Abstract
Aims/hypothesis
Vitamin D is necessary for normal insulin action and suppresses renin production. Increased renin–angiotensin system (RAS) activity causes islet damage, including reduced insulin secretion. We therefore sought to determine whether hypovitaminosis D-induced upregulation of islet RAS in vivo impairs islet cell function and increases insulin resistance, and whether pharmacological suppression of the RAS during continuing vitamin D deficiency might correct this.
Methods
C57BL/6 mice were rendered vitamin D-deficient by diet, and glucose and insulin tolerance was assessed. The expression and translation of islet functional, and islet RAS, genes were measured and the effects of pharmacological renin suppression examined.
Results
Mice with diet-induced hypovitaminosis D developed impaired glucose tolerance, increased RAS component expression and impaired islet function gene transcription. Treatment with pharmacological renin inhibition (aliskiren), without vitamin D status correction, reduced islet RAS over-reactivity, islet dysfunction and insulin resistance, and improved glucose tolerance.
Conclusions/interpretation
Upregulation of islet RAS genes can contribute to hypovitaminosis D-induced impairment of islet function and increase insulin resistance independently of vitamin D status. Thus, our findings support the use of RAS inhibitors in impaired glucose homeostasis or early diabetes. They also suggest that combining RAS inhibition with correction of hypovitaminosis D might be useful in treating impaired glycaemic control and also in type 2 diabetes prevention. However, the use of aliskiren in established diabetes is contraindicated due to the increased risk of side effects such as hyperkalaemia, so other more suitable RAS blockers need to be identified.
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Introduction
Accumulating evidence has demonstrated many functions of vitamin D beyond its classical roles in calcium homeostasis and bone health. Experimental and clinical studies have implicated poor vitamin D repletion as a risk factor for numerous diseases, including metabolic syndrome [1]. Low serum 25-hydroxyvitamin D (25[OH]D3) concentrations lead to defective insulin secretion, reduced glucose homeostasis, and increased risk of metabolic syndrome and type 2 diabetes, both experimentally and in cross-sectional studies in humans [2, 3]. These risks reflect increases in insulin resistance as well as islet beta cell dysfunction [4]. Higher baseline vitamin D status can predict better islet function, better glucose tolerance and reduced risk of hyperglycaemia prospectively [5]. However, observations from clinical studies remain inconclusive with regard to the causality of associations between vitamin D status and diabetes risk, as both conditions are associated with factors such as obesity and sodium intake, and there is also variation between studies [6]. Vitamin D supplementation can reduce insulin resistance in human deficiency [1], but it is not clear whether it can reduce insulin resistance or improve islet function in established diabetes; thus, further investigation of the underlying mechanisms is warranted.
VDR polymorphisms are common and contribute to the modulation of serum 25(OH)D3 concentrations and to the determination of some relevant aspects of vitamin D function affecting the renin–angiotensin system (RAS) in humans [7]; moreover, in some human studies, polymorphism, gene expression and formation of the VDR were associated with variation in insulin secretion [8]. Vitamin D status is also associated directly with insulin secretion in murine islets [9], and mice with mutant Vdr have impaired insulin gene expression and secretion [10]. However, it remains uncertain whether there are mechanisms by which vitamin D affects islet function and insulin sensitivity, other than through direct effects on calcium metabolism [11].
Many clinical studies suggest that treatment with RAS blockade is associated with a reduced type 2 diabetes risk and fewer diabetic complications [12]. Our previous work has demonstrated: (1) the existence of a local pancreatic islet RAS [13]; (2) that islet function is improved in mouse models of diabetes by angiotensin II type 1 (AT1) receptors antagonism [14, 15]; and (3) that local islet RAS can regulate islet cell proliferation and apoptosis, while modulating oxidative stress and beta cell mass [14, 16]. Moreover, clinical and basic studies implicate additional factors regulated by or affecting, directly or indirectly, the islet RAS [14, 17]. Overall, suppression of islet RAS presents a potential target for the reduction of type 2 diabetes risk and, potentially, for the protection of islet function in type 2 diabetes.
The RAS is recognised to be a major blood pressure regulation system, and associations between hypertension and vitamin D deficiency have been suggested by several clinical studies [18]. The rate-limiting RAS component, renin, was shown to be suppressed by vitamin D in a study on Vdr-knockout (KO) mice, which develop elevated renin expression [19]. Mice without the vitamin D-activating 1α-hydroxylase develop hyperreninaemia, independently of calcium levels [20]. The administration of calcitriol (1,25[OH]2D3), the active hormonal metabolite of vitamin D, or its analogues, reduces plasma renin activity and angiotensin II levels in experiments and in humans [21, 22]. Vitamin D status has shown inverse relationships with plasma renin activity in humans [23, 24], while activated vitamin D and AT1 receptor antagonism have synergistic beneficial effects on RAS regulation and on outcomes in diabetic nephropathy [25].
Since pancreatic islet RAS components are involved in the regulation of whole-body glycaemic control, vitamin D availability can be expected to contribute to modulation of this process. Recently, we found that in isolated islets 1,25(OH)2D3 provided potential protection against and ameliorated RAS component overabundance induced by hyperglycaemic conditions, as well as increasing insulin synthesis and secretion as expected [26]. However, it remains to be determined whether islet RAS mediates the effects of vitamin D deficiency on glycaemic control in vivo.
The present study is therefore based on the hypothesis that vitamin D deficiency may lead to increased islet RAS activity in vivo, contributing to abnormal glucose homeostasis. To test this hypothesis, we examined glucose tolerance, insulin sensitivity, islet architecture and RAS component activity, islet insulin secretion and related gene activity in genetically normal mice with diet-induced vitamin D deficiency, with and without pharmaceutical RAS inhibition. Our aim was to determine whether RAS blockade can reduce hypovitaminosis D-induced disorders of glucose homeostasis in animals with untreated vitamin D deficiency.
Methods
Animals
Vitamin D deficiency was induced by feeding 4-week-old male C57BL/6 mice with a vitamin D-deficient diet (TD89123; Harlan Teklad, Madison, WI, USA) for 8 weeks and control groups with a normal, vitamin D-containing diet (TD89124; Harlan Teklad). Mice were housed under ultraviolet B-free incandescent light to minimise endogenous vitamin D production. Blood glucose and body weight were recorded regularly. Mice were killed for further study when aged 12 weeks. The animal studies were approved by the Laboratory Animal Services Center of the Chinese University of Hong Kong (Ref No. 08/049/ERG).
Measurement of serum 25(OH)D 3 and 1,25(OH) 2 D 3 concentrations
Retro-orbital blood samples were collected from mice, centrifuged at 1,000 g for 10 min and serum aliquots stored at −80°C until assay for 25(OH)D3 and 1,25(OH)2D3 using IDS-EIA kits (Immunodiagnostics-Systems, Boldon, UK) according to the manufacturer’s protocol (CV < 10%).
Treatment with a renin inhibitor
Aliskiren (CGP060536) was provided by Novartis Pharma, Basel, Switzerland. After 8 weeks of vitamin D-deficient diet treatment, 12-week-old mice that had been fasted for 6 h and had fasting blood glucose > 9 mmol/l were treated for 7 days with aliskiren (30 mg kg−1 day−1) by daily gavage. Pancreatic islets were then isolated for further study.
Isolation of pancreatic islets
Pancreatic islets were isolated as described previously in our laboratory [26]. Briefly, pancreatic islets were isolated from the pancreases from the different groups of mice by intra-ductal injection with 0.3 mg/ml collagenase-P (Roche Diagnostics, Mannheim, Germany) in Hanks’-balanced-salt-solution (Sigma-Aldrich, St Louis, MO, USA). After washing and gradient centrifugation (500 g), isolated islets were hand-picked under a stereomicroscope.
Pancreatic islet staining
Immunohistochemistry was used for morphological assessments, and to locate pancreatic islet proteins and gene expression [14, 26]. Briefly, air-dried cryo-sections were rinsed with PBS, followed by 1 h of blocking using 6% (wt/vol.) normal donkey serum (Jackson-ImmunoResearch, West-Grove, PA, USA). Primary antibodies against insulin (Invitrogen Life Technologies, Carlsbad, CA, USA) and/or glucagon (Abcam, Cambridge, MA, USA) and/or Ki67 (Abcam) were added and incubated on the slides overnight at 4°C. After three washes with PBS, appropriate fluorescent-conjugated secondary antibodies were added to the slides, which were then incubated at room temperature for 1 h. After counterstaining with DAPI, slides were washed three times with PBS and mounted using a medium (VectaShield; Vector-Laboratories, Burlingame, CA, USA). Signals were then detected by fluorescent microscopy (DMLB digital camera; Leica, Heidelberg, Germany).
Haematoxylin–eosin staining was used to examine islet morphology and size. Briefly, freshly cut, air-dried pancreatic sections were rinsed with PBS and washed twice with double distilled H2O before haematoxylin staining for 1 min and rinsing in Scott’s tap water for colour development. Slides were then counterstained with eosin. After washing with water and graded dehydration using ethanol and xylene, slides were mounted using entellan (Merck, Darmstadt, Germany). Islet size was then measured by automatic histomorphometry (ImageJ software; http://rsb.info.nih.gov/ij) [27].
Islet mRNA expression
Total islet mRNA was extracted by TRIzol reagent (GIBCO/BRL-Invitrogen, Carlsbad, CA, USA) using the manufacture’s protocol. Also using the manufacture’s protocol (Invitrogen), first-strand cDNA was generated from 3 μg mRNA in 20 μl volume system using SuperScript II reverse transcriptase with oligo (dT) 12–18 primers. Real-time-PCR was used to quantify mRNA expression. A real-time PCR detection system (iCycler; Bio-Rad Laboratories, Richmond, CA, USA) was used to perform real-time-PCR in amplification using 1 μl undiluted cDNA as template, with SYBR-Green-I-mix (Bio-Rad). mRNA expression was detected and Gapdh mRNA co-amplified as an internal control. Results were calculated using the 2−∆∆Ct method, while melting curve analysis was used to confirm PCR amplification specificity [26]. The primers used are listed in electronic supplementary material (ESM) Table. 1.
Western blot analysis
Pancreatic islets isolated from mice in each of the different groups were used for western blotting. Total protein was extracted from 100 size-matched islets per group using CytoBuster Protein Extraction Reagent (Novagen, Darmstadt, Germany). After electrophoresis on 10% (wt/vol.) polyacrylamide gels, blotted protein was transferred to nitrocellulose membranes (Bio-Rad) and blocked for 1 h at room temperature with 5% (wt/vol.) skimmed milk in PBS with 0.1% (vol/vol.) Tween-20. Blotted membranes were then incubated overnight at 4°C with primary antibodies against renin, renin receptor, ACE and AT1 receptor; appropriate horseradish peroxide-conjugated secondary antibodies were then added and incubated at room temperature for 1 h. Labelled protein bands were revealed by western blotting detection reagents (ECLplus; GE-Healthcare, Piscataway, NJ, USA) on autoradiography films (Fuji Film, Tokyo, Japan). Signals were measured using ImageJ software and expressed as fold change of the target protein:actin intensity ratios [26]. The antibodies used are listed in ESM Table 2.
Measurement of growth, glucose homeostasis and islet function
Mouse body weight was recorded during growth and glucose homeostasis assessed as previously described [14]. In brief, for random blood glucose measurement mouse-tail vein blood was collected weekly between 10.00 and 11.00 h during growth. Fasting blood glucose and serum insulin concentrations were measured after 6 h of fasting. Glucose tolerance was assessed by an intraperitoneal glucose tolerance test (IPGTT). Briefly, after 6 h fasting, mice were given 1.5 g/kg body weight of glucose by intraperitoneal injection. Blood glucose concentrations were measured in tail blood samples taken before and at 15, 30, 60, 90 and 120 min after glucose administration. Insulin sensitivity was assessed by an insulin tolerance test (ITT). After 4 h of fasting, mice were given an i.p. injection of insulin (0.75 U/kg body weight), and blood glucose was measured in samples taken at 0, 15, 30 and 60 min after insulin injection. To assess islet beta cell function, glucose-stimulated insulin secretion (GSIS) was examined as previously described [15]. Briefly, for each set of experiments, ten size-matched islets isolated from each different mouse group were incubated (1 h, 37°C, 95:5 O2/CO2) in KRB (supplemented with 10 mmol/l HEPES and 2 mg/ml BSA) with 1.7 mmol/l glucose, before transfer to KRB with 16.7 mmol/l glucose for a further hour in the same conditions. After incubation, the KRB supernatant fraction was collected for measurement of the insulin secreted using commercial mouse insulin ELISA kits (Mercodia, Uppsala, Sweden) (CV < 10%). Data were expressed as the change of insulin released by each ten-islet group at 16.7 mmol/l glucose compared with 1.7 mmol/l glucose incubation (Δ insulin secretion). The HOMA of beta cell function (HOMA-B) was used to assess pancreatic beta cell function, calculated as described [28].
Measurements of serum calcium and parathyroid hormone levels
Blood was collected from the heart immediately after death and random serum calcium levels measured by a calcium assay kit (Biovision, Mountain View, CA, USA). Serum parathyroid hormone (PTH) concentrations were measured by mouse PTH(1–84) ELISA (Immunotopics, San Clemente, CA, USA) (CV <10%).
Statistical analysis
Results are expressed as mean ± SEM for all groups of normally distributed data and as medians for non-normally distributed data. One-way ANOVA followed by Tukey’s post-hoc test was used for multiple comparisons between groups. Two-tailed Student’s t tests or Mann–Whitney tests were used to compare parametric and non-parametric data respectively. A value of p < 0.05 was considered statistically significant.
Results
25(OH)D 3 and 1,25(OH) 2 D 3 concentrations in vitamin D-deficient diet-fed mice and the effects of this diet on growth
The body weight of mice on vitamin D-deficient diets was similar to that of control-fed mice (Fig. 1a), while serum 25(OH)D3 and 1,25(OH)2D3 concentrations were greatly decreased after 8 weeks on the diet, confirming the establishment of vitamin D-deficiency (Fig. 1b, c).
Glucose homeostasis in vitamin D-deficient mice
Mice fed the vitamin D-deficient diet exhibited higher blood glucose concentrations than control-fed mice from the age of 6 to 12 weeks (Fig. 2a, b). By 8 weeks (4 weeks after starting on the vitamin D-deficient diet), random blood glucose concentrations were already higher in vitamin D-deficient mice (8.22 ± 0.479 mmol/l [mean ± SEM]) than in normal-diet-fed controls (6.675 ± 0.5721 mmol/l). At 12 weeks of age (8 weeks after starting on vitamin D-deficient diets), random blood glucose concentrations in vitamin D-deficient mice were significantly higher than in control-fed mice (10.28 ± 0.587 vs 7.925 ± 0.701 mmol/l) (Fig. 2a) and fasting glucose was also significantly increased (9.673 ± 0.425 mmol/l) vs normal-diet-fed mice (6.9 ± 0.609 mmol/l) (Fig. 2b). Glucose intolerance developed by 12 weeks of age in vitamin D-deficient mice (increased AUC vs normal-diet-fed mice) (Fig. 2c, d). Insulin tolerance was impaired in vitamin D-deficient mice, with abnormally high glucose concentrations at 15 and 30 min compared with those in control-fed mice after insulin injection (Fig. 2e). Serum insulin after 6 h fasting and the insulin resistance index (HOMA-IR) were also increased, the former significantly, in vitamin D-deficient mice compared with controls (Fig. 2f, g). Islet function assessment showed that GSIS was blunted in vitamin D-deficient mouse islets (Fig. 2h), while the HOMA-B index, representing beta cell function, was decreased in islets from that mouse group (Fig. 2i).
Islet histomorphology in vitamin D-deficient mice
The islet glucagon:insulin expression ratio in actively labelled areas of pancreas from vitamin D-deficient mice was similar to that in normal-diet-fed control mice (Fig. 3a). However, vitamin D-deficient mouse islets were larger (median 20,217.7 μm2) than normal-diet-fed control mouse islets (median 13,766.3 μm2; p < 0.0001 by Mann–Whitney test) (Fig. 3b).
Regulation of islet RAS component levels in vitamin D-deficient mice
The effects of hypovitaminosis D on islet RAS activity were examined through the profiles of several RAS components, including renin and the renin receptor. Protein levels of major islet RAS components, i.e. renin (Fig. 4a), renin receptor (Fig. 4b), ACE (Fig. 4c) and AT1 receptor (Fig. 4d), were all upregulated in islets from vitamin D-deficient vs those from islets of normal-diet-fed mice.
Islet function-related gene expression in vitamin D-deficient mice
Several genes related to islet function were significantly downregulated in vitamin D-deficient mouse islets, including Pdk1 (Fig. 5a), Foxo1 (Fig. 5b), Tcf7l2 (Fig. 5c) and Glut2 (also known as Slc2a2) (Fig. 5d). Among islet insulin-signalling-related genes, Irs1 mRNA expression and the expression of the anti-oxidative stress-related gene catalase were downregulated in islets of vitamin D-deficient mice (ESM Fig. 1a, b), although expression of the NADPH oxidase subunits p22 (also known as Cyba) and p47 (also known as Ncf1) was unchanged (ESM Fig. 1c, d). Consistent with the mRNA expression data, protein production of total IRS1, forkhead box O1 (FOXO1) and phosphoinositide-dependent kinase 1 (PDK1) was decreased in vitamin D-deficient vs control mice islets (ESM Fig. 2a–c).
The effect of the renin inhibitor aliskiren on glucose homeostasis in vitamin D-deficient mice
After 7 days of treatment with the renin inhibitor aliskiren, random and 6 h fasting blood glucose values in 12-week-old vitamin D-deficient mice were unchanged (Fig. 6a, b), while fasting serum insulin concentrations and HOMA-IR tended towards an increase (Fig. 6f, g). Impaired glucose tolerance in vitamin D-deficient mice was improved by aliskiren (Fig. 6c, d), as was insulin tolerance (assessed 15 min after insulin administration during an ITT) (Fig. 6e), i.e. postprandial, but not fasting insulin resistance was improved by RAS blockade. Islet beta cell function was significantly increased in aliskiren-treated vitamin D-deficient mice, as evidenced by the increased GSIS (Fig. 6h) and HOMA-B index (Fig. 6i). However, serum 25(OH)D3 concentrations remained low in aliskiren-treated mice (Fig. 6j).
The effects of aliskiren on islet renin, renin receptor levels, islet function-related gene expression, islet cell proliferation, and on serum calcium and PTH levels in vitamin D-deficient mice
In vitamin D-deficient mice, renin protein levels were not altered by aliskiren treatment (Fig. 7a), but renin receptor protein levels were reduced (Fig. 7b). Among genes relevant to islet function, no obvious changes were observed in Irs1 mRNA expression after aliskiren treatment (ESM Fig. 3a). Increases in Glut2 mRNA expression were marginal (Fig. 7c), while the decreased Pdk1 mRNA expression (Fig. 7d) seen in vitamin D-deficient mice was reversed after aliskiren treatment. Islet expression of the oxidative stress-related genes, NADPH oxidase subunits p22 and p47, was unaltered by aliskiren treatment (ESM Fig. 3c, d). However, and significantly, the decrease in catalase mRNA expression seen in vitamin D-deficient animals was reversed by aliskiren (ESM Fig. 3b).
Islet size and morphology were unchanged by aliskiren treatment (data not shown), but the increase in islet alpha cell proliferation seen in vitamin D-deficiency (i.e. increases in Ki67-labelled cells) was decreased by aliskiren treatment (ESM Fig. 4a, b), suggesting that renin inhibition exerts protective effects against increased glucagon action. We found no explanation for the increased islet size in vitamin D-deficient mice and this requires further study, as it may reflect increased cell proliferation or cell junction. Random calcium and PTH concentrations were similar in normal, vitamin D-deficient and vitamin D-deficient, aliskiren-treated groups of mice (ESM Fig. 4c, d).
Discussion
The present study confirms our earlier finding that chronic hypovitaminosis D increases local pancreatic islet RAS gene expression in vivo, and decreases islet beta cell function and insulin sensitivity, thereby contributing to loss of glycaemic control, with increased islet RAS component expression occurring independently of glycaemia (as also seen in Vdr-KO mice) [26]. However, stunted growth and the short life-span of Vdr-KO mice limit their use in this research. Furthermore, in human studies, the associations between vitamin D status and insulin sensitivity are often lost in obesity [29], while vitamin D supplementation did not improve glucose homeostasis in non-deficient patients with type 2 diabetes [30]. We therefore extended these studies in vivo using a genetically normal mouse model, which was healthy apart from dietary vitamin D deficiency. This allowed us to demonstrate that the increased RAS activity induced by vitamin D deficiency can be ameliorated by renin blockade, with improvements in islet function, postprandial insulin sensitivity and glucose homeostasis, in vivo, despite continuing vitamin D deficiency. These findings support the proposal that RAS overactivity can contribute, mechanistically, to hyperglycaemia related to vitamin D deficiency and suggest that renin inhibition may protect islet function and reduce insulin resistance, thereby improving glycaemic control in vivo.
In addition to well-known effects on the circulatory system, clinical trials of RAS blockade/inhibition have demonstrated a reduction in risk of diabetes [31]. Key to the development of type 2 diabetes is the combination of insulin resistance and islet dysfunction; a reduction of these effects can reduce diabetes risk and glycaemia. Chronic RAS overactivation (systemic and local) is known to contribute to insulin resistance, and RAS component blockade improves insulin sensitivity [32]. Angiotensin II regulates insulin actions in several peripheral tissues by modulating downstream signalling of the insulin receptor [33]. Inhibition of renin, the rate-limiting enzyme of the RAS, improves insulin sensitivity in adipocytes and skeletal muscles through effects on insulin action and glucose transport [34]. With the development of insulin resistance, reduced insulin secretion in response to glucose (GSIS) is a major hallmark of type 2 diabetes risk and it has been suggested that RAS blockade may prevent the beta cell loss that leads to overt diabetes. Isolated islets develop increased RAS component abundance in prolonged hyperglycaemia, with reduced GSIS and (pro)insulin synthesis [26, 35]. Indeed, our earlier studies showed that RAS blockade in pancreatic islets from diabetic animals improved islet function and glucose homeostasis, increased islet proliferation, reduced oxidative stress and inflammation in islets, and also reduced beta cell apoptosis [14, 15], thereby helping to prevent beta cell loss.
Elevated renin levels have been found in mutant Vdr-KO mice [19]. Furthermore, inverse relationships between vitamin D status and RAS activity help explain the beneficial effects of optimal vitamin D replacement therapy in chronic renal failure and cardiovascular disorders [36, 37]. Since vitamin D suppresses renin and RAS activity, but RAS activity increases with hyperglycaemia (aggravating islet damage and insulin resistance), vitamin D deficiency may aggravate loss of glycaemic control through increased RAS activity. Thus, the reduction of RAS overactivity, whether by vitamin D replacement (as we recently showed in isolated islets) [26] or by pharmacological means, could improve islet function and insulin sensitivity.
Although our young, genetically intact, but vitamin D-deficient, mouse model showed no changes in body weight, serum total PTH or calcium, the increased islet RAS component expression we found was consistent with the known upregulation of human RAS activity by the common problem of hypovitaminosis D (low circulating 25[OH]D3) [38]. Glycaemia increased over time in our mouse model, with decreased GSIS and HOMA-B index by 3 months of age, and with glucose intolerance, impaired insulin sensitivity and fasting hyperglycaemia, which we suggest is due to the combination of increased islet RAS activity and decreased vitamin D availability (since vitamin D reduces RAS overactivity and improves GSIS in hyperglycaemia) [26]. Although aliskiren-induced renin inhibition improved glycaemia, insulin sensitivity and islet function despite continuing vitamin D deficiency, the improvement in GSIS was only partial (by 25%), suggesting that the reduction of insulin resistance was an important contributor to the beneficial effects of renin inhibition on glycaemic control. Reductions in overall insulin resistance (as seen in the ITT) and in glucose tolerance (in OGTT) were marked, while fasting HOMA-IR increased, suggesting that RAS blockade reduces postprandial, but not fasting, insulin resistance. Increased serum insulin levels were observed, suggesting that the improved islet insulin secretory ability may also partially contribute to glycaemic control.
Overall, our findings support the proposition that control of RAS overactivity could help counteract the adverse effects of hyperglycaemia and hypovitaminosis D, through partially reducing insulin resistance, as well as by protecting islet beta cells. Additional support for this postulate is provided by several other aspects of our study. Islet FOXO1 abundance decreases in vitamin D-deficient states and FOXO1 normally increases beta cell mass, reduces insulin signalling [39] and signals islet enlargement, as in other models of type 2 diabetes [40]. Vitamin D deficiency-related Tcf7l2 downregulation, as in the present study, may aggravate hyperglycaemia, as Tcf7l2 variants and expression are associated with diabetic renal disease [41] and reduced insulin secretion [42]. Islets are themselves insulin-sensitive, through signalling pathways, including IRS1 and IRS2 [43]. Our finding of decreased Irs1 transcription in the presence of vitamin D deficiency could contribute to reduced insulin action on islets, in turn impairing islet growth and function through increased islet insulin resistance [44]. Adverse angiotensin II-induced effects on the vasculature have been reported [45, 46]. These effects normally regulate the maintenance of islet function and beta cell mass, probably due to similar effects on smooth muscle in vessel walls acting through target genes like Pdk1. Indeed, we found that the reduced Pdk1 expression seen in vitamin D deficiency was corrected by RAS blockade, implying RAS involvement in PDK1 regulation.
Insulin-signalling is impaired by glucagon [47]; thus the reversal of vitamin D deficiency-induced proliferation of glucagon-secreting alpha cells that we found with aliskiren treatment may reduce or prevent potential overactivation of glucagon actions in vitamin D-deficient states. Islet GLUT2, the major islet glucose transporter, is reduced in type 2 diabetes and by hyperglycaemia in the presence of increased insulin resistance [48], but aliskiren is unlikely to improve glucose homeostasis through this mechanism, as GLUT2 was not affected by RAS blockade.
In contrast to data from genetically modified mouse models of diabetes [16], our vitamin D-deficient mouse model showed no gene defects related to reactive oxygen species, but the reduced islet catalase activity seen in vitamin D-deficient islets may worsen islet oxidative stress in vitamin D deficiency. Since we found that renin blockade increased catalase expression, therapeutic RAS blockade may increase antioxidant protection in the islets.
Our findings are relevant to reported reductions in the risk of diabetes with RAS blockade [12]. However, aliskiren can increase the risk of hypotension and hyperkalaemia in clinical use. Indeed, the US Federal Drugs Authority recently advised that aliskiren should not be given to patients with renal dysfunction or diabetes, due to the risk of diabetic nephropathy [49, 50]. Other RAS-modulating medication that proves to be safe in patients with diabetes may have similar protective effects and, if so, may help protect against diabetes progression, as well as reducing the risk of diabetes. Further investigations are also needed to determine the detailed relationships between hypovitaminosis D and insulin resistance, as well as the underlying mechanisms.
Abbreviations
- AT1 :
-
Angiotensin II type 1
- FOXO1:
-
Forkhead box O1
- GSIS:
-
Glucose-stimulated insulin secretion
- HOMA-B:
-
HOMA of beta cell function
- HOMA-IR:
-
HOMA of insulin resistance
- IPGTT:
-
Intraperitoneal glucose tolerance test
- ITT:
-
Insulin tolerance test
- KO:
-
Knockout
- 1,25(OH)2D3 :
-
Calcitriol
- 25(OH)D3 :
-
25-Hydroxyvitamin D
- PDK1:
-
Phosphoinositide-dependent kinase 1
- PTH:
-
Parathyroid hormone
- RAS:
-
Renin–angiotensin system
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Acknowledgements
Aliskiren was from Novartis, Basel, Switzerland (MTA #33405).
Funding
This work was supported by the General Research Fund from the Research Grants Council of Hong Kong (reference numbers: CUHK 470709 and CUHK 468912), awarded to P.S. Leung.
Duality of interest
The authors declare that there is no duality of interest associated with this manuscript.
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QC contributed to the conception and design of the study, the acquisition of data, data analysis and interpretation, drafting and final approval of the manuscript. BJB contributed to data analysis and interpretation, manuscript revision and final approval of the manuscript. PSL contributed to the conception and design of the study, provision of study material, data analysis and interpretation, manuscript writing and final approval of the manuscript.
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ESM Fig. 1
The effect of vitamin D deficiency on islet insulin signalling and oxidative stress related gene expression. (a), Irs1 mRNA expression in islets from normal diet and from vitamin D deficient diet fed mice. (b), anti-oxidative stress gene catalase mRNA expression, (c), islet NADPH oxidase subunits p22 and (d), p47 mRNA expression (*: p < 0.5 vs. Deficient diet). (PDF 88 kb)
ESM Fig. 2
The protein levels of total IRS1 (a), FOXO1 (b) and PDK1 (c) in islets isolated from normal diet or vitamin D deficient diet treated mice. (*: p < 0.5, **; p < 0.01 vs. Normal diet). (PDF 146 kb)
ESM Fig. 3
The effect of aliskiren treatment on islet insulin signalling and oxidative stress related gene expression. (a), Irs1 mRNA expression in islets from vitamin D deficient and from D deficient + aliskiren treated mice. (b), anti-oxidant system related gene catalase mRNA expression, (c), islet NADPH oxidase subunits p22 and (d), p47 mRNA expression in the islets from vitamin D deficient and from D deficient + aliskiren treated mice. (*: p < 0.5 vs. Deficient diet). (PDF 88 kb)
ESM Fig. 4
(a), Islet alpha-cell proliferation [co-stained with ki67] and glucagon content in islets from normal, vitamin D deficient and D deficient + aliskiren treated mice (red = ki67; green = glucagon; blue = DAPI; purple = co-stained cell nucleus; white arrow indicated Ki67 and glucagon positive cells), shown as percentage of ki67-glucagon positive cells/total numbers of alpha-cells (b). The random serum level of calcium (c) and total PTH (1-84) (d) were also determined in mice from different groups (***:p < 0.001 vs. Deficient diet respectively, original magnification ×400). (PDF 290 kb)
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Cheng, Q., Boucher, B.J. & Leung, P.S. Modulation of hypovitaminosis D-induced islet dysfunction and insulin resistance through direct suppression of the pancreatic islet renin–angiotensin system in mice. Diabetologia 56, 553–562 (2013). https://doi.org/10.1007/s00125-012-2801-0
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DOI: https://doi.org/10.1007/s00125-012-2801-0