Abstract
Aims/hypothesis
MicroRNAs are key regulators of gene expression involved in health and disease. The goal of our study was to investigate the global changes in beta cell microRNA expression occurring in two models of obesity-associated type 2 diabetes and to assess their potential contribution to the development of the disease.
Methods
MicroRNA profiling of pancreatic islets isolated from prediabetic and diabetic db/db mice and from mice fed a high-fat diet was performed by microarray. The functional impact of the changes in microRNA expression was assessed by reproducing them in vitro in primary rat and human beta cells.
Results
MicroRNAs differentially expressed in both models of obesity-associated type 2 diabetes fall into two distinct categories. A group including miR-132, miR-184 and miR-338-3p displays expression changes occurring long before the onset of diabetes. Functional studies indicate that these expression changes have positive effects on beta cell activities and mass. In contrast, modifications in the levels of miR-34a, miR-146a, miR-199a-3p, miR-203, miR-210 and miR-383 primarily occur in diabetic mice and result in increased beta cell apoptosis. These results indicate that obesity and insulin resistance trigger adaptations in the levels of particular microRNAs to allow sustained beta cell function, and that additional microRNA deregulation negatively impacting on insulin-secreting cells may cause beta cell demise and diabetes manifestation.
Conclusions/interpretation
We propose that maintenance of blood glucose homeostasis or progression toward glucose intolerance and type 2 diabetes may be determined by the balance between expression changes of particular microRNAs.
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Introduction
Type 2 diabetes is characterised by insulin resistance of target tissues and insufficient insulin secretion from pancreatic beta cells to meet the organism’s needs. Insulin resistance is normally compensated by expansion of the beta cell mass and a rise in the insulin secretory activity [1]. However, in predisposed individuals this compensatory process fails, resulting in beta cell dysfunction, eventually accompanied by reduction of the beta cell mass and type 2 diabetes manifestation [2]. A better knowledge of the molecular mechanisms underlying beta cell adaptation and failure will be instrumental for designing new strategies to prevent or treat this disease.
MicroRNAs (miRNAs) are small non-coding RNAs that play central roles in a number of physiological and pathological processes [3]. Several studies have shown that miRNAs participate in the control of beta cell differentiation, function and mass. These non-coding RNAs regulate insulin production by directly or indirectly affecting the expression of key transcription factors and they contribute to fine-tuning of hormone release by modulating the levels of important components of the beta cell secretory machinery [4]. The expression of several miRNAs is affected by prolonged exposure to elevated concentrations of glucose, NEFA and proinflammatory cytokines [4]. Moreover, alterations in the levels of many islet miRNAs have been reported in different models of diabetes [5–9]. However, the functional impact of these miRNA expression changes and their potential role in the development of diabetes were, in most cases, not explored.
In this study, we analysed the global variations in islet miRNA expression in prediabetic and diabetic db/db mice [10] and in mice fed a high-fat diet (HFD) [11]. Differentially expressed miRNAs in these models of obesity-associated diabetes were systematically investigated for their effects on rat and human beta cell function and for their impact on cell survival on chronic exposure to pro-apoptotic conditions. The results indicate that specific changes in islet miRNA expression in prediabetic and diabetic states reflect the coexistence of adaptive processes elicited to compensate insulin resistance and of pathological reactions promoting beta cell failure. The balance between these opposing phenomena is likely to determine progression from normoglycaemia to hyperglycaemic states and the manifestation of diabetes.
Methods
Materials
TNFα and INFγ were obtained from R&D Systems (Minneapolis, MN, USA). IL-1β, prolactin (PRL), exendin-4 and palmitate were purchased from Sigma-Aldrich (St Louis, MO, USA).
Animals
Prediabetic (6 weeks old) and diabetic (14–20 weeks old) C57BL/KsJ db/db mice and age-matched C57BL/KsJ control animals were obtained from the Garvan Institute breeding colonies (Sydney, NSW, Australia) [10]. Five-week-old male C57BL/6 mice were purchased from Charles River Laboratories (Saint-Constant, QC, Canada) and fed a normal diet or HFD (Bio-Ser Diet number F3282, Frenchtown, NJ, USA; 60% [wt/wt] energy from fat) for 8 weeks as described [11]. Male Wistar rats were purchased from Charles River Laboratories (L’Arbresle, France). All animal procedures were performed in accordance with National Institutes of Health (NIH) guidelines and were approved by the respective Australian, Canadian and Swiss research councils and veterinary offices.
Microarray profiling
Total RNA was isolated with the mirVana RNA isolation kit (Ambion, Austin, TX, USA) from islets of C57BL/KsJ db/db mice or control animals. Total RNA from islets of C57BL/6 mice fed a normal diet or HFD was isolated with the miRNeasy kit (Qiagen, Hombrechtikon, Switzerland). Global miRNA expression profiling was carried out at the Genomic Technologies Facility of the University of Lausanne using miRNA gene microarrays (Agilent Technologies, Morges, Switzerland). Microarrays included probes for mouse miRNAs listed on www.mirbase.org/ (release 14, 2009).
Isolation and culture of dissociated islet cells
Pancreatic islets were isolated as described previously [12] by collagenase digestion followed by purification on a Histopaque (Sigma-Aldrich) density gradient. The islets were first cultured overnight in RPMI 1640 Glutamax medium (Invitrogen, Carlsbad, CA, USA) supplemented with 10% (vol./vol.) FCS (Amimed, BioConcept, Allschwill, Switzerland), 50 U/ml penicillin, 50 μg/ml streptomycin, 1 mmol/l Na pyruvate and 250 μmol/l HEPES, and then dissociated by incubation with trypsin (5 mg/ml at 37°C for 4–5 min). Human pancreatic islets were obtained from the Cell Isolation and Transplantation Center (University of Geneva), through the ECIT ‘Islets for Research’ distribution programme sponsored by the JDRF. The use of human islets was approved by the Geneva institutional Ethics Committee. Dissociated human islet cells prepared using the procedure described above were cultured in CMRL medium (Invitrogen) supplemented with 10% (vol./vol.) FCS, 100 U/ml penicillin, 100 μg/ml streptomycin, 2 mmol/l glutamine and 250 μmol/l HEPES. Detailed information about the human islet preparations used in this study is presented in electronic supplementary material (ESM) Table 1.
MIN6B1 cell culture
The murine insulin-secreting cell line MIN6B1 [13] was cultured at a density of 1.5 × 105 cells/cm2 in DMEM-Glutamax medium (Invitrogen) supplemented with 15% (vol./vol.) FCS, 50 U/ml penicillin, 50 μg/ml streptomycin, and 70 μmol/l β-mercaptoethanol.
Transfection and modulation of miRNA levels
MIN6B1 and dissociated rat or human islet cells were transfected with Lipofectamine 2000 (Invitrogen) with RNA oligonucleotide duplexes (Eurogentec, Seraing, Belgium) corresponding to the mature miRNA sequence (overexpression) or with single-stranded miScript miRNA inhibitors (Qiagen, Hombrechtikon, Switzerland) that specifically block endogenous miRNAs [14]. A custom-designed small interfering (si)RNA duplex directed against green fluorescent protein (sense 5′-GACGUAAACGGCCACAAGUUC-3′ and antisense 5′-ACUUGUGGCCGUUUACGU CGC-3′) and the miScript miRNA reference inhibitor (Qiagen) were used as negative controls for miRNA overexpression and downregulation, respectively.
Measurement of miRNA and mRNA expression
Mature miRNA expression was assessed with the miRCURY LNATM Universal RT MicroRNA PCR kit (Exiqon, Vedbaek, Denmark). Measurement of the levels of putative target mRNAs was performed by conventional reverse transcription (Promega, Dübendorf, Switzerland) followed by quantitative RT-PCR (qRT-PCR; Biorad, Reinach, Switzerland) with custom-designed primers (Microsynth, Balgach, Switzerland), details of which are available on request. MiRNA expression was normalised to the level of U6 or miR-7 (an islet-specific miRNA used as internal control) while mRNA expression was normalised to 18S.
Insulin secretion
At 2 days after transfection, MIN6B1 or dissociated rat islet cells were pre-incubated for 30 min at 37°C in Krebs buffer (127 mmol/l NaCl, 4.7 mmol/l KCl, 1 mmol/l CaCl2, 1.2 mmol/l KH2PO4, 1.2 mmol/l MgSO4, 5 mmol/l NaHCO3, 0.1% [wt/vol.] BSA, 25 mmol/l HEPES, pH 7.4) containing 2 mmol/l glucose. The pre-incubation medium was discarded and the cells incubated for 45 min in the same buffer (basal conditions). After collecting the supernatant fractions, the cells were incubated for 45 min in Krebs buffer containing 20 mmol/l glucose (stimulatory conditions). The incubation medium was collected and total cellular insulin contents recovered in acidified ethanol (75% [vol./vol.] ethanol, 0.55% [vol./vol.] HCl). The amount of insulin in the samples was determined using an insulin enzyme immunoassay kit (SPI-Bio, Bertin Pharma, Montigny le Bretonneux, France).
Cell death assessment
Transfected MIN6B1, rat or human dissociated islet cells were incubated with 1 μg/ml Hoechst 33342 (Invitrogen) for 1 min. The fractions of cells (at least 1 × 103 per condition) displaying pycnotic nuclei were scored under fluorescence microscopy (AxioCam MRc5; Zeiss, Feldbach, Switzerland). Apoptosis was triggered by exposing the cells to cytokines (30 ng/ml INFγ, 10 ng/ml TNFα and 0.1 ng/ml IL-1β) for 24 h or to medium (5% [vol./vol.] FCS) supplemented with 0.5 mmol/l palmitate bound to 0.5% [wt/vol.] BSA [15] for 48 h.
Proliferation assay
Transfected MIN6B1 or dissociated islet cells cultured on poly-l-lysine-coated glass cover slips were fixed with ice-cold methanol and permeabilised with 0.5% (wt/vol.) saponin (Sigma-Aldrich, St Louis, MO, USA). The cover slips were incubated with antibodies against Ki67 (1:500) (Abcam, Cambridge, UK) and insulin (1:500) (Millipore, Zug, Switzerland) and then with anti-rabbit Alexa-Fluor-488 and anti-mouse Alexa-Fluor-555 antibodies (Invitrogen). At the end of the incubation, the cover slips were washed with PBS containing Hoechst 33342 (Invitrogen) and images of at least 1 × 103 cells per condition were collected using a fluorescence microscope. PRL (500 ng/ml for 48 h) was used as positive control.
Protein extraction and western blotting
Protein lysates (30–50 μg) from MIN6B1 cells prepared as described previously [9] were separated on polyacrylamide gels and transferred to polyvinylidine fluoride membranes. The membranes were incubated overnight with antibodies against granuphilin [16] (1:2,000); mammalian target of rapamycin (mTOR; 2972, 1:1,000 Cell Signaling, Danvers, MA, USA), met proto-oncogene (hepatocyte growth factor receptor) (cMET; Cell Signaling, 3127, 1:1,000) and glycogen synthase kinase 3β (GSK-3β; Cell Signaling 9315, 1:1,000). Antibodies against α-tubulin (T9026, 1:10,000, Sigma-Aldrich) and actin (Clone C4 MAB1501, 1:15,000, Millipore) were used to verify equal loading. After exposure to IRDye (Li-Cor Biosciences, Bad Homburg, Germany) or horseradish-peroxidase-coupled secondary antibodies for 1 h, the bands were visualised via the Odyssey imaging system (Li-Cor Biosciences) and chemiluminescence (GE Healthcare Europe, Glattbrugg, Switzerland), respectively. Band intensity was quantified by ImageJ software.
Statistical analysis
Statistical differences were assessed using a Student’s t test or, for multiple comparisons, one-way ANOVA of the means, followed by a post-hoc Dunnett test (SAS statistical package; SAS, Carry, NC, USA).
Results
Islet miRNA expression in rodent models of type 2 diabetes
To investigate the contribution of miRNAs to beta cell dysfunction and the development of type 2 diabetes, we performed global miRNA expression profiling in pancreatic islets obtained from: db/db mice, which lack the leptin receptor and develop severe obesity associated with type 2 diabetes [10, 17]; and diet-induced obese mice, which display mild hyperglycaemia and beta cell dysfunction after being fed an HFD for 8 weeks [11]. The characteristics of the animals used in this study are presented in ESM Tables 2–4. We identified more than 60 differentially expressed miRNAs in db/db and HFD-fed mice islets compared with their respective controls, with overlapping changes in the two models (Fig. 1).
For db/db mice, miRNA expression was determined in both prediabetic (6 weeks old) and diabetic (14–20 weeks old) animals. In prediabetic mice, the miRNAs displaying the most striking changes were miR-132, with expression increasing by 8.2-fold, and miR-210, miR-184 and miR-203, for which expression decreased by 4.0-, 3.4- and 2.0-fold, respectively (ESM Table 5). In agreement with our previous findings [9], the islets of prediabetic db/db mice contained lower levels of miR-338-3p. The reduction of miR-210 and miR-184 was more dramatic in the islets of overtly diabetic db/db mice (10.4- and 115-fold decrease, respectively), whereas upregulation of miR-132 and downregulation of miR-203 and miR-338-3p remained approximately constant in prediabetic and diabetic animals (ESM Tables 5 and 6). In addition to these changes, the islets of adult diabetic mice were characterised by alterations in the levels of additional miRNAs, including an upregulation of miR-199a-5p (12.6-fold) and miR-199a-3p (9.4-fold), a decline of miR-383 (13.7-fold) and, as previously reported [6], an increase of miR-34a and miR-146a (ESM Table 6). The results obtained by microarray analysis were confirmed by qRT-PCR (Fig. 2a–l). Our microarray data also revealed a 2.2-fold increase in miR-21, which we have previously shown to inhibit insulin secretion [8], a 1.6-fold decrease in miR-26a, which controls insulin biosynthesis [18], and an increase in miR-802 (sixfold), which regulates Hnf1b expression [19] (ESM Tables 6). The role of these miRNAs was not further investigated in this study.
Islet miRNA expression was also analysed in HFD-fed mice. For this purpose we selected the group of mice displaying the strongest response to HFD. These animals were markedly obese, insulin resistant, hyperinsulinaemic and clearly hyperglycaemic (ESM Table 4). HFD mice showed miRNA expression changes analogous to those observed in the islets of diabetic db/db mice, with the exception of miR-21, miR-34a, miR-146a, miR-199a-5p and miR-199a-3p, which were not significantly modified (ESM Table 7 and Fig. 2m–s).
Overall, the data indicate that a subset of islet miRNAs is similarly altered in two obesity-associated animal models of type 2 diabetes, suggesting a role of specific miRNAs in beta cell failure and the development of hyperglycaemia.
miRNA expression is affected by glucolipotoxic conditions
To determine the possible causes of the changes in miRNA expression detected in the islets of db/db and HFD-fed mice, we tested whether the levels of these non-coding RNAs are affected by chronic exposure of beta cells to elevated concentrations of glucose and NEFA. We found that prolonged incubation of rat islets (Fig. 3) under glucolipotoxic conditions mimicked the modifications in miR-132, miR-184, miR-199a-3p, miR-203 and miR-383 expression observed in animal models. In contrast, under these glucolipotoxic conditions the levels of miR-210 and miR-199a-5p were not affected (Fig. 3).
Particular differentially expressed miRNAs influence beta cell functions and survival
Modifications of miRNA expression in islets could reflect the activation of adaptive processes counterbalancing the increased insulin needs caused by obesity and insulin resistance or the onset of pathological conditions leading to beta cell dysfunction. Indeed, we have previously shown that downregulation of miR-338-3p contributes to compensatory beta cell mass expansion [9], whereas overexpression of miR-21, miR-34a and miR-146a negatively impacts on beta cell function [6, 8]. To assess the possible role of other differentially expressed miRNAs in these phenomena, we mimicked the changes observed in the animal models by transfecting dissociated rat islet cells and MIN6B1 cells with oligonucleotide duplexes corresponding to the mature miRNA sequences or with anti-miRNA molecules that specifically inhibit miRNAs (ESM Fig. 1). The transfected cells were then analysed for their functional properties.
We first assessed whether the miRNAs differentially expressed in type 2 diabetes models are involved in the regulation of insulin biosynthesis and release. Most of the studied miRNAs did not affect insulin content (Fig. 4a–c) or insulin release in dissociated rat islet cells (Fig. 4d–f) and MIN6B1 cells (ESM Fig. 2). However, overexpression of miR-132 resulted in improved glucose-stimulated insulin release from dissociated rat islet cells (Fig. 4d). In contrast, upregulation of miR-199a-5p led to an insulin secretory defect in MIN6B1 cells (ESM Fig. 2), but not in islet cells, where it only diminished the insulin content (Fig. 4a).
We next investigated whether the miRNAs differentially expressed in type 2 diabetes models regulate beta cell expansion. In MIN6B1 cells, upregulation of miR-132 or downregulation of miR-184, miR-203 and miR-383 led to an increase in proliferation while modification of the levels of other miRNAs had no significant effects (ESM Fig. 3). Proliferation of insulin-positive cells was also observed on upregulation of miR-132 (Fig. 5a) and, to a lesser extent, downregulation of miR-184 in dispersed rat islet cells (Fig. 5b). In contrast, downregulation of miR-203 and miR-383 in primary cells had no effect (Fig. 5c, d). Similar to our previous work with miR-338-3p [9], these findings suggest that modification of the levels of miR-132 and miR-184 contributes to compensatory beta cell mass expansion elicited in response to insulin resistance.
As an increase in beta cell apoptosis and a reduction in beta cell mass are thought to play a role in the development of type 2 diabetes [20], we investigated the impact of miRNAs of interest on beta cell survival. As previously observed for miR-34a and miR-146a [6], upregulation of miR-199a-3p or reduction of miR-203, miR-210 and miR-383 expression increased the number of apoptotic MIN6B1 cells (ESM Fig. 4) as well as dispersed rat islet cells (Fig. 6a, c, e). Similar results were obtained using dissociated human islet cells (Fig. 6b, d, f). In contrast, overexpression of miR-132 or silencing of miR-184 did not induce beta cell death, but rather protected dispersed rat (Fig. 7a–d) and human (Fig. 7e–h) islet cells from apoptosis when the cells were chronically exposed to elevated concentrations of NEFA or to proinflammatory cytokines. Analogous results were also obtained in MIN6B1 cells (ESM Fig. 5).
Impact of particular miRNA changes on candidate target gene expression
As described above, db/db mouse islets are characterised by a specific rise in the levels of miR-21, miR-34a, miR-146a, miR-199a-3p and -5p and a downregulation of miR-203, miR-210 and miR-383 that possibly result in beta cell dysfunction and death. We previously found that miR-34a affects beta cell survival by directly targeting the anti-apoptotic protein B cell CLL/lymphoma 2 (BCL2) [6]. Combining bioinformatics-prediction algorithms (http://mirsystem.cgm.ntu.edu.tw/) and a literature search, we identified other miRNA targets potentially explaining the functional effects observed. In hepatocytes, miR-199a-3p regulates the expression of mTOR and of the transcription factor cMET [21], two proteins known to play important roles in the control of beta cell mass and survival [22, 23]. We found that upregulation of miR-199a-3p results in decreased expression of mTOR and cMET also in MIN6B1 cells (ESM Fig. 6), possibly explaining the negative impact of this miRNA on beta cell survival.
Increased expression of miR-132 displays beneficial effects on both beta cell mass and function. Computational prediction algorithms (http://mirsystem.cgm.ntu.edu.tw/) indicate that granuphilin (also known as synaptotagmin-like 4 [SLP-4]), a granule-associated protein that negatively affects insulin release [16], and GSK-3β, which negatively regulates beta cell function and mass [24, 25], are potential miR-132 targets. Translational repression of these two genes could explain, at least in part, the phenotypic traits of beta cells overexpressing miR-132. However, western blot analysis did not reveal any significant impact of miR-132 on the level of these proteins in MIN6B1 cells (ESM Fig. 6). MiRNAs often have small impacts on the expression of single direct targets [26]. However, cumulative effects can have major indirect influences on gene expression and cellular activities. Thus, instead of searching for direct targets, we measured the cellular level of a group of transcription factors known from the literature to improve survival and function of beta cells [27–29]. We found that upregulation of miR-132 in rat islet cells did not affect the mRNA levels of Foxm1 and Pdx1 but increased the level of Mafa (Fig. 8b). Downregulation of miR-184 that induces overlapping phenotypic changes did not alter the expression level of these genes (not shown).
Discussion
We have identified two groups of miRNAs displaying differential expression in pancreatic islets isolated from two animal models characterised by obesity, insulin resistance and beta cell dysfunction: db/db mice and HFD-fed mice. The changes in expression of miR-21, miR-34a, miR-132, miR-146a, miR-184, miR-210 and miR-383 detected in this study are consistent with those described by Zhao et al in the islets of leptin-deficient ob/ob mice [5] and are in agreement with previous findings from our laboratory [6, 8]. Elevated miR-21 levels were also detected in islets of glucose-intolerant human donors [30]. Moreover, our microarray data confirm the upregulation of miR-802 in the islets of db/db mice recently observed by Kornfeld et al [19]. Increased expression of miR-132, miR-199a-5p and miR-199a-3p have also been reported in the islets of GK rats, a lean model of type 2 diabetes [7]. Consistent with results obtained in ob/ob mice [5], our microarray data did not reveal significant changes in the level of many miRNAs that play important roles in the control of beta cell functions, including miR-9, miR-24, miR-124a and miR-148 [18, 31–33]. Moreover, we did not detect differences in the levels of miR-375, an islet-enriched miRNA that regulates insulin secretion and beta cell proliferation and that is slightly upregulated (about 30%) in ob/ob mice [34]. Thus, although appropriate expression of these miRNAs is required for ensuring optimal beta cell function, the development of type 2 diabetes appears not to be associated with major changes in the level of these non-coding RNAs. However, individuals expressing inappropriate levels of these miRNAs may display defective beta cell functions [30] and may be more susceptible to type 2 diabetes manifestation. Indeed, ob/ob mice lacking miR-375 develop diabetes [34].
The analysis of the functional impact of individual changes in miRNA expression in isolated islet cells revealed that some of them have beneficial effects on the activity of insulin-secreting cells whereas others result in beta cell death. Upregulation of miR-132 and downregulation of miR-184 and miR-338-3p are already observed in 6 week-old prediabetic obese db/db mice. These adaptive changes in miRNA expression that have a positive impact on beta cell functions are conserved or even more pronounced in HFD-fed and 14–20-week-old diabetic db/db mice. Indeed, when the level of these particular miRNAs was modulated in vitro, both tumoral and normal beta cells displayed enhanced proliferation and resistance to pro-apoptotic stimuli (present study and Jacovetti et al [9]). Moreover, a rise in the level of miR-132 improved the secretory response of the cells to glucose. These observations suggest that adaptive expression of miR-132, miR-184 and miR-338-3p may contribute to beta cell compensation processes.
The increased miR-132 content and the decreased miR-184 expression observed in db/db and HFD-fed mice were mimicked by incubation of dissociated rat islet cells in the presence of chronically elevated concentrations of palmitate and glucose. This suggests that these miRNAs may be induced in response to hyperglycaemia and hyperlipidaemia, two conditions typically encountered in prediabetic and diabetic states. In neurons, the expression of miR-132 is triggered following activation of the cAMP-dependent pathway and of the transcription factor cAMP response element-binding protein (CREB) [35–40]. Incubation of rat insulinoma INS-1 832/13 cells with cAMP-raising agents has been shown to cause a rapid increase in the miR-132 precursor [41], indicating that a similar regulatory mechanism may also operate in beta cells.
The mechanisms underlying the effects caused by changes in the level of miR-132 and miR-184 remain to be fully elucidated. We found that upregulation of miR-132 in dissociated rat islet cells leads to increased expression of Mafa, a gene playing an important role in the control of beta cell function and survival [28]. The expression of this transcription factor is decreased by palmitate [42] and is strongly reduced in the islets of diabetic db/db mice [10, 43]. Moreover, nuclear MAFA was recently reported to be diminished in the islets of individuals affected by type 2 diabetes [44]. Our data suggest that the induction of miR-132 helps preserve the level of MAFA during obesity-associated beta cell compensation.
Over the long term, the adaptive changes elicited by miR-132, miR-184 and miR-338-3p may become insufficient to counterbalance insulin resistance; alterations in the levels of additional miRNAs with deleterious impacts on beta cells also add to the effect. Indeed, the islets of HFD-fed and of diabetic db/db mice displayed changes in the levels of several other miRNAs, including miR-21, miR-34a, miR-146a, miR-199a-5p, miR-199a-3p, miR-203, miR-210 and miR-383; variation in expression of these miRNAs in vitro causes beta cell dysfunction and death (Lovis et al [6], Roggli et al [8] and present study). We previously showed that induction of miR-34a and miR-146a triggers beta cell apoptosis and that miR-21 and miR-34a have a deleterious impact on insulin secretion [6, 8]. Experiments carried out in this study revealed an increase in apoptosis after overexpression of miR-199a-3p or downregulation of miR-203, miR-210 and miR-383 in dissociated rat and human islet cells and in MIN6B1 cells. These phenotypic changes are not unique to beta cells as modifications in the level of some of these miRNAs promote apoptosis in other cell systems [21, 45–47]. Overexpression of miR-199a-3p resulted in a reduction of the levels of mTOR and cMET, two well-characterised targets of this miRNA [21, 48]. Disruption of the signalling pathways involving these two proteins is detrimental for beta cells [23, 49]. Moreover, mTOR is an important regulator of autophagy, a process thought to contribute to type 2 diabetes onset [50]. Thus, the toxic effects of miR-199a-3p may be the consequence of diminished expression of mTOR and cMET.
In conclusion, the present study is the first globally addressing the role of miRNAs in the aetiology of type 2 diabetes by systematically investigating the impact on primary beta cell function of miRNA changes observed in two animal models of obesity-associated diabetes. Our data demonstrate that obesity and insulin resistance are associated with modifications in two distinct groups of islet miRNAs that have opposing phenotypic effects on beta cells. Expression changes in miRNAs promoting beta cell mass expansion and boosting glucose-induced insulin secretion already occur in normoglycaemic animals and probably belong to adaptive processes allowing beta cells to compensate for insulin resistance. If these mechanisms fail to compensate for the diminished insulin sensitivity, additional modifications in miRNA expression may accumulate, causing beta cell failure and manifestation of type 2 diabetes. We propose that beta cell activities are tuned by a balance between the levels of particular miRNAs associated with enhanced function and mass, such as miR-132, miR-184 and miR-338-3p, and others having negative impacts, including miR-21, miR-34a, miR-146a, miR-199a-5p, miR-199a-3p, miR-203, miR-210 and miR-383. A better understanding of the precise role of particular miRNAs involved in the natural history of the beta cell in diabetes may be harnessed to design novel therapeutic strategies for diabetes prevention and treatment.
Abbreviations
- cMET:
-
Met proto-oncogene (hepatocyte growth factor receptor)
- GSK-3β:
-
Glycogen synthase kinase 3 β
- HFD:
-
High-fat diet
- miRNA:
-
microRNA
- mTOR:
-
Mammalian target of rapamycin
- PRL:
-
Prolactin
- qRT-PCT:
-
Quantitative RT-PCR
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Acknowledgements
We warmly thank Bryan Gonzalez (University of Lausanne, Switzerland) for expert technical help.
Funding
The authors are supported by Grants from the Swiss National Science Foundation (31003A-127254) (to RR), the European Foundation for the Study of Diabetes (to RR), the Canadian Institute of Health Research (to MP), the National Health and Medical Research Council of Australia (to DRL) and Société Francophone du Diabète (SFD)-Servier (to CJ). MP is a recipient of a Canada research chair in diabetes and metabolism. CG is supported by a fellowship from the Fonds de la Recherche en Santé du Québec (FRSQ), the SFD and the Canadian Diabetes Association.
Duality of interest
The authors declare that there is no duality of interest associated with this manuscript.
Contribution statement
VN and CG generated the data, wrote the manuscript and approved its final version. CJ, VM and M-LP contributed to the acquisition of data, critically reviewed the manuscript and approved its final version. DRL contributed to data acquisition and interpretation, reviewed the manuscript and approved its final version. MP contributed to the interpretation of the data, critically reviewed the manuscript and approved its final version. RR conceived the experiments, interpreted the data, reviewed the manuscript and approved its final version.
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Valeria Nesca and Claudiane Guay contributed equally to this work.
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ESM Table 1
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ESM Fig 1
Up or downregulation of miRNA expression in rat islet and MIN6B1 cells. Dispersed rat pancreatic islets cells (A) or MIN6B1 cells (B) were transfected with the indicated miRNA mimics, anti-miRNAs or their respective controls (Ctrl or anti-ctrl). miRNA overexpression or downregulation was measured by qRT-PCR and normalized to U6 or miR-7 levels. Results are expressed as fold change versus Ctrl or as percentage of anti-ctrl and correspond to the mean ± SD of at least three independent experiments. *Significantly different from control (p value ≤ 0.05, Student’s t test). (PDF 25.5 kb)
ESM Fig 2
Impact of specific miRNA changes on insulin content and secretion in MIN6B1 cells. MIN6B1 cells were transfected with the indicated miRNA mimics, antimiRNAs or respective controls (Ctrl or anti-ctrl). Two days later, insulin secretion under basal (glucose 2 mmol/l, black bars) and stimulatory conditions (glucose 20 mmol/l, white bars) (A) and insulin contents (B) were determined. Insulin release is expressed as percentage of insulin content. The results represent means ± SD of four to five independent experiments. *Significantly different from control condition (p value ≤ 0.05, ANOVA, Dunnett’s post-hoc test). (PDF 34.6 kb)
ESM Fig 3
Impact of specific miRNA changes on MIN6B1 proliferation. MIN6B1 cells transfected with the indicated miRNA mimics (A) or anti-miRNAs (B) were stained with an antibody against Ki67 to assess cell proliferation. Prolactin (PRL 500 ng/ml during 48 h) and exendin-4 (100 nmol/l, 48 h) were used as positive controls (grey bars). The results are expressed as fold change versus the respective control and correspond to the mean ± SD of at least three independent experiments. * Significantly different from control condition (p value ≤ 0.05, ANOVA, Dunnett’s post-hoc test). (PDF 12.0 kb)
ESM Fig 4
Impact of specific miRNA changes on apoptosis in MIN6B1 cells. MIN6B1 cells were transfected with the indicated miRNA mimics, anti-miRNAs or the respective controls. Cell death was assessed two days later by determining the percentage of cells displaying pycnotic nuclei upon Hoechst staining. A mix of pro-inflammatory cytokines (Cyt. mix) was used as a positive control for cell death (grey bar). The results are expressed as means ± SD of at least three independent experiments. *Significantly different from control condition (p value ≤ 0.05, ANOVA, Dunnett’s posthoc test). (PDF 12.1 kb)
ESM Fig 5
Protective effect of miR-132 overexpression and miR-184 inhibition on palmitate- or cytokine-induced apoptosis. MIN6B1 cells transfected with miR-132 mimic, anti-miR-184 or the respective controls were exposed for 48 h with (white bars) or without (black bars) 0.5 mmol/l palmitate coupled to 0.5% BSA (A) or for 24 h with (grey bars) or without (black bars) a mix of pro-inflammatory cytokines (B). Apoptosis was assessed 48 h post-transfection by counting the fraction of cells displaying pycnotic nuclei after Hoechst staining. The results correspond to the mean ± SD of four to six independent experiments. *Significantly different from control cells treated with the pro-apoptotic stimuli (p value ≤ 0.05, ANOVA, Dunnett’s post-hoc test). (PDF 13.6 kb)
ESM Fig 6
Potential targets of miR-199a-3p and miR-132. MIN6B1 cells were transfected with the indicated miRNA mimics. Two days later, the cells were homogenized and the lysates analyzed by Western blotting with antibodies against mTOR and cMET (A), GSK-3β (B) and granuphilin (C). The figure shows representative blots and band quantification from at least 3 independent experiments (means ± SEM). Protein levels were normalized to tubulin and expressed as fold change over control. *Significantly different from control condition (p value ≤ 0.05 by ANOVA analysis and Dunnett’s post-hoc test). (PDF 103 kb)
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Nesca, V., Guay, C., Jacovetti, C. et al. Identification of particular groups of microRNAs that positively or negatively impact on beta cell function in obese models of type 2 diabetes. Diabetologia 56, 2203–2212 (2013). https://doi.org/10.1007/s00125-013-2993-y
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DOI: https://doi.org/10.1007/s00125-013-2993-y