Abstract
Aims/hypothesis
In rodent models of diabetes, treatment with sodium glucose co-transporter 2 (SGLT2) inhibitors improves beta cell function. This analysis assessed the effects of the SGLT2 inhibitor, canagliflozin, on model-based measures of beta cell function in patients with type 2 diabetes.
Methods
Data from three Phase 3 studies were analysed, in which: (Study 1) canagliflozin 100 and 300 mg were compared with placebo as monotherapy for 26 weeks; (Study 2) canagliflozin 100 and 300 mg were compared with placebo as add-on to metformin + sulfonylurea for 26 weeks; or (Study 3) canagliflozin 300 mg was compared with sitagliptin 100 mg as add-on to metformin + sulfonylurea for 52 weeks. In each study, a subset of patients was given mixed-meal tolerance tests at baseline and study endpoint, and model-based beta cell function parameters were calculated from plasma glucose and C-peptide.
Results
In Studies 1 and 2, both canagliflozin doses increased beta cell glucose sensitivity compared with placebo. Placebo-subtracted least squares mean (LSM) (SEM) changes were 23 (9) and 18 (9) pmol min−1 m−2 (mmol/l)−1 with canagliflozin 100 and 300 mg, respectively (p < 0.002, Study 1), and 16 (8) and 10 (9) pmol min−1 m−2 (mmol/l)−1 (p < 0.02, Study 2). In Study 3, beta cell glucose sensitivity was minimally affected, but the insulin secretion rate at 9 mmol/l glucose increased to similar degrees from baseline with canagliflozin and sitagliptin [LSM (SEM) changes 38 (8) and 28 (9) pmol min−1 m−2, respectively; p < 0.05 for both].
Conclusions/interpretation
Treatment with canagliflozin for 6 to 12 months improved model-based measures of beta cell function in three separate Phase 3 studies.
Trial registration: Clinicaltrials.gov NCT01081834 (Study 1); NCT01106625 (Study 2); NCT01137812 (Study 3)
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Introduction
Defects in beta cell function, including reduced insulin secretion and reduced efficiency of proinsulin conversion to insulin, are key pathophysiological factors underlying the hyperglycaemia of patients with type 2 diabetes mellitus [1, 2]. Declining beta cell function is a major contributing factor to the progressive nature of type 2 diabetes, with many patients eventually requiring insulin therapy to achieve and maintain glycaemic control [3, 4]. Glucose-lowering agents, which in addition to lowering plasma glucose levels, can improve beta cell function or slow the progression of beta cell dysfunction, may be useful for the long-term management of type 2 diabetes [1].
Pharmacological inhibition of the sodium glucose co-transporter 2 (SGLT2) is a novel approach to lowering plasma glucose in individuals with hyperglycaemia. SGLT2 inhibitors block renal glucose reabsorption and lower the renal threshold for glucose, thereby markedly increasing urinary glucose excretion (UGE) [5, 6]. Studies in animals have shown that beta cell function is restored when normoglycaemia is achieved by treatment with SGLT2 inhibitors [7–10]. The improvements in beta cell function observed in animal models are believed to be secondary to the improved glucose control, rather than due to direct effects of SGLT2 inhibitors on beta cells.
Canagliflozin is an SGLT2 inhibitor developed for the treatment of patients with type 2 diabetes [11–18]. In Phase 3 clinical studies, canagliflozin 100 and 300 mg provided significant improvements in glycaemic control in adult patients with type 2 diabetes, both as monotherapy and as add-on therapy to various background diabetes treatments [11–13, 15–17]. In addition, three clinical studies have evaluated the effects of canagliflozin treatment on measures of beta cell function in patients with type 2 diabetes. The first (Study 1) [16] was a study of canagliflozin 100 and 300 mg monotherapy compared with placebo at 26 weeks. The second (Study 2) [18] studied canagliflozin 100 and 300 mg as add-on therapy to metformin plus a sulfonylurea compared with placebo at 26 weeks; and the third (Study 3) [15] studied canagliflozin 300 mg as add-on therapy to metformin plus a sulfonylurea compared with sitagliptin 100 mg at 52 weeks. In these studies, canagliflozin treatment was generally associated with improvements in surrogate measures of beta cell function, including HOMA-2-derived beta cell function (HOMA2-%B), the proinsulin:C-peptide ratio and the C-peptide AUC:glucose AUC ratio. The current report presents further data from these three studies characterising the effects of canagliflozin treatment on additional indices of beta cell function obtained from the model-based analysis of plasma glucose and C-peptide responses to mixed-meal tolerance tests (MMTTs).
Methods
Patients and study design
Study 1 (canagliflozin monotherapy; ClinicalTrials.gov identifier NCT01081834) [16] and Study 2 (canagliflozin as add-on to metformin and sulfonylurea; ClinicalTrials.gov identifier NCT01106625) [18] were both randomised, double-blind, placebo-controlled, Phase 3 studies with a 26 week core treatment period followed by a 26 week extension period; findings on beta cell function from the core treatment periods are reported here. Study 3 (ClinicalTrials.gov identifier NCT01137812) [15] was a 52 week, randomised, double-blind, active-controlled, Phase 3 study comparing canagliflozin 300 mg with sitagliptin 100 mg as add-on therapy to metformin plus sulfonylurea. Details of study design, including patient inclusion and exclusion criteria, have been previously reported [15, 16, 18]. For all three studies, key aspects of study design, eligibility criteria and patient populations are summarised in Table 1.
These studies were conducted in accordance with the ethical principles detailed in the Declaration of Helsinki, and are consistent with good clinical practice and applicable regulatory requirements. Approval of the study protocols and amendments was obtained from institutional review boards and independent ethics committees of the participating centres. All patients provided informed written consent prior to participation.
Randomisation and study treatments
In Studies 1 and 2, patients were randomly assigned to receive daily oral doses of canagliflozin 100 or 300 mg or placebo (1:1:1); randomisation was stratified according to whether individuals had participated in the frequently sampled (FS)-MMTT (Studies 1 and 2), and whether they were taking glucose-lowering agents at screening (Study 1) or had begun a glucose-lowering agent adjustment period (Study 2). In Study 3, patients were randomly assigned to receive daily oral doses of canagliflozin 300 mg or sitagliptin 100 mg (1:1). Randomisation was stratified according to whether individuals had participated in the FS-MMTT and whether their pre-randomisation HbA1c value was ≥9.0% (75 mmol/mol).
In Studies 1 and 2, glycaemic rescue therapy with metformin (Study 1) or insulin (Study 2) was initiated at fasting plasma glucose (FPG) >15.0 mmol/l (270 mg/dl) from Day 1 to Week 6, >13.3 mmol/l (240 mg/dl) from Week 6 to Week 12 and >11.1 mmol/l (200 mg/dl) from Week 12 to Week 26. No glycaemic rescue therapy was provided in Study 3; patients meeting pre-specified glycaemic criteria (same as for Studies 1 and 2 through to Week 26, HbA1c >8.0% [64 mmol/mol] after Week 26) were discontinued.
Endpoints and assessments
A subset of patients from each study underwent an FS-MMTT on Day 1 and at Week 26 in Studies 1 and 2, and at Week 52 in Study 3. For the Day 1 test, patients took their first dose of study medication after blood samples for the MMTT were collected. For the FS-MMTT at Week 26 (Studies 1 and 2) or Week 52 (Study 3), the last dose of study medication was administered approximately 30 min before the start of the standard meal. Patients fasted for at least 8 h before the start of the FS-MMTT. The standardised meal was given between 07:00 and 10:00 hours, and consisted of two servings of liquid supplement containing approximately 100 g of total carbohydrates and approximately 2930 kJ (700 kcal). Water or non-caffeinated energy-free beverages could be consumed without restriction. The entire meal was to be completed within a 15 min period.
During the FS-MMTT, blood samples were collected for the measurement of glucose, insulin and C-peptide 15 min before and immediately prior to the start of the meal, and at 30, 60, 90, 120 and 180 min after the meal. Patients were asked to empty their bladders immediately prior to collection of the first blood sample. Urine was then collected over the interval from 15 min before the meal through to 180 min after the meal for the measurement of UGE. In Study 3, mean plasma glucose during the 3 h postprandial period (MPG0–3 h) was calculated as the AUC for the plasma glucose profile (calculated by the trapezoid rule) divided by the 3 h time interval.
Modelling analysis
Beta cell function was assessed from the FS-MMTT using a model that describes the relationship between insulin secretion and glucose concentration, and which has previously been described in detail [19, 20]. The model expresses insulin secretion (in pmol min−1 m−2) as the sum of two components. The first of these components consists of a dose–response function relating the insulin secretion rate and the absolute glucose concentration at any time point during the MMTT. Characteristic parameters of the dose–response function are the mean slope over the observed glucose range, denoted as beta cell glucose sensitivity, and the insulin secretion rate (ISR) at a fixed glucose level of 9 mmol/l (i.e. ISR at 9 mmol/l glucose). The dose–response function is modulated by a potentiation factor encompassing several potentiating mechanisms (e.g. prolonged exposure to hyperglycaemia, non-glucose substrates, gastrointestinal hormones and neural modulation), which is set to be a positive function of time and is constrained to average unity during the experiment. The second insulin secretion component, termed the derivative component, represents the dependence of insulin secretion on the rate of change of glucose concentration and is determined by a single parameter, denoted as rate sensitivity, that is related to early insulin release [21].
The model parameters were estimated from glucose and C-peptide concentrations by regularised least squares, as previously described [19]. The regularisation process involves a choice of smoothing factors. These were selected to obtain glucose and C-peptide model residuals with SDs close to the expected measurement error (∼1% for glucose, ∼4% for C-peptide). The ISR was calculated from the model every 5 min. The integral of insulin secretion during the 3 h MMTT was denoted as total insulin secretion, and insulin clearance was calculated by dividing total insulin secretion by plasma insulin AUC. Insulin clearance was calculated only for participants with at least five measurements of plasma insulin during the MMTT.
Insulin sensitivity was estimated from the MMTT data using the oral glucose insulin sensitivity (OGIS) index as previously described [22, 23]. However, because this index does not account for the insulin-independent glucose lowering occurring due to UGE in canagliflozin-treated participants, the OGIS index will tend to overestimate improvements in insulin sensitivity in canagliflozin-treated participants. To account for this, UGE-corrected OGIS values (OGISc) were calculated by subtracting renal glucose clearance (calculated as UGE divided by plasma glucose AUC during the MMTT) from the OGIS value to provide a more appropriate index of insulin sensitivity for assessing the effects of canagliflozin treatment.
Statistical analyses
Results for all model parameters are presented for all patients in the modified intent-to-treat (mITT) analysis set (i.e. all randomised patients who received ≥1 dose of study drug) with MMTT data at baseline and study endpoint. Statistical analyses for ISR at 9 mmol/l glucose, beta cell glucose sensitivity, OGIS, UGE, total insulin secretion and insulin clearance were performed using ANCOVA models, with the model parameter as the response variable, the baseline parameter value and baseline glycaemic control (binary value assessing whether baseline HbA1c was <9.0% [75 mmol/mol]) as covariates, and treatment as the experimental factor. The distribution of values for beta cell glucose sensitivity and the OGIS measures were better approximated by a log-normal than a normal distribution, so analyses of these parameters were performed using both original and log-transformed data; for clarity, the results (change in least squares mean [ΔLSM] and SEM) are presented in the original scale, but statistical significance testing was performed using the log-transformed values. The distribution of values for the rate sensitivity parameter was highly non-normal, so between-group comparisons were assessed using Kruskal–Wallis tests. In Study 3, similar ANCOVA models to those used for ISR at 9 mmol/l glucose were used for comparison of FPG, MPG0–3 h and peak postprandial plasma glucose concentrations. Differences between treatments were considered statistically significant at p < 0.05.
Results
Patient disposition and baseline characteristics
Baseline demographic and disease characteristics for patients in the FS-MMTT subpopulations are summarised in Table 2. The characteristics of these patients are similar to those observed in the overall population in each study [15, 16, 18]. The baseline relationship between ISR and plasma glucose in each of the three studies is shown in Fig. 1. Consistent with the well established progressive nature of beta cell failure in type 2 diabetes, baseline beta cell function was better in patients in Study 1 than in the patients with longer duration of diabetes evaluated in Studies 2 and 3; this is shown by the steeper slope for the relationship between ISR and plasma glucose in Study 1 compared with Studies 2 and 3. Within each study, baseline plasma glucose, insulin and C-peptide profiles, and the corresponding ISR–plasma glucose relationships at baseline were generally similar between the different treatment groups, with the exception of the placebo group in Study 1, which had modestly lower mean plasma glucose concentrations and modestly higher plasma C-peptide concentrations than the two canagliflozin groups, leading to a shift in the mean relationship between baseline ISR and plasma glucose concentration in the placebo compared with the canagliflozin groups (Figs 2, 3, 4).
Effects of canagliflozin treatment on HbA1c, body weight and waist circumference
As previously reported [15, 16, 18], in each of the three studies canagliflozin treatment reduced HbA1c, body weight and waist circumference. Greater reductions were observed for all three of these measures with canagliflozin treatment than with placebo (Studies 1 and 2) or sitagliptin (Study 3). The changes in these measures in the subset of patients with MMTT data (Table 3) were similar to the changes observed in the complete studies.
Effects of canagliflozin treatment on UGE, fasting and postprandial glucose, and insulin and C-peptide
In each of the three studies, canagliflozin treatment increased UGE (Table 4), resulting in reduced fasting and postprandial glucose concentrations (Figs 2, 3, 4). Despite the decreases in plasma glucose concentrations observed with canagliflozin treatment, C-peptide concentrations were generally similar at baseline and the study endpoint (Week 26 for Studies 1 and 2, Week 52 for Study 3) in canagliflozin-treated patients, whereas in the same patients plasma insulin concentrations tended to be modestly lower at the study endpoint relative to baseline (Figs 2, 3, 4). In the sitagliptin comparator study (Study 3), greater reductions in fasting and postprandial glucose were seen with canagliflozin 300 mg than with sitagliptin 100 mg (electronic supplementary material [ESM] Table 1).
Measures of beta cell function and insulin sensitivity
In Study 1, both doses of canagliflozin led to an upward shift in the relationship between ISR and plasma glucose, as well as an increased slope (Fig. 2j–l), whereas a slight downward shift was observed with placebo. The model-assessed parameters for ISR at 9 mmol/l glucose and beta cell glucose sensitivity were significantly increased with both doses of canagliflozin (Table 5). Changes in the rate sensitivity parameter varied considerably between patients, with no significant effect of canagliflozin compared with placebo. Total insulin secretion during the MMTT was not statistically significantly different between the canagliflozin and placebo groups. Insulin clearance was increased by approximately 15% with both doses of canagliflozin compared with placebo (ESM Table 2).
The effects of canagliflozin on beta cell function observed in Study 2 were generally similar to those seen in Study 1, with both doses of canagliflozin leading to an upward shift and steepening of the curve expressing the relationship between ISR and plasma glucose. No change was observed with placebo (Fig. 3j–l). In Study 2, the placebo-subtracted LSM increases in ISR at 9 mmol/l glucose and in beta cell glucose sensitivity were smaller than those observed in Study 1 (Table 5), with the former (ISR at 9 mmol/l) not quite achieving statistical significance (p = 0.10 for canagliflozin 100 mg, p = 0.07 for canagliflozin 300 mg). Insulin clearance was increased with both doses of canagliflozin compared with placebo, although the increase observed with the 100 mg dose did not reach statistical significance (p = 0.07) (ESM Table 2); the increase in insulin clearance observed with the 300 mg dose compared with placebo was approximately 24% (p < 0.0001).
In Study 3, treatment with sitagliptin 100 mg and canagliflozin 300 mg produced similar upward shifts in the relationship between ISR and plasma glucose (Fig. 4g, h). Increases from baseline in ISR at 9 mmol/l glucose were observed with sitagliptin (28 pmol min−1 m−2) and canagliflozin (38 pmol min−1 m−2; p < 0.05 vs baseline for both) (Table 5), with the increase observed with canagliflozin being similar to that observed in Study 2. However, the difference between canagliflozin and sitagliptin was not statistically significant (p = 0.4). Only minimal changes in beta cell glucose sensitivity were observed in either treatment group (1–2 pmol min−1 m−2 [mmol/l]−1) in this study, while no differences in rate sensitivity were observed between groups. Consistent with the greater reductions in plasma glucose concentrations in the canagliflozin group, total insulin secretion was reduced with canagliflozin treatment compared with sitagliptin (p = 0.005) (Table 5). Insulin clearance was increased by approximately 30% with canagliflozin 300 mg, whereas no change was observed with sitagliptin treatment (ESM Table 2).
Insulin sensitivity, as assessed by the UGE-corrected OGIS values, also improved with canagliflozin treatment (Table 5), with mean values of OGISc increasing by approximately 15% in canagliflozin-treated patients (although the differences were not significantly different from placebo in Study 2). As expected, the correction made to OGIS to account for UGE led to smaller increases in the index than those obtained using the uncorrected values.
Discussion
Progressive loss of beta cell function is a hallmark of type 2 diabetes and contributes to the progressive nature of the disease [1]. Several treatments for type 2 diabetes (e.g. sulfonylureas, meglitinides, glucagon-like peptide-1 [GLP-1] receptor agonists and dipeptidyl peptidase-4 [DPP-4] inhibitors) directly stimulate beta cells to increase insulin release. Using the same methods as in this paper, the DPP-4 inhibitors vildagliptin and sitagliptin [24, 25] and the GLP-1 receptor agonists liraglutide and exenatide [26, 27] have all been previously shown to improve indices of beta cell function.
SGLT2 inhibitors lower plasma glucose concentrations through a novel mechanism of action that does not directly affect insulin secretion or insulin sensitivity. SGLT2 inhibition reduces the renal threshold for glucose excretion, leading to increased UGE and thereby lowering plasma glucose concentrations [5, 6]. In several preclinical studies, the reversal of hyperglycaemia by treating hyperglycaemic rodents with SGLT2 inhibitors led to improved beta cell function and mass [7–10]. The present studies demonstrate that sustained treatment with the SGLT2 inhibitor canagliflozin for 6 to 12 months improved fasting and postprandial measures of beta cell function in humans. The plasma glucose and HbA1c reductions observed in the FS-MMTT patient subsets are consistent with the corresponding reductions observed in the overall populations of the three studies [15, 16, 18]. In Study 3, the improvements in beta cell function obtained from the FS-MMTT analysis were similar with canagliflozin and sitagliptin treatment, even though sitagliptin has direct effects on beta cells through the elevation of GLP-1 and glucose-dependent insulinotropic peptide, whereas canagliflozin is not believed to have any direct effects on beta cells. Although both treatments caused similar increases in ISR relative to glucose during the MMTT, the fasting proinsulin:C-peptide ratio was decreased with canagliflozin treatment compared with sitagliptin treatment [15], suggesting that the treatments have different effects on proinsulin processing [28]. The improvements in measures of beta cell function observed in canagliflozin-treated patients are believed to be secondary to improvements in plasma glucose control, rather than direct effects of canagliflozin, as no changes in measures of insulin secretion have been observed in normoglycaemic participants treated with canagliflozin. For example, no notable changes in 24 h plasma insulin profiles were observed in healthy participants treated with canagliflozin [29] and, in a separate study with an MMTT in healthy participants treated with canagliflozin 300 mg or placebo, no differences in the relationship between ISR and plasma glucose were observed between the canagliflozin and placebo treatment groups [5].
Canagliflozin treatment generally led to greater reductions in plasma insulin concentrations compared with C-peptide concentrations, suggesting that canagliflozin treatment altered insulin and/or C-peptide clearance, with the calculated increases in insulin clearance with canagliflozin treatment generally ranging from approximately 15% to 30%. The ISRs and the corresponding insulin clearance values calculated in this study were obtained using the assumption that canagliflozin treatment did not alter C-peptide kinetics. Because the kidney is the primary site of C-peptide clearance and canagliflozin acts directly on the kidney, a separate study was performed to assess whether canagliflozin treatment alters C-peptide clearance. This study showed that canagliflozin had only minimal effects on C-peptide clearance (<4%), confirming that the deconvolution procedure used to estimate ISR is appropriate in canagliflozin-treated patients [30]. Thus, it is likely that insulin clearance, which is known to be highly variable due to large and variable first-pass hepatic extraction [31], was increased with sustained canagliflozin treatment.
In conclusion, the results from three separate Phase 3 studies demonstrate that sustained treatment with canagliflozin for 6 to 12 months improves measures of beta cell function. It is now important to obtain data from longer term studies to assess whether treatment with canagliflozin can help slow the progressive decline of beta cell function over a longer period.
Abbreviations
- DPP-4:
-
Dipeptidyl peptidase-4
- FPG:
-
Fasting plasma glucose
- FS:
-
Frequently sampled
- GLP-1:
-
Glucagon-like peptide-1
- ISR:
-
Insulin secretion rate
- LSM:
-
Least squares mean
- mITT:
-
Modified intent-to-treat
- MMTT:
-
Mixed-meal tolerance test
- MPG0–3 h :
-
Mean plasma glucose during the 3 h postprandial period
- OGIS:
-
Oral glucose insulin sensitivity
- OGISc :
-
UGE-corrected OGIS values
- SGLT2:
-
Sodium glucose co-transporter 2
- UGE:
-
Urinary glucose excretion
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Acknowledgements
The authors thank all investigators, study teams and patients for their participation in these studies. Editorial support was provided by Cherie Koch of MedErgy and was funded by Janssen Global Services, LLC.
Canagliflozin was developed by Janssen Research & Development, LLC, in collaboration with Mitsubishi Tanabe Pharma Corporation.
The results from Study 1 were previously presented, in part, in abstract form at the 72nd Scientific Sessions of the American Diabetes Association (ADA), 8–12 June 2012, Philadelphia, PA. Results from Study 2 were previously presented, in part, in abstract form at the 48th Annual Meeting of the European Association for the Study of Diabetes (EASD), 1–5 October 2012, Berlin, Germany, and at the 48th Annual Meeting of the German Diabetes Association (DDG), 8–11 May 2013, Leipzig, Germany. Results from Study 3 were previously presented, in part, in abstract form at the 49th Annual Meeting of the EASD, 23–27 September 2013, Barcelona, Spain.
Funding
These studies were supported by Janssen Research & Development, LLC.
Duality of interest
AM has acted as a consultant for Boehringer Ingelheim Pharmaceuticals and Eli Lilly, and has received research support from Boehringer Ingelheim Pharmaceuticals. EF has been on advisory panels for AstraZeneca LP, Bristol–Myers Squibb, Boehringer Ingelheim Pharmaceuticals, Sanofi-Aventis, Johnson & Johnson, GlaxoSmithKline, Novartis Pharmaceuticals and Merck Sharp & Dohme, and has received research support from Boehringer Ingelheim Pharmaceuticals, Eli Lilly and Merck Sharp & Dohme. DP is a full-time employee of Janssen Research & Development, LLC.
Contribution statement
DP contributed to the design and conduct of the study, and the analysis and interpretation of the data. AM and EF contributed to the analysis and interpretation of the data. All authors contributed to the writing and reviewing of the manuscript and approved the final version of the manuscript. DP is responsible for the integrity of the work as a whole.
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Polidori, D., Mari, A. & Ferrannini, E. Canagliflozin, a sodium glucose co-transporter 2 inhibitor, improves model-based indices of beta cell function in patients with type 2 diabetes. Diabetologia 57, 891–901 (2014). https://doi.org/10.1007/s00125-014-3196-x
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DOI: https://doi.org/10.1007/s00125-014-3196-x