise free fatty acid concentrations caused translocation of the novel PKC-
isoform (26). Thus translocation of novel PKC isozymes to cell membranes was assessed in soleus muscle after6hof glucose infusion. There were no significant differences noted between groups for translocation of the novel PKC isoforms-
, -
, or -
(Table 3).
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We previously found that high concentrations of NAC, 25 mM, prevented high glucose and insulin-induced insulin resistance in primary cultures of rat adipocytes (19). We subsequently determined that this was associated with the disappearance of immunoreactive insulin in the medium, likely due to the reduction of the inter- and/or intrachain disulfide bonds. This observation has also been recently reported by Greene et al. (25). The decrease in circulating insulin concentration during the first 6 h of infusion in the HG + NAC group compared with the HG group (Fig. 2) could have been due either to a decrease in insulin secretion, suggested by the C-peptide measurements, or to insulin degradation. To determine the effect of NAC on immunoreactive insulin, 100 nM insulin was incubated in the presence and absence of NAC in tissue culture medium, as well as in the serum of the rats infused with and without NAC. As depicted in Fig. 5A, there was a small effect of 1 mM NAC in vitro after 2 h to decrease immunoreactive insulin compared with incubation in medium without NAC. However, exposure of insulin to 5 mM NAC resulted in a rapid and marked reduction in insulin by 80% within 1 h. In contrast, addition of an equivalent amount of insulin (100 nM) to blood samples obtained from control or NAC-infused rats after 36 h (before the clamp) showed no effect of NAC to decrease immunoreactive insulin (Fig. 5B). In fact, there was a tendency to detect a greater amount of residual insulin after 14 h of incubation at 37°Cinthe presence of NAC, but it was not statistically significant.
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DISCUSSION |
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The mechanism by which hyperglycemia causes insulin resistance is not completely understood. Exposure to an elevated glucose concentration of a number of tissues that take up glucose independently of insulin has been shown to result in increased cellular glucose entry and metabolism (15, 44, 80) and to be associated with oxidative stress (6, 15, 16, 28, 33). The latter has been documented by measurement of ROS, e.g., H2O2 (33, 37), intracellular concentrations of GSH (reduced glutathione), levels of antioxidant enzymes (glutathione peroxidase, glutathione reductase, and superoxide dismutase), and resultant oxidative changes to protein, lipid, and DNA (6, 36, 66, 82). There is likely more than one mechanism by which increased glucose generates ROS. Although glucose autoxidation has been well documented and in the presence of redox cycling metal ions (Fe2+/3+, Cu1+/2+) can cause protein oxidation, this requires long-term exposure to high glucose. On the other hand, glucose metabolism results in the formation of reactive 3-carbon metabolites such as glyoxal and methylglyoxal, which, by more rapid nonenzymatic protein glycation, may generate ROS and protein carbonyls (6, 33, 37, 84). Another source of ROS may be the mitochondria. In endothelial cells, exposure to high glucose was found to cause elevated ROS, which was inhibited by blocking mitochondrial complex III and IV of the electron transport chain (15). It was postulated that the oxidative stress generated was reflected in the cytosol and inhibited glyceraldehyde-3-phosphate dehydrogenase. In the present study, evidence of oxidative stress after 6 h of hyperglycemia was observed in skeletal muscle, an insulin target tissue, manifested by a markedly increased level of protein carbonyls. Furthermore, this was inhibited by coinfusion of the antioxidant NAC. There was also evidence of lipid peroxidation induced by the HG infusion, manifested by significantly elevated circulating levels of MDA and the more specific 4-HNE, which was inhibited by the antioxidant taurine. Importantly, the coinfusion of NAC or taurine with HG also inhibited the insulin resistance. Consistent with these observations, we have recently found that exposure of rat adipocytes in primary culture to high levels of glucose combined with insulin resulted in the increased generation of ROS, which was prevented by preincubation with NAC (48). These data suggest, but do not prove, that oxidative stress caused, or at least contributed to, the insulin resistance induced by high glucose.
There is previously published evidence suggesting that oxidative stress may play such a role. First, direct exposure of cultured cells, 3T3-L1 adipocytes, and L6 muscle cells to H2O2 has been reported to cause insulin resistance (10, 29, 76, 85). In addition, several in vivo studies have reported a partial improvement of insulin resistance in subjects with type 2 diabetes mellitus by oral administration of vitamin E (63), intravenous administration of vitamin C (61), or intravenous GSH (65). These were all small studies; clearly, further work is required to firmly establish this relationship in both rodent models and human subjects.
The mechanism by which oxidative stress may contribute to insulin resistance is not clear. Exposure of cells to H2O2 will activate numerous signaling systems, including PKC (43), MAPK family enzymes (10, 27), and the small G protein Ras (60, 69). Of these, the PKCs have been previously implicated as mediators of insulin resistance (9, 12, 41, 68). However, we were not able to demonstrate membrane translocation of any novel PKC isoforms in the muscle tissue from the insulin-resistant rats. This may be due to the short duration of hyperglycemia, as some studies using longer (2496 h) glucose infusion in normal rats (45) and studies of chronic hyperglycemia in diabetic rats (3) reported translocation of PKC- and of PKC-
, -
, -
, and -
, respectively, in soleus muscle. Although the lack of membrane translocation suggests that PKC is not involved in this short-term model, this possibility cannot be entirely dismissed, as translocation of conventional PKC isoforms was not evaluated and PKC activation in the absence of translocation has been reported (58).
The mechanism by which NAC inhibits the induction of insulin resistance appears to be its antioxidant properties (2, 20). However, NAC provides cysteine for and promotes the synthesis of GSH (20). GSH has been found to have cellular functions unrelated to its antioxidant activity, such as serving as a cofactor in the glyoxalase-catalyzed metabolism of methylglyoxal (6). However, the finding that taurine, which cannot be converted to cysteine and GSH, was also effective supports an antioxidant mechanism. The end product of the glyoxalase pathway is D-lactate (6, 7). In preliminary studies, measurements of circulating D-lactate in the control and HG- and HG + taurine-infused groups at the end of 6 h were all undetectable (<0.3 mM). Of interest, NAC has also been found to protect -cells in culture and in vivo from "glucose toxicity," preserving insulin synthesis and secretion (40, 81). Oxidative stress may thus play a role in the dual abnormalities of insulin action and insulin secretion found in type 2 diabetes mellitus.
Finally, we noted a somewhat decreased insulin concentration in the rats infused with glucose combined with NAC compared with those receiving glucose alone. Because a previous report demonstrated that high concentrations of a -SH group containing antioxidants such as NAC and lipoic acid could decrease immunoreactive insulin (25), presumably by disrupting disulfide bonds, we determined whether this might have occurred during the infusions of NAC. In contrast to in vitro results, which showed a rapid and significant effect of >1 mM NAC on insulin concentrations, there was no effect of the NAC present in the circulation of the infused rats (Fig. 5). This was consistent with a much lower estimated concentration of NAC achieved with this infusion protocol. On the basis of clearance values determined in humans (0.11 to 0.207 l · h1 · kg1), and with the assumption that clearance rates in rats would be similar or even higher, the maximum concentration at steady state during our infusions was estimated to range between 0.66 and 1.25 mM (13, 20, 59). Furthermore, in contrast to insulin, NAC in vitro did not decrease immunoreactive C-peptide (data not shown). Taken together, the data suggest that the lower insulin concentration in the presence of NAC reflects the state of increased insulin sensitivity observed in this group.
In summary, this study demonstrates that NAC and taurine prevent short-term hyperglycemia-induced insulin resistance in vivo. This model of insulin resistance is associated with increased oxidative stress, which is concomitantly inhibited by both antioxidants. The data support the hypothesis that oxidative stress contributes to the pathogenesis of insulin resistance.
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DISCLOSURES |
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ACKNOWLEDGMENTS |
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FOOTNOTES |
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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.
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REFERENCES |
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