Department of Human Biology, Nutrition and Toxicology Research Institute Maastricht (NUTRIM), Maastricht University, Maastricht, the Netherlands
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ABSTRACT |
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INTRODUCTION |
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Elevated FFA concentrations may result from increased fasting rates of lipolysis, which seem to result from both the enlarged adipose tissue stores and an impaired insulin-mediated suppression of lipolysis (6). On the other hand, defects in FFA uptake and/or oxidation could also result in elevated circulating levels of FFA. Colberg et al. (7) reported that in viscerally obese women, there was a negative relation between visceral fat content and postabsorptive FFA utilization by skeletal muscle. Similar results were shown by Kelley and associates (8,9) using the leg-balance technique in combination with indirect calorimetry. They reported a diminished uptake of plasma FFA and a diminished oxidation rate of fatty acids in the postabsorptive state in patients with type 2 diabetes in comparison with lean healthy subjects. We have shown in obese type 2 diabetic patients that the uptake and oxidation of plasma FFA are diminished in the forearm muscles in the postabsorptive state and during ß-adrenergic stimulation (10). Type 2 diabetic subjects also had a diminished plasma FFA oxidation and a higher triglyceride-derived fatty acid oxidation at the whole-body level as compared with weight-matched control subjects during rest and moderate-intensity exercise (50% VO2max) (11).
Skeletal muscle is believed to be the main site responsible for the impaired fatty acid utilization and oxidation because of its large mass and since lipids are the principal oxidative substrate of skeletal muscle after an overnight fast and during moderate-intensity exercise. An imbalance between FFA uptake and FFA could easily lead to fat accumulation within skeletal muscle. Indeed, skeletal muscle triglyceride content is increased up to sixfold in patients with diabetes (12,13). Furthermore, the content of intramuscular triglycerides (IMTGs) shows a strong negative correlation with the degree of insulin resistance (i.e., insulin-stimulated glucose disposal) (14,15).
Thus, there is a lot of evidence indicating that disturbances in muscle fatty acid utilization may play an important role in the etiology of insulin resistance and type 2 diabetes. However, it is difficult to assess the pathophysiological abnormalities leading to type 2 diabetes when the type 2 diabetic state has already developed, since it is impossible to differentiate between primary factors and adaptational responses. Subjects with impaired glucose tolerance (IGT) have an elevated risk for the development of type 2 diabetes. Within 10 years, up to 50% of individuals with IGT become diabetic (16). If the disturbances in skeletal muscle fatty acid metabolism described above are already present in the glucose-intolerant state, this could indicate that the defects might be important etiological factors in the development of type 2 diabetes.
Therefore, the objective of this study was to investigate to what extent disturbances in fatty acid metabolism found in the diabetic state are already present in subjects at high risk for developing type 2 diabetes (i.e., IGT). We measured components of fatty acid metabolism with the use of stable isotope tracers in combination with indirect calorimetry in subjects with IGT and compared those values with previously published findings in type 2 diabetic subjects and obese subjects during postabsorptive conditions and during 60 min of moderate-intensity exercise (11).
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RESEARCH DESIGN AND METHODS |
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Body composition.
Body weight was determined on an electronic scale; body composition was determined by hydrostatic weighing with simultaneous lung volume measurement (Volugraph 2000; Mijnhardt, Bunnik, the Netherlands) and calculated according to the method of Siri (17). Waist and hip circumference measurements were made with subjects standing in the upright position to the nearest 1 cm, halfway between the spina iliaca and the last rib, and at the level of the trochanter major, respectively.
Study design.
Each subject participated in random order in two different trials, separated by at least 1 week. Subjects were asked not to participate in any exhausting physical activity during the 3 days immediately preceding the trials to exclude changes in substrate metabolism induced by the last bout of exercise. They also were asked not to consume any products of high natural 13C-abundance during the week immediately preceding both tests, as this might disturb the 13C/12C measurement in blood and expired air (18). In the palmitate test, total fat and carbohydrate oxidation as well as several parameters of fat metabolism were determined by means of the stable isotope technique with a [U-13C]palmitate tracer (Protocol 1) in the postabsorptive state while subjects were resting supine on a comfortable bed in a room kept at 2123°C, and during submaximal exercise (50% VO2max). During a separate test, the stable isotope tracer [1,2-13C]acetate was infused to determine the acetate recovery factor (ARF) necessary for correction of palmitate oxidation rates for loss of label in the tricarboxylic acid cycle and bicarbonate pool (protocol 2) (19).
Protocol 1.
Subjects reported to the laboratory at 8:00 A.M., arriving there by car or bus after a fast that started at 10:00 P.M. the day before. Two cannulas were inserted: one into a forearm vein for the infusion of palmitate, and the other in retrograde direction into a contralateral dorsal hand vein for blood sampling. The cannulated hand was placed in a hot box in which air was circulated at 60°C to arterialize the venous blood. Background blood and breath samples were taken 30 min after placement of the catheters. Then, at t = 0 min an intravenous dose of 0.085 mg/kg NaH13CO3 was given to prime the bicarbonate pool, followed by a constant-rate continuous infusion of [U-13C]palmitate (0.0067 µmol · kgbm-1 · min-1) via a calibrated infusion pump (IVAC560 pump; IVAC, San Diego, CA) until the end of the resting period (0120 min). During the last 20 min of the resting period (t = 100, 110, and 120 min), breath and blood samples were taken. Thereafter, exercise was started at 50% of the predetermined individual VO2max (45% Wmax) for 1 h (120180 min). The rate of infusion of [U-13C]palmitate was doubled at the start of exercise. During the last 20 min of exercise, blood and breath samples were taken (t = 160, 170, and 180 min). The palmitate tracer (potassium salt of [U-13C]palmitate, 99% enriched; Cambridge Isotope Laboratories, Andover, MA) was dissolved in heated sterile water and passed through a 0.2-µm filter into 5% warm human serum albumin (Central Blood Bank, Leiden, the Netherlands) to make a 0.65 mmol/l solution. The exact infusion rate of [U-13C]palmitate was determined for each experiment by measuring the concentration of the infusate.
Protocol 2.
During this trial, the same regimen as described for protocol 1 was followed, with the exception that in place of a [U-13C]palmitate tracer, a [1,2-13C]acetate tracer was infused. A priming dose of NaH13CO3 (0.085 mg/kg) was given, followed by a constant-rate continuous infusion of [1,2-13C]acetate at 0.046 µmol · kgbm-1· min-1 during rest (0120 min) and twice during exercise (120180 min), thereby giving the same 13C infusion rate as for palmitate. At the same time points as described in protocol 1, breath samples were obtained, and no blood samples were drawn. The acetate tracer (sodium salt of [1,2-13C]acetate, 99% enriched; Cambridge Isotope Laboratories) was dissolved in 0.9% saline and infused at the same 13C infusion rate per time unit as that for the palmitate tracer.
Breath, blood, and urine sampling.
Breath samples were obtained by having the subjects breathe normally for at least 3 min into a mouthpiece connected to a 6.75-liter mixing chamber and then collecting a breath sample into a 20-ml vacutainer tube (Becton Dickinson, Meyland Cedex, France) to determine the enrichment of CO2 (13C/12C ratio). VO2 and VCO2 were determined by means of open-circuit spirometry (Oxycon ß; Mijnhardt) during the resting period and the last 30 min of exercise. Arterialized blood samples were collected in EDTA-containing tubes on ice and were immediately centrifuged at 3,000 rpm at 4°C, and the plasma was put away in liquid nitrogen and stored at -80°C until analysis. Urine was collected overnight in containers with H2SO4 to determine nitrogen excretion for calculating the nonprotein respiratory exchange ratio.
Biochemical methods.
Breath samples were analyzed for 13C/12C ratio by injecting 20 µl of the gaseous head space into a gas chromatographisotope ratio mass spectrometer (GC-IRMS) (Finnigan MAT 252; Finnigan, Bremen, Germany). Total plasma FFA, glucose, and infusate acetate concentrations were measured using standard enzymatic techniques automated on the Cobas Fara centrifugal analyzer at 340 nm (for FFA: FFA-C test kit; Wako Chemicals, Neuss, Germany; for glucose: Roche Unikit III; Hoffman-LaRoche, Basel, Switzerland; for acetate: kit no. 148261; Boehringer Mannheim, Mannheim, Germany). For the determination of plasma palmitate concentration and enrichment, FFAs were extracted from plasma, isolated by thin-layer chromatography, and derivatized to their methyl esters. Palmitate concentrations were determined on an analytical gas chromatograph with ion-flame detection using heptadecanoic acid as an internal standard; on average, palmitate concentration was 25 ± 1% of total FFA concentration. Isotopic enrichment of palmitate was determined by GC-IRMS after online combustion of fatty acids to CO2 (Finnigan MAT 252), with correction for the extra methyl group in the derivate. The concentration of infusate palmitate was determined as described above for plasma samples.
Calculations.
The metabolic rate was calculated from VO2 and VCO2 according to the equation of Weir (20). Carbohydrate and fat oxidation rates were calculated from VO2, VCO2, and urinary nitrogen excretion (21). Protein oxidation (as calculated from nitrogen excretion) was assumed to be similar during the overnight-fasted state and during exercise.
Tracer calculations.
Total fatty acid oxidation was calculated by converting the rate of fat oxidation (triglyceride oxidation) to its molecular equivalent, with the assumption that the average molecular weight of triglyceride was 860 g/mol, and multiplying the molar rate of triglyceride oxidation by 3 because each molecule contains 3 mol/l of fatty acids.
Enrichment of breath CO2 and plasma palmitate and acetate is given as tracer-to-tracee ratio (TTR).
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Fractional recovery of label in breath CO2, derived from the infusion of labeled acetate, is calculated as follows:
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where F is the infusion rate of acetate (millimoles per minute) and the number 2 in the denominator is to correct for the number of 13C molecules in acetate. VCO2 is the expired CO2 (millimoles per minute).
During the last 20 min of the resting period (time points 110 and 120 min), a physiological and isotopic steady state was present; therefore, Steeles equation for steady state was applied to calculate the palmitate rate of appearance (Ra) or rate of disappearance (Rd).
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where F is the infusion rate of palmitate (micromoles per minute).
During the last 20 min of the exercise period (160170 and 170180 min), the single-pool nonsteady state equations of Steele adapted for use with stable isotopes were used to calculate Ra and Rd of palmitate.
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where F is the infusion rate (µmol · kg-1 · min-1); V is the volume of distribution, which was assumed to be 0.040 l/kg; C1 and C2 are the palmitate concentrations at times t1 and t2, respectively.
The Ra and Rd of FFA during rest and exercise, respectively, were calculated by dividing the palmitate flux and palmitate Ra and Rd by the fractional contribution of palmitate to the total FFA concentration.
The percent of infused [U-13C]palmitate oxidized was calculated with the following formula:
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where F is the infusion rate of palmitate (micromoles per minute) and the number 16 in the denominator is to correct for the number of 13C molecules in palmitate. VCO2 is the expired CO2 (micromoles per minute).
At the end, plasma FFA oxidation (micromoles per minute) was calculated as follows:
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The fatty acid oxidation from plasma triglycerides and IMTGs was calculated according to the following formula:
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Statistical analysis.
Data are presented as means ± SE. Oxidation rates and Ra and Rd are expressed as µmol · kg FFM-1 · min-1. Differences among groups were analyzed by a two-way analysis of variance. Changes in concentration of metabolites over time were analyzed with a repeated-measures analysis of variance. Statistical significance was set at P < 0.05. In case of significance, Scheffes post hoc test was performed.
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RESULTS |
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During the last 20 min of exercise, oxygen consumption reached a plateau (data not shown). No differences were observed in oxygen consumption among groups during exercise (1.55 ± 0.07, 1.36 ± 0.06, and 1.35 ± 0.11 l/min for obesity, IGT, and type 2 diabetes). During the last 20 min of exercise, mean relative workload was comparable (57.8 ± 3.6, 55.2 ± 2.1, and 54.9 ± 4.6% VO2max for obesity, IGT, and type 2 diabetes).
Arterialized concentrations of metabolites.
Plasma glucose levels were higher during rest in type 2 diabetic subjects than in obese and IGT subjects (P < 0.05). During exercise, blood glucose levels declined in type 2 diabetic subjects (P < 0.05) and remained stable in obese and IGT subjects; differences among groups in blood glucose concentration were no longer significant during exercise. Insulin levels were elevated in type 2 diabetic subjects at rest and during exercise (P < 0.05). Insulin levels declined as a result of the exercise (P < 0.01); the decline was not different among groups. Circulating levels of plasma FFA were not different among groups at rest, nor were they different during exercise (Table 2). Plasma FFA levels increased during the exercise period (P < 0.01) and kept increasing throughout the whole exercise period in all three groups to the same extent.
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Plasma palmitate 13C enrichment was slightly elevated in subjects with IGT compared with obese and type 2 diabetic subjects at rest (P < 0.05); however, during the exercise period, these differences were no longer significant. Acetate recovery gradually increased during both rest and exercise (Fig. 1). No differences were found in ARF among groups under resting conditions; during exercise, ARF tended to be higher in obese subjects compared with subjects with IGT and type 2 diabetes (P = 0.07) (Fig. 1).
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DISCUSSION |
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ARF and isotopic enrichment.
Oxidation rates of plasma fatty acid were determined with use of the stable isotope [U-13C]palmitate in combination with indirect calorimetry. To correct for the loss of 13C label due to fixation in products of the tricarboxylic acid cycle and the bicarbonate pool, Sidossis et al. (19) introduced the ARF. Failure to use the ARF may lead to a substantial underestimation of plasma FFA oxidation. A recent study pointed out that the ARF needs to be determined in every subject because of the large interindividual variation, especially during exercise (22). In the present study, the ARF tended to be lower in the glucose-intolerant and diabetic state during exercise compared with obese control subjects (P = 0.07). This is in agreement with previous studies showing a lower ARF in type 2 diabetic patients (11,22). The explanation for this is not fully understood, but it is suggested that an increased rate of gluconeogenesis in the IGT or diabetic state leads to additional loss of 13C label from the tricarboxylic acid cycle and thus a lower ARF. This study again stresses the importance of individual determination of the ARF to improve estimations of plasma substrate oxidation.
Subjects.
Obese, glucose-intolerant, and type 2 diabetic subjects were matched according to body composition and aerobic capacity. However, subjects with IGT were older than obese and type 2 diabetic subjects (58.3 ± 2.4 years for subjects with IGT vs. 45.1 ± 1.7 and 51.3 ± 3.4 years for obese and type 2 diabetic subjects, respectively; P < 0.01). Aging is associated with a diminished ability to use fat as a fuel during exercise (23,24); however, those observations were made comparing young adults (2033 years of age) with middle-aged (5055 years of age) or elderly (6679 years of age) subjects. Furthermore, disturbances in fat utilization in the elderly are partly related to a decline in physical activity observed with aging (24). In this study, no differences in aerobic capacity (VO2max) were present among the groups. Also, during the exercise period, no significant differences in absolute and relative workload, oxygen consumption, and energy expenditure existed. This finding seems to suggest that the muscle oxidative capacity (mitochondrial density) was matched, too. Thus, on the basis of the comparable VO2max and the relatively small age differences, it seems highly unlikely that this age difference has disturbed the results of the present study.
Fatty acid metabolism.
Total fat and carbohydrate oxidation were not different among the groups throughout the experiment. This result is in agreement with other studies showing that whole-body fat and carbohydrate oxidation were not different in diabetic subjects compared with obese and lean subjects during rest and exercise (25,26). As indicated above, plasma fatty acid uptake and oxidation are lowered, and triglyceride-derived fatty acid oxidation (IMTG or VLDL triglyceride oxidation) is elevated, in subjects with IGT and diabetes compared with obese control subjects. Thus, although whole-body fat oxidation is the same, there is a redistribution of the source of fatty acids oxidized. Skeletal muscle is by far the most important tissue responsible for uptake and oxidation of lipids, especially during exercise. Increased levels of muscle triglycerides, as reported in diabetic subjects (12,13) and most likely also in subjects with IGT, could lead to increased rates of triglyceride-derived fatty acid oxidation in muscle by a mass action effect, as utilization of muscle triglycerides during exercise is directly related to the content at rest in diabetic subjects (13). This would explain the higher rate of triglyceride-derived fatty acid oxidation in glucose-intolerant and diabetic subjects found in this study. It can be speculated that the tendency toward increased triglyceride-derived fatty acid oxidation may be one of the mechanisms linking increased IMTG content toward insulin resistance, as discussed in more detail below.
In the present study, Ra of plasma FFA was lower in subjects with IGT and type 2 diabetes than in weight-matched obese subjects. Type 2 diabetes is frequently accompanied by obesity, which makes it difficult to ascertain the impact of diabetes itself on lipolysis and FFA release. For that reason, diabetic subjects must be compared with body compositionmatched control subjects, as done in this study. Using microdialysis, Jansson et al. (27) concluded that adipose tissue lipolysis (expressed per unit of fat mass) was not different between well-controlled type 2 diabetic subjects and weight-matched control subjects. The lower Ra FFA found in the present study can most likely be explained by a difference in the fraction of FFA undergoing reesterification in adipose tissue and not by differences in adipose tissue lipolysis.
IGT is considered a prediabetic state, a necessary transition state en route to type 2 diabetes. Up to 15% of the people diagnosed with IGT develop diabetes each year (16). It would be of use if subjects at risk for progression to type 2 diabetes could be identified. Major risk factors for progression from IGT to type 2 diabetes are basal and 2-h glucose level, basal proinsulin level, age, and obesity (16). The results of the present study suggest that an impaired skeletal muscle fatty acid metabolism could be another important factor in the progression from IGT to type 2 diabetes. An increased level of physical activity in combination with a healthy diet and weight loss improved glucose tolerance in a Finnish study (28). One could speculate that changes in fatty acid metabolism as a consequence of the change in lifestyle partly explain the improved glucose tolerance.
Underlying mechanisms.
Several mechanisms may explain the observed impaired plasma FFA uptake and oxidation in subjects with IGT and type 2 diabetes. Throughout the experiment, the Ra and Rd of plasma FFA were lower in subjects with IGT and type 2 diabetes than in obese subjects (P < 0.05). This diminished Ra of plasma FFA could lead to a diminished uptake and subsequent oxidation of plasma FFA. The lower Ra of FFA may possibly be explained by an increased reesterification of fatty acid in adipose tissue or by differences in the regulation of lipolysis between obese subjects and obesity-associated type 2 diabetic subjects (26). However, the present study cannot be conclusive about this possibility. The fraction of the Rd oxidized was not different among groups, which means that once taken up, plasma FFAs are oxidized to the same extent in all groups, suggesting that the uptake of plasma FFA is more impaired than its oxidation.
A second factor that may play a role in the disturbed uptake and oxidation of plasma FFA is a lowered transport of FFA across the membrane. Alterations in content or expression of transport proteins could influence the capacity of the muscle to utilize lipids. In muscle biopsies from type 2 diabetic patients, the content of cytoplasmatic fatty acid binding protein was decreased as compared with control subjects, which could contribute to the decreased utilization and oxidation of plasma FFA (10). More studies, however, are needed to better understand the role and the importance of fatty acid transporters in the disturbances in muscle lipid metabolism as found in the diabetic state.
Thirdly, subjects with IGT may have increased stores of IMTG, as seen in diabetic subjects (12). Enlarged stores of triglycerides within the muscle in combination with an increased rate of lipolysis, as a result of a mass action effect, can flood the prediabetic muscle with FFA and lead to an increased concentration of FFA in the muscle cell. Indeed, we recently observed an increased release of glycerol from the forearm muscle of type 2 diabetic subjects, suggesting an increased lipolysis of IMTGs (10). Elevated levels of fatty acids within the cytosol of the muscle cell would diminish the blood tissue FFA concentration gradient, which is a very important determinant of plasma fatty acid uptake and oxidation and may explain the impaired uptake and oxidation of plasma fatty acid found in subjects with IGT and type 2 diabetes. This hypothesis is a very attractive one, because elevated levels of FFA in the cell could also interfere with insulin signaling and disturb insulin-stimulated glucose uptake (29). Interestingly, the tendency toward increased triglyceride-derived fatty acid oxidation found in this study may link increased IMTG content and utilization to decreased insulin-stimulated glucose uptake (insulin resistance). More studies, however, are needed to draw more definitive conclusions.
In conclusion, this study shows that the previously reported disturbances in fatty acid utilization in type 2 diabetes (8,11) are already present in a prediabetic state, i.e., in subjects with IGT. During rest and exercise, plasma FFA uptake and oxidation were diminished in subjects with IGT and type 2 diabetes, whereas triglyceride-derived fatty acid oxidation was increased during exercise in subjects with IGT and type 2 diabetes compared with obese subjects. An increased IMTG content, a diminished FFA transport capacity, or a decreased Ra of plasma FFA could be involved in the impaired plasma FFA uptake and oxidation. These data demonstrate that male subjects with milder forms of hyperglycemia (IGT) have the same defects in fatty acid utilization as subjects with type 2 diabetes, suggesting that these disturbances may play an important role in the progression from IGT to type 2 diabetes.
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ACKNOWLEDGMENTS |
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We thank Jos Stegen and Annemie Gijssen for their analytical support.
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FOOTNOTES |
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Received for publication 16 March 2001 and accepted in revised form 2 August 2001.
ARF, acetate recovery factor; FFA, free fatty acid; FFM, fat-free mass; GC-IRMS, gas chromatographisotope ratio mass spectrometer; IGT, impaired glucose tolerance; IMTG, intramuscular triglyceride; OGTT, oral glucose tolerance test; Ra, rate of appearance; Rd, rate of disappearance; TTR, tracer-to-tracee ratio; Wmax, maximal aerobic power output.
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REFERENCES |
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