1 Department of Endocrinology (M & C), University Hospital of Aarhus, and Department of Clinical Pharmacology, University of Aarhus, Aarhus, Denmark
2 Novo Nordisk A/S, Bagsværd, Denmark
3 Case Western Reserve University School of Medicine, Cleveland, Ohio
![]() |
ABSTRACT |
---|
![]() ![]() ![]() ![]() ![]() ![]() |
---|
Type 2 diabetes is characterized by insulin resistance and progressive islet cell dysfunction leading to insulin deficiency (1). Increased hepatic glucose release is considered to play a key role in fasting, as well as postprandial hyperglycemia, and increased gluconeogenesis seems to be essential in this scenario (2,3). In addition, elevated glucagon levels (4,5) and a reduced response of glucagon-like peptide 1 (GLP-1) to meals (6) are common features.
The importance of aggressive glucose-lowering therapy to prevent late diabetes complications in type 2 diabetes has been convincingly established (7,8). However, the U.K. Prospective Diabetes Study also demonstrated that the antidiabetic treatment used failed to maintain acceptable glycemic control in the vast majority of the patients, emphasizing the need for more effective antidiabetic agents.
GLP-1 is an incretin hormone secreted from the intestinal mucosa in response to meal ingestion (9). Insulin secretion is stimulated, and glucagon secretion is inhibited; both actions are glucose dependent. Also, GLP-1 has trophic effects on pancreatic ß-cells and inhibits their apoptosis (10). Furthermore, it delays gastric emptying (9,11) and may even be a satiety factor. These observations support GLP-1 as a novel candidate for treatment of type 2 diabetes, and the beneficial effects of GLP-1 on glycemic control in individuals with type 2 diabetes have been demonstrated (12,13). However, native GLP-1 has a very short half-life because of its rapid degradation by the ubiquitous enzyme dipeptidylpeptidase IV (DPP-IV) (14), making GLP-1 per se unsuitable as a therapeutic drug. Derivatives that are resistant to DPP-IV are one way to overcome this failing. Liraglutide is an acylated GLP-1 derivative that binds to albumin. This limits its sensitivity to DPP-IV and delays absorption from its injection site. A prolonged pharmacokinetic profile in humans is attained, the half-life after subcutaneous administration being 12 h (15,16). A single-dose study demonstrated significant glucose lowering in individuals with type 2 diabetes in both the fasting and postprandial states (16), and in a 12-week repeated-dose study, liraglutide lowered blood glucose to the same extent as a sulfonylurea compound (glimepiride) and the prevalence of hypoglycemia was very low (17).
The present study was undertaken to gain further insight into GLP-1 derivatives as novel antidiabetic drugs. We sought to do this by administering liraglutide to individuals with type 2 diabetes for 7 days and assessing the impact on 24-h glucose and hormone levels during daily life conditions, gastric emptying rate, endogenous glucose release (EGR), and various aspects of the pancreatic islet cell function.
![]() |
RESEARCH DESIGN AND METHODS |
---|
![]() ![]() ![]() ![]() ![]() ![]() |
---|
Patients.
Thirteen patients (5 women and 8 men) with type 2 diabetes according to World Health Organization criteria were examined. Their age (mean ± SD) was 56.4 ± 9.2 years, BMI was 31.2 ± 3.6 kg/m2, last measured HbA1c before inclusion was 7.3 ± 0.4% (normal range <6.4%), and the duration of diabetes was 3.0 ± 2.6 years (range 5 months to 8 years). At study entry, six patients were treated with diet alone and seven were additionally treated with oral hypoglycemic agents (OHAs; sulfonylurea n = 3, metformin n = 3, sulfonylurea and metformin n = 1). Concomitant medications were angiotensin-converting enzyme inhibitors (n = 4), thiazide diuretics (n = 1), ß-blockers (n = 1), calcium antagonists (n = 1), HMG-CoA reductase inhibitors (n = 2), and acetyl salicylic acid (n = 3). Three patients had retinopathia simplex, and three had nephropathy (microalbuminuria).
Experimental design.
This crossover trial was double-blinded, placebo-controlled, and randomized. After inclusion, the patients discontinued their OHA for 2 weeks before beginning study medication. Liraglutide (6 µg/kg body wt) or placebo was injected subcutaneously into the abdomen once daily (at 0745) for 9 days using a NovoPen (1.5 with Novofine 30-G, 0.3- to 8-mm needle) as the dispensing device. After 7 days of treatment, the patients arrived at the clinical research unit at 2200. In the next 2 days (days 8 and 9), the following experiments were carried out during continuous treatment.
On day 8 at 0730, a catheter was placed in an antecubital vein for blood sampling. Three standard meals were served at 0800, 1200, and 1800, to be finished within 20 min. Breakfast contained 2,660 kJ (protein 14 E%, carbohydrate 55 E%, and fat 31 E%), lunch contained 2,865 kJ (protein 16 E%, carbohydrate 50 E%, and fat 34 E%), and dinner contained 3,397 kJ (protein 28 E%, carbohydrate 53 E%, and fat 19 E%). With breakfast and dinner, 1 g of acetaminophen dissolved in 150 ml of water was given to assess gastric emptying rate (18). Serum acetaminophen was determined every 1530 min during the following 4 h, and area under the curve (AUC) for acetaminophen (AUCacetaminophen) and the time of occurrence for maximum drug concentration (tmax) were calculated. During day 8, blood was collected with changing intervals for determination of glucose, insulin, C-peptide, proinsulin (only fasting and after breakfast), glucagon, free fatty acids (FFAs), and liraglutide.
On day 9, the following procedures were performed (Fig. 1).
|
EGR.
EGR was estimated by use of an isotope dilution technique. At 0600, a bolus of 3-3H-glucose (adjusted priming: 6 µCi x plasma glucose level in mmol/l) was given followed by a continuous infusion (0.3 µCi/min) until 0900. Blood samples were drawn before the bolus and every 15 min from 0800 to 0900 for determination of glucose 3H specific activity. Steady state was achieved during this period in both situations, the average specific activity of glucose being 2,078, 2,180, and 2,160 cpm/mg at time points 0800, 0830, and 0900 during active treatment and 1,927, 1,822, and 1,906 cpm/mg at the same time points during placebo.
First-phase insulin secretion.
First-phase insulin secretion was determined using an intravenous glucose bolus. At 0915, 25 g of glucose was administered intravenously over 2 min. Blood was then collected every 25 min until 0932 for determining glucose and insulin.
Hyperglycemic clamp.
From 0932 to 1145, 20% glucose was infused to maintain plasma glucose at 16 mmol/l. After 75 min, when approximate steady state was attained, blood was drawn every 10 min (from 1045 to 1115) for determining plasma glucose and serum insulin, C-peptide, and proinsulin.
Arginine stimulation test.
At 1115, a bolus of 5 g of arginine was given intravenously over 30 s followed by collection of blood every 5 min until 1145 for determining circulating glucose, insulin, C-peptide, glucagon, and proinsulin.
Safety.
Adverse events, vital signs, hematology, and biochemistry were monitored throughout the study.
Assays.
All biochemical analyses were performed in duplicate. Plasma glucose was measured immediately on a glucose analyzer (Beckman Instruments, Palo Alto, CA) using the glucose oxidase technique. All other serum and plasma samples were stored at 20°C (C-peptide at 80°C) until analyzed. Serum insulin was determined using a highly specific and sensitive two-site enzyme-linked immunosorbent assay (ELISA; DAKO Diagnostics, Cambridgeshire, U.K.), and serum C-peptide was measured by a two-site monoclonal-based ELISA with an intra-assay coefficient of variation of 5.1% (DAKO Diagnostics). Serum proinsulin was analyzed by specific immunoassay with no cross-reaction with insulin and C-peptide (DAKO Diagnostics). Serum acetaminophen was determined by high-performance liquid chromatography after extraction. Plasma glucagon was measured using a radioimmunoassay kit (Linco Research). Liraglutide concentrations were analyzed by ELISA using a monoclonal antibody against GLP-1/liraglutide as capture antibody and another monoclonal antibody specific for the NH2-terminal part of GLP-1/liraglutide for detection. Before the latter analysis, samples were incubated at 37°C to remove endogenous GLP-1, liraglutide being stable toward this incubation. Determination of 3-3H-glucose activity was as previously described (19). Measurement of deuterium enrichment at carbons 2 and 5 glucose was as described by Landau et al. (20). In brief, 15 ml of blood was diluted with 30 ml of demineralized water and deproteinized using 15 ml of 0.3 N ZnSO4 and 15 ml of 0.3 N Ba(OH)2. The samples were then centrifuged at 2,000 rpm for 15 min, and the pellet was diluted in 15 ml of demineralized water to wash out the remaining glucose. Glucose was isolated by high-performance liquid chromatography. For determination of deuterium enrichment on C5, glucose was first converted to xylose, and the carbon 5 with its hydrogens was cleaved by periodate oxidation to formaldehyde, which was condensed with ammonium hydroxide to form hexamethylenetetramine (HMT). The 2H bound to C2 of glucose was isolated after conversion of glucose to ribitol-5-phosphate and arabitol-5-phosphate and treated to form HMT. Enrichments in the HMTs were measured using a Hewlett-Packard mass spectrometry system with standards of HMTs analyzed along with the unknown samples.
Calculations and statistics.
Fasting data are presented as the mean values at 0730 and 0800 on days 8 and 9. Furthermore, fasting plasma glucose on day 9 is presented. AUCs of substrates and hormones were calculated by applying the trapezoidal rule and represent the total AUC. EGR was determined using Steeles equations for steady state, as modified by Finegood et al. (21). The fractional contribution of GNG to glucose production equals the ratio between deuterium bound to carbon 5 in glucose and that bound to carbon 2. The rate of GNG in the fasting state was obtained by multiplying the mean EGR from 0800 to 0900 by the mean fractional contribution of GNG during that same hour. The rate of glycogenolysis (GLY) was calculated by subtracting the rate of GNG from total EGR. Insulin secretion rates (ISRs) were estimated by mathematical analysis (deconvolution) of peripheral C-peptide concentrations using a two-compartment model, as described by Polonsky et al. (22) and the standard C-peptide kinetic parameters published by Van Cauter et al. (23). This model allows accurate estimation of ISR also under nonsteady-state conditions. Another estimate of ß-cell function and an estimate of insulin resistance were calculated by homeostasis model assessment (HOMA-B and R) (24), using glucose and insulin values after a 14-h long fast and 24 h after the last liraglutide injection. As a supplement to the latter, insulin sensitivity was calculated by dividing glucose infusion rate during steady state of the hyperglycemic clamp with mean serum insulin level. Finally, an analog to the disposition index was calculated by multiplying 1/HOMA-R by the peak insulin concentrations during the first-phase insulin secretion test (25).
Statistical analysis was performed using a mixed model with sequence of treatment, visit, and treatment as fixed factors and patient as a random factor. Differences were considered significant at P < 0.05. All results are given as liraglutide versus placebo.
![]() |
RESULTS |
---|
![]() ![]() ![]() ![]() ![]() ![]() |
---|
|
|
Liraglutide exposure significantly reduced the 24-h AUC of glucagon (P = 0.04), primarily as a result of a marked reduction in glucagon concentrations after the protein-rich evening meal (P < 0.01). Fasting plasma glucagon concentrations were unaltered. The 24-h AUC insulin/glucagon ratio did not differ in the two situations (1.78 ± 0.28 pmol/µg vs. 1.72 ± 0.32 pmol/µg; P = 0.20). Fasting value and 24-h AUC of FFAs were similar in the two regimens.
Gastric emptying rate.
AUCacetaminophen during the breakfast meal (210 ± 16 vs. 210 ± 12 µmol · l1 · h) and AUCacetaminophen during dinner (178 ± 10 vs. 179 ± 9 µmol · l1 · h) were almost identical. Similarly, tmax did not show a significant difference after breakfast (40 ± 8 min during liraglutide treatment vs. 32 ± 4 min during placebo) or dinner (62 ± 10 vs. 50 ± 7 min).
EGR.
The rate of EGR in the fasting state was significantly reduced by liraglutide (1.92 ± 0.06 vs. 2.13 ± 0.09 mg · kg1 · min1; P = 0.04). This was due to diminished GLY (0.83 ± 0.04 vs. 1.02 ± 0.04 mg · kg1 · min1; P = 0.01). In contrast, GNG did not change (Fig. 3).
|
|
|
Pharmacokinetic properties.
The half-life of liraglutide in steady state was 17.9 h, and tmax was 10.1 ± 3 h (Fig. 5).
|
![]() |
DISCUSSION |
---|
![]() ![]() ![]() ![]() ![]() ![]() |
---|
Improved glycemic control during liraglutide treatment is probably orchestrated by changes in insulin and glucagon secretion. Basal and prandial ISRs were unchanged despite the substantial reduction in glycemia, clearly indicating improved ß-cell function during daily life conditions. This is in accordance with previous studies exploring native GLP-1 actions (12,13,27) and demonstrates that GLP-1 and/or GLP-1 derivatives augment the ability of the ß-cell to respond to prevailing prandial stimuli, e.g., glycemia and glucose dynamics.
A second important observation is that liraglutide significantly reduces 24-h circulating glucagon levels. In particular, the large postprandial glucagon excursion after the protein-rich evening meal was amply decreased. An impaired postprandial inhibition of glucagon is a common feature in type 2 diabetes (5,28), and this contributes notably to the postprandial hyperglycemia (4). Of particular note is that hyperglycemia per se inhibits glucagon secretion, and the decrement in plasma glucagon during liraglutide administration was seen despite a lower glycemic level.
The lowering effect of native GLP-1 on upper gastrointestinal motility is well established (29). In a single-dose study using liraglutide in patients with type 2 diabetes, reduced gastric emptying rate was also reported (16). In contrast, we did not in the current study observe delayed gastric emptying during liraglutide administration. The data achieved from the acetaminophen assessment technique has been proved to agree with data from using much more sophisticated methods for assessment of gastric emptying (30). A possible explanation behind the apparent discrepancy between the present and earlier data might be that the effect on upper gastrointestinal motility undergoes tachyphylaxis. However, two studies of liraglutide/native GLP-1 in animals (31) and humans (12) report an effect on gastric emptying after several weeks of treatment. Thus, it is conceivable that the lack of effect of liraglutide on gastric emptying observed in our study may be due to the dose used. Probably the dose-response relationships between blood glucoselowering effects and delaying gastric emptying differ, the latter being rightward shifted.
Another novel finding is the decline in fasting EGR after liraglutide administration. This could be due to an increased insulin/glucagon ratio. However, a significant increase was not observed in peripheral blood. It is essential to emphasize that circulating FFA levels did not differ in the two situations. In our diabetic individuals, fasting EGR was within what may be defined as the normal range. Presumably, a 10% reduction in fasting EGR (10 g glucose overnight) shall have an effect on fasting glycemic levels. It is also reasonable to assume that a much greater decrease in EGR will be present during daytime, taking into consideration the importance of dynamic changes in circulating glucagon on hepatic glucose handling in the prandial state (4,32,33).
Our interest was also in exploring the influence of liraglutide treatment on the contribution of GNG and GLY to EGR. The method allowed us to examine only fasting glucose kinetics. Several authors reported that the elevated EGR of individuals with type 2 diabetes is mainly attributable to an augmented GNG (2,3,34,35). The current study showed that the restraining effect of the GLP-1 derivative liraglutide on fasting EGR was solely due to inhibition of GLY, fasting GNG being unchanged. The opposite result might have been suspected, namely a reduction of GNG. However, studies, e.g., by Cherrington et al. (36), have demonstrated that the inhibitory effect of physiological insulin concentrations (in contrast to supraphysiological levels) on hepatic glucose production is primarily mediated through decreased GLY, whereas GNG is less sensitive to the direct action of insulin. Similarly, the stimulatory effect of glucagon on hepatic glucose release is primarily due to glycogen breakdown, whereas the hormone has less effect on GNG (36,37). Very high portal insulin levels are capable of suppressing hepatic GNG, but this may primarily be due to an indirect effect via decreased lipolysis and hence plasma FFA levels (36).
Again, although there was no significant change in the concentrations of fasting levels of insulin and glucagon, these were relatively augmented or decreased, respectively, considering the lowered level of glycemia. Furthermore, peripheral blood does not necessarily precisely reflect portal concentration. The effect of GLP-1/GLP-1 derivatives on GLY and GNG in patients with type 2 diabetes and more deranged glycemic control, i.e., with a substantial elevation of EGR, remains unknown.
Progressive impaired ß-cell function leading to insulin deficiency is a key feature of type 2 diabetes (1,38). Both a reduction in ß-cell mass and a functional abnormality of the islet cells seem to be responsible for the islet cells deterioration (39). It seems to be an ongoing process hardly influenced by concomitant glucose lowering treatment (38). Loss of first-phase insulin response to glucose is an early ß-cell defect, followed by a weakened basal and second-phase insulin output as the disease progresses (39,40). This, combined with an abnormal circadian glucagon secretory pattern (5,33) and diminished ability of hyperglycemia to suppress glucagon secretion, demonstrates the necessity for opposing both the - and ß-cell malfunction in the treatment of type 2 diabetes.
Improved ß-cell function in patients with type 2 diabetes has been reported after 612 h of GLP-1 infusion as assessed by first- and second-phase insulin response (41). A 6-week study demonstrated similar effects on ß-cell function, strongly indicating maintenance of this beneficial GLP-1 action (12). We found a dramatic improvement in ß-cell function after 8 days of liraglutide treatment. All ß-cell function tests were substantially ameliorated, indicating an effect on first- and second-phase insulin response to glucose as well as (near) maximal insulin secretory capacity. In addition, we found an almost 50% reduction of the proinsulin/insulin ratio in the circulation during both fasting and stimulation. The latter observation may indicate an improved processing of insulin in the ß-cell. In fact, in the current study, liraglutide treatment almost led to a normalized fasting proinsulin/insulin ratio. An elevated proinsulin/insulin ratio is a cardinal feature in type 2 diabetes and the pre-diabetic state (42,43) and is a well-established indicator of ß-cell dysfunction (44). Furthermore, liraglutide treatment led to an almost doubling of the disposition index, which reflects the ability of the ß-cells to adapt to the contemporary insulin resistance (glucose allostasis) (45), again emphasizing the powerful effects of GLP-1/GLP-1 derivatives on the ß-cell.
Another important impact of liraglutide on pancreatic glucoregulatory function was the significant inhibition of glucagon secretion during hyperglycemia and in particular during arginine infusion, demonstrating that liraglutide efficiently improves the secretory pattern of both - and ß-cells in the pancreatic islets of patients with type 2 diabetes, and it is anticipated that these beneficial actions will be maintained during long-term treatment. Very conceivable, the impact of GLP-1 derivatives on islet-cell function and consequently on glycemic control will further benefit from long-term treatment both directly via the GLP-1 trophic effects on the ß-cells and indirectly via decreased glucose toxicity.
The pharmacokinetic properties of liraglutide were evaluated by means of a 30-h plasma profile during steady state. The plasma half-life was 18 h, and tmax was
10 h postdosing. Medication was in this study given in the morning, resulting in the peak plasma concentration at
1800. Both the 24-h lasting beneficial effect on glycemia and the relatively high plasma concentrations maintained for 24 h clearly document that once-daily dosing is sufficient. Dosing at bedtime is another interesting option. Whether it is superior to morning dosing needs to be clarified.
In summary, we report that once-daily dosing with the GLP-1 derivative liraglutide for 1 week in individuals with type 2 diabetes results in 1) substantially decreased glucose concentration lasting 24 h and is ascribable to a relative increase in insulin secretion and decrease in glucagon concentration; 2) reduced EGR, as a result of diminished GLY; and 3) substantially improved AIR and maximal insulin secretory capacity. During longer lasting treatment, these promising antidiabetic effects may be further supplemented by an increase in ß-cell mass and the benefit achieved by weight loss.
![]() |
ACKNOWLEDGMENTS |
---|
Ms. Annette Mengel, Ms. Lene Ring, and Ms. Elsebeth Hornemann are thanked for outstanding technical assistance.
Address correspondencereprint requests to Ole Schmitz, MD, Department of Medicine M (Endocrinology & Diabetes), University Hospital of Aarhus, AKH, Nørrebrogade 42-44 DK-8000 Aarhus C, Denmark. E-mail: ole.schmitz{at}iekf.au.dk
Received for publication October 14, 2003 and accepted in revised form January 23, 2004
AUC, area under the curve; DPP-IV, dipeptidylpeptidase IV; EGR, endogenous glucose release; ELISA, enzyme-linked immunosorbent assay; FFA, free fatty acid; GLP-1, glucagon-like peptide 1; GLY, glycogenolysis; GNG, gluconeogenesis; HMT, hexamethylenetetramine; HOMA, homeostasis model assessment; ISR, insulin secretion rate; OHA, oral hypoglycemic agent; tmax, time of occurrence for maximum drug concentration
![]() |
REFERENCES |
---|
![]() ![]() ![]() ![]() ![]() ![]() |
---|