Abstract
Characterising the molecular networks that negatively regulate pancreatic β-cell function is essential for understanding the underlying pathogenesis and developing new treatment strategies for type 2 diabetes. We recently identified serine/threonine protein kinase 25 (STK25) as a critical regulator of ectopic fat storage, meta-inflammation, and fibrosis in liver and skeletal muscle. Here, we assessed the role of STK25 in control of progression of non-alcoholic fatty pancreas disease in the context of chronic exposure to dietary lipids in mice. We found that overexpression of STK25 in high-fat-fed transgenic mice aggravated diet-induced lipid storage in the pancreas compared with that of wild-type controls, which was accompanied by exacerbated pancreatic inflammatory cell infiltration, stellate cell activation, fibrosis and apoptosis. Pancreas of Stk25 transgenic mice also displayed a marked decrease in islet β/α-cell ratio and alteration in the islet architecture with an increased presence of α-cells within the islet core, whereas islet size remained similar between genotypes. After a continued challenge with a high-fat diet, lower levels of fasting plasma insulin and C-peptide, and higher levels of plasma leptin, were detected in Stk25 transgenic vs wild-type mice. Furthermore, the glucose-stimulated insulin secretion was impaired in high-fat-fed Stk25 transgenic mice during glucose tolerance test, in spite of higher net change in blood glucose concentrations compared with wild-type controls, suggesting islet β-cell dysfunction. In summary, this study unravels a role for STK25 in determining the susceptibility to diet-induced non-alcoholic fatty pancreas disease in mice in connection to obesity. Our findings highlight STK25 as a potential drug target for metabolic disease.
Introduction
Type 2 diabetes, characterised by hyperglycaemia in the context of insulin resistance, is one of the most common metabolic diseases in the world. Insulin production from pancreatic β-cells plays a vital role in maintaining the glucose homeostasis in the body, and β-cell dysfunction is central to the pathogenesis of type 2 diabetes. During the progression of obesity and insulin resistance, pancreatic islets initially increase β-cell mass and overproduce insulin; however, the ability of the β-cell to counteract an increased glucose load is short-lived and eventually pancreatic islets fail, giving rise to hyperglycaemia (Saltiel 2001). Hence, characterisation of the critical molecular pathways that negatively modulate pancreatic β-cell function is imperative for understanding the underlying pathogenesis of type 2 diabetes and identifying new pharmacological approaches to effectively restore glycaemia in diabetic patients.
In the search for novel targets regulating energy metabolism, we recently identified serine/threonine protein kinase 25 (STK25, also referred to as YSK1 or SOK1), a broadly expressed member of the sterile 20 (STE20) kinase superfamily (Thompson & Sahai 2015), as a central regulator of whole-body glucose and insulin homeostasis (Nerstedt et al. 2012, Cansby et al. 2013, Amrutkar et al. 2015a,b, 2016a,b, Chursa et al. 2017). We found that STK25-overexpressing transgenic mice display impaired systemic glucose tolerance and insulin sensitivity compared with wild-type littermates when both genotypes are fed a high-fat diet (Cansby et al. 2013). Reciprocally, Stk25 knockout mice are protected against high-fat diet-induced whole-body glucose intolerance and insulin resistance compared with their wild-type littermates (Amrutkar et al. 2015a). Furthermore, we observed a markedly accelerated ectopic lipid accumulation, combined with aggravated inflammatory infiltration and fibrosis, in the liver and skeletal muscle of high-fat-fed Stk25 transgenic mice compared with wild-type controls (Amrutkar et al. 2015b, Chursa et al. 2017), and the reciprocal effect of reduced diet-induced hepatic and muscle lipid storage was seen with STK25 knockdown (Amrutkar et al. 2015a). Consistent with these preclinical results, we found a significant positive correlation in human liver biopsies between STK25 expression and progression of non-alcoholic fatty liver disease (NAFLD) (Amrutkar et al. 2016a,b), and higher STK25 mRNA levels were detected in the skeletal muscle of type 2 diabetic patients compared with individuals with normal glucose tolerance (Nerstedt et al. 2012).
Increasing evidence supports the role of fat accumulation in the pancreas (i.e., pancreatic steatosis) in the development of type 2 diabetes, atherosclerosis, acute pancreatitis and pancreatic cancer (Catanzaro et al. 2016). In spite of this high medical relevance and an estimated prevalence between 16 and 35% (Wang et al. 2014, Lesmana et al. 2015, Zhou et al. 2016), the pathogenesis of non-alcoholic fatty pancreas disease (NAFPD) is still largely unknown. Our previous investigations demonstrating a critical role of STK25 in regulation of lipid partitioning and ectopic fat storage in liver and skeletal muscle (Nerstedt et al. 2012, Cansby et al. 2013, Amrutkar et al. 2015a,b, 2016a,b, Chursa et al. 2017) prompted us to hypothesise that STK25 also controls pancreatic steatosis in the context of chronic exposure to excess amount of dietary lipids. By characterisation of pancreatic morphology and function in Stk25 transgenic mice and wild-type littermates challenged with a high-fat diet, this study unravels a hitherto unknown role of STK25 in determining the susceptibility to NAFPD.
Materials and methods
Animals
Stk25 transgenic mice were generated and genotyped as described previously (Cansby et al. 2013). From the age of 6 weeks, male transgenic mice and wild-type littermates were fed a pelleted high-fat diet (45% kilocalories from fat; D12451; Research Diets, New Brunswick, NJ, USA). At the age of 24 weeks, the mice were killed after 4 h of food withdrawal and blood was collected by heart puncture. Pancreas was weighed and collected for histological analysis (see Histology and immunofluorescence) or snap frozen in liquid nitrogen and stored at –80°C for the analysis of gene expression (see Supplementary Fig. 1 for schematic overview, see section on supplementary data given at the end of this article). All animal experiments were performed after approval from the local Ethics Committee for Animal Studies at the Administrative Court of Appeals in Gothenburg, Sweden, and followed appropriate guidelines.
Histology and immunofluorescence
Pancreas samples were fixed with 4% formaldehyde in phosphate buffer (Histolab Products, Gothenburg, Sweden), embedded in paraffin and sectioned. Islet area, islet perimeter, the number of islets, islet distribution and the number of vessels were assessed in full pancreatic sections stained with hematoxylin-eosin (H-E; Histolab Products). For immunofluorescence, sections were incubated with primary antibodies for STK25, insulin, glucagon or α-smooth muscle actin (α-SMA), followed by incubation with secondary antibodies (see Supplementary Table 1 for antibody information). The distribution of inflammatory cell infiltrate was assessed, and a total insulitis score was calculated as described previously (Fukuda et al. 2008) in all islets present in full pancreatic sections stained with Periodic Acid Schiff (PAS) kit (Sigma-Aldrich). Sections were also stained with Picrosirius Red (Histolab Products) and counterstained with Fast Green (Sigma-Aldrich). Apoptotic cells were detected by TUNEL assay using the Apo-BrdU-IHC In Situ DNA Fragmentation Assay kit (BioVision).
Pancreas samples were also embedded in optimal cutting temperature mounting medium (Histolab Products) and frozen in liquid nitrogen followed by cryosectioning and staining with Oil Red O (Eastman Kodak Company, Rochester, NY, USA) or MitoTracker Red (Thermo Fisher Scientific). For immunofluorescence, sections were incubated with primary antibodies for Ly6C, followed by incubation with secondary antibodies (see Supplementary Table 1 for antibody information).
All the quantifications were performed in 4–6 non-consecutive pancreatic sections per mouse using the ImageJ software (ImageJ, v1.47; NIH, Bethesda, MD, USA).
Ultrastructural analysis of pancreas was performed by transmission electron microscopy (TEM; LEO 912AB; Omega; Carl Zeiss NTS) as previously described (Anderberg et al. 2013).
Quantitative real-time PCR
Relative quantification of mRNA was performed as described (Cansby et al. 2013) using QuantStudioTM 6 Flex System (Applied Biosystems; see Supplementary Table 2 for custom-designed primer sequences). Relative quantities of target transcripts were calculated from duplicate samples after normalisation of the data against the endogenous control, 18S rRNA (Applied Biosystems).
Biochemical assays
The fasting plasma insulin, C-peptide, leptin and glucagon levels were assessed using the Ultrasensitive Mouse Insulin ELISA kit (Chrystal Chem Inc., Downers Grove, IL, USA), the Mouse C-Peptide ELISA kit (Chrystal Chem Inc.), the Mouse Leptin ELISA kit (Abcam) and the Mouse Glucagon ELISA kit (Chrystal Chem Inc.), respectively. Pancreas homogenates were analysed using the Triglyceride Quantification Colorimetric kit (BioVision) and the Free Fatty Acid Quantification Colorimetric kit (BioVision).
Determination of Mitochondrial DNA (MtDNA) content
Total DNA was extracted from pancreas using the EZNA Tissue DNA kit (Omega Bio-Tek). MtDNA content was measured with quantitative real-time PCR using the Power UP™ SYBR Green Master Mix (Applied Biosystems) and QuantStudioTM 6 Flex System.
Intraperitoneal Glucose Tolerance Test (IPGTT)
Following 4 h of food withdrawal, mice were injected with glucose (1 g/kg; Fresenius Kabi, Bad Homburg, Germany) intraperitoneally at time 0. Blood was taken from the tail tip to determine blood glucose concentrations at 0, 15, 30, 60, 90 and 120 min post-injection, using an Accu-Chek glucometer (Roche Diagnostics). The plasma insulin was assessed at 0, 5, 15 and 30 min, and plasma C-peptide was determined at 0 and 15 min after glucose challenge.
Insulin secretion assay in isolated pancreatic islets
Pancreatic islets were isolated by collagenase digestion as described before (Ammala et al. 1993) and incubated overnight at 37ºC in RPMI 1640 medium (Thermo Fisher Scientific) containing 11 mM glucose. The experiments for insulin secretion were carried out in 12-well plates (ten islets per well) for 60 min in RPMI 1640 medium containing 5.5 or 16.5 mM glucose. The medium was collected, and insulin concentration was determined using the Ultrasensitive Mouse Insulin ELISA kit.
Statistical analysis
Statistical significance between groups was calculated with an unpaired two-tailed Student t-test. P < 0.05 was considered statistically significant.
Results
Overexpression of STK25 alters the distribution of pancreatic α- and β-cells and reduces the islet β/α-cell ratio without any change in islet size
We found that STK25 protein could be detected by immunofluorescence analysis of pancreatic sections both in islets and in surrounding exocrine tissue of Stk25 transgenic mice as well as corresponding wild-type littermates (Supplementary Fig. 2). The immunofluorescence assessment does not allow to reliable quantify the level of overexpression in transgenic mice; however, our previous investigations by quantitative real-time PCR and western blot revealed that STK25 mRNA and protein abundance are increased by approximately 20- and 6-fold, respectively, in whole pancreatic extracts of high-fat-fed Stk25 transgenic mice compared with those in wild-type mice (Cansby et al. 2013). We also found 25.1 ± 3.2-fold overexpression of Stk25 mRNA in the pancreatic islets isolated from high-fat-fed Stk25 transgenic mice compared with that in wild-type mice (Supplementary Fig. 3).
We first investigated the overall pancreas morphology in high-fat-fed Stk25 transgenic and wild-type mice. Our previous studies have shown that Stk25 transgenic mice challenged with a high-fat diet develop peripheral insulin resistance compared with wild-type littermates (Cansby et al. 2013). Diminished insulin sensitivity and a consequent rise in insulin demand are normally compensated by increased islet size (Prentki & Nolan 2006). Notably, we found that the pancreas weight was similar in Stk25 transgenic vs wild-type mice (Fig. 1A). Moreover, the comprehensive morphometric analysis on H-E-stained pancreatic sections showed that the mean islet area and perimeter, the islet size distribution and the distribution of islets in the head, body and tail region of the pancreas were similar comparing the genotypes (Fig. 1B, C and D), suggesting no compensatory hyperplasia as a result of aggravated insulin resistance in transgenic mice compared with their wild-type controls.
Immunofluorescence staining of the pancreatic sections for insulin and glucagon revealed 1.8 ± 0.2-fold lower insulin-positive area size, with a tendency for higher glucagon-positive area size, in Stk25 transgenic islets compared with wild-type islets, resulting in 2.6 ± 0.4-fold decrease in islet β/α-cell ratio (Fig. 1E). In wild-type mice, a typical pattern of insulin-producing β-cells clustered in the core of the islet, and a few glucagon-immunoreactive α-cells localised to the periphery of the islet, was observed (Fig. 1E). In contrast, a presence of α-cells within the islet core was frequently seen in transgenic islets (Fig. 1E).
The mRNA expression of insulin (Ins1 and Ins2) in whole pancreatic extracts did not differ, however, between genotypes, while glucagon mRNA expression (Gcg) was 4.6 ± 1.0-fold increased in Stk25 transgenic mice (Supplementary Fig. 4). At the time of termination, approximately 2-fold lower levels of fasting plasma insulin and C-peptide, and 1.3 ± 0.1-fold higher levels of plasma leptin, were observed in Stk25 transgenic vs wild-type mice, whereas circulating glucagon levels were similar in both genotypes (Fig. 2).
STK25 overexpression aggravates diet-induced fat storage in the pancreas
We next compared lipid accumulation in the pancreatic tissue of high-fat-fed Stk25 transgenic and wild-type mice. We found that triacylglycerol content extracted from whole pancreas was 1.7 ± 0.3-fold higher in Stk25 transgenic vs wild-type mice (Fig. 3A). Consistently, histological analysis showed 2.4 ± 0.5- and 2.2 ± 0.4-fold increase in neutral lipids, as judged by Oil Red O staining, in the pancreatic islets and the exocrine pancreatic tissue of Stk25 transgenic mice, respectively (Fig. 3B). Notably, the content of free fatty acids in the pancreatic extracts was determined to be similar comparing the two genotypes (Fig. 3C).
There are several possible pathways that could underlie the increase in diet-induced lipid deposition in the pancreas of Stk25 transgenic mice such as enhanced lipid synthesis from one side (input) and repressed mitochondrial fatty acid oxidation on the other side (output) – or a combination of these mechanisms. We found that the pancreatic mRNA expression of the two key enzymes in de novo lipogenesis – acetyl-CoA carboxylase 1 (Acaca, also known as Acc1) and fatty acid synthase (Fasn) – as well as glycerol-3-phosphate acyltransferase (Gpam, also known as Gpat1), which catalyses the final and only committed step in triacylglycerol synthesis pathway, was similar in Stk25 transgenic and wild-type mice (Supplementary Fig. 4). To assess mitochondrial activity, we measured the signal for MitoTracker Red, a fluorescent dye that specifically accumulates within respiring mitochondria. Surprisingly, we found that the relative area staining for MitoTracker Red was 6.4 ± 1.9-fold higher, rather than lower, in Stk25 transgenic vs wild-type pancreas (Fig. 3D). MtDNA copy number in the pancreatic extracts was, however, not altered between genotypes (Supplementary Fig. 5) and imaging by TEM did not reveal any ultrastructural differences comparing the mitochondria in the pancreatic islets of Stk25 transgenic vs wild-type mice (Supplementary Fig. 6). The mRNA expression of carnitine palmitoyltransferase 1α (Cpt1α), an enzyme regulating long-chain fatty acyl-CoA uptake and oxidation in mitochondria, and the components of tricarboxylic acid (TCA) cycle – citrate synthase (Cs) and cytochrome c (Cycs) – were also similar in Stk25 transgenic and wild-type pancreas (Supplementary Fig. 4). Similarly, mRNA for fatty acyl-CoA oxidase (Acox1), which performs the first step of peroxisomal β-oxidation, was not altered comparing the genotypes (Supplementary Fig. 4).
Increased inflammatory cell infiltration, fibrosis and apoptosis in the pancreas of Stk25 transgenic mice
There is a growing recognition that proinflammatory cell infiltration into pancreatic islets in humans and animals with diabetes is involved in the progression of compensated insulin resistance to insulin-dependent type 2 diabetes (Ehses et al. 2007, Jourdan et al. 2013). We therefore performed histological analysis of the distribution of inflammatory cell infiltrate in pancreatic islets from Stk25 transgenic and wild-type mice fed a high-fat diet. We found that the percentage of non-inflamed islets was significantly lower in Stk25 transgenic mice, whereas the percentage of islets with peri-insulitis, defined by the presence of aggregates of mononuclear inflammatory cells surrounding the islets, was significantly higher in Stk25 transgenic mice compared with wild-type controls (Fig. 4A and B). Furthermore, the relative amount of islets with insulitis, defined by the presence of inflammatory infiltrate within the islets, was also increased in Stk25 transgenic mice, although this difference did not reach statistical significance (P = 0.07; Fig. 4A and B). The total insulitis score based on semi-quantitative grading of non-inflamed islets (score 0), peri-insulitis (score 1) and insulitis (score 2) was 1.5 ± 0.1-fold higher in Stk25 transgenic vs wild-type mice (Fig. 4C).
Macrophages have been demonstrated to be the most frequent immune cells in the insulitic type 2 diabetic pancreases (Boni-Schnetzler et al. 2008, Lundberg et al. 2017). Notably, we have previously shown that the liver of Stk25 transgenic mice fed a methionine- and choline-deficient (MCD) diet displays markedly enhanced staining for the marker of activated macrophages Ly6C compared with corresponding wild-type livers (Amrutkar et al. 2016a). Consistently, here we found that Ly6C-positive area was augmented by 1.8 ± 0.2-fold in pancreatic islets of Stk25 transgenic mice compared with corresponding wild-type mice (Supplementary Fig. 7).
To assess the degree of fibrosis, the pancreatic sections were stained with Picrosirius Red for collagen fibres. The Picrosirius Red signal was 1.3 ± 0.1-fold higher in Stk25 transgenic pancreas, with staining being apparent both outside the islets, within the islets and at the islet boundary (Fig. 5A). Furthermore, α-SMA immunohistochemistry was performed to quantify the number of activated pancreatic stellate cells (PSCs), the putative cells responsible for fibrosis in the pancreas. In consistent with Picrosirius Red staining, the α-SMA signal was increased by 1.8 ± 0.3-fold in pancreatic sections from Stk25 transgenic mice (Fig. 5B). PSCs are also considered to regulate the angiogenesis (Masamune et al. 2008, Erkan et al. 2009). However, no difference in vessel structure/counts was observed comparing the histological sections from both genotypes (Supplementary Fig. 8).
Lipid overload in the β-cells is known to correlate with programmed cell death in both animal models and humans (Pick et al. 1998, Butler et al. 2003). We therefore examined in situ apoptosis by TUNEL staining that identifies DNA fragmentation within apoptotic cells. TUNEL-positive area was increased 3.0 ± 0.3- and 2.4 ± 0.4-fold in the pancreatic islets and the exocrine pancreatic tissue, respectively, in Stk25 transgenic mice compared with wild-type littermates (Fig. 5C).
Overexpression of STK25 represses glucose-stimulated insulin secretion in vivo
To study whether the aggravated fat infiltration, inflammation and fibrosis in the pancreas of Stk25 transgenic mice leads to an impairment of the in vivo glucose-stimulated insulin release, we performed IPGTT in high-fat-fed mice. We found that blood glucose levels were higher in Stk25 transgenic mice compared with wild-type littermates over the whole time course of the IPGTT (the area under the curve (AUC) for glucose was 22.4 ± 4.8% higher for Stk25 transgenic than for wild-type mice; Fig. 6A), which is consistent with our previous observation based on a different cohort of mice (Cansby et al. 2013). Notably, in spite of higher net change in plasma glucose levels in Stk25 transgenic mice during IPGTT, the concomitant plasma insulin levels remained lower compared with wild-type littermates (the AUC for insulin was 28.7 ± 5.2% lower for Stk25 transgenic than for wild-type mice; Fig. 6B), suggesting a relative impairment in glucose-stimulated insulin secretion. The C-peptide/insulin ratio, a marker of insulin clearance (Poy et al. 2002, Tamaki et al. 2013), was similar comparing the two genotypes at basal conditions as well as at 15 min of glucose challenge (Supplementary Fig. 9).
To evaluate the effect of glucose on insulin secretion from isolated pancreatic islets, we incubated the islets from high-fat-fed mice in vitro with 5.5 or 16.5 mM glucose. However, there was no difference in insulin secretion comparing the islets of Stk25 transgenic vs wild-type mice (Supplementary Fig. 10).
Discussion
Recent evidence suggests that obesity-related fat accumulation within the pancreas (i.e. NAFPD) is associated with pancreatic inflammation and PSC-mediated fibrogenic processes, and leads to β-cell dysfunction (Smits & van Geenen 2011, Catanzaro et al. 2016). In this present study, we unravelled a role for protein kinase STK25 in determining the susceptibility to diet-induced NAFPD in mice by aggravation of pancreatic fat accumulation, inflammatory cell infiltration, PSC activation and fibrosis. Consistent with these morphological alterations in the pancreas, we showed that high-fat-fed STK25-overexpressing transgenic mice had impaired glucose-stimulated insulin release in vivo compared with high-fat-fed wild-type controls, which likely contributes to the previously reported systemic glucose intolerance (Cansby et al. 2013).
Interestingly, we observed that Stk25 transgenic mice displayed alterations in islet architecture. Specifically, we noted increased presence of glucagon-producing α-cells in the islet core of transgenic mice, in contrast to the typical arrangement of centrally located insulin-producing β-cells with a satellite distribution of α-cells in the periphery in wild-type mice. The molecular mechanisms linking STK25 overexpression to changes in islet structure remain unclear at present; however, an abnormal spatial relationship between α- and β-cells is frequently observed in mouse models of diet-induced diabetes (Hinault et al. 2011, Kai et al. 2013, Trasino et al. 2015) and it is thought to contribute to β-cell dysfunction by interfering with coordination of β-cell oscillatory activity throughout the islet (Cabrera et al. 2006).
We previously showed that peripheral insulin resistance in high-fat-fed Stk25 transgenic mice compared to wild-type controls is accompanied by hyperinsulinaemia (Cansby et al. 2013), suggesting that pancreatic β-cells could potentially increase insulin production in response to increased insulin demands. However, in this study, we observed that, after prolonged high-fat diet challenge, fasting insulin concentrations were lower in Stk25 transgenic than in wild-type mice at the time of termination. Furthermore, circulating levels of C-peptide were also decreased in Stk25 transgenic mice at this time point; because C-peptide has a longer half-life than insulin, it is considered a more sensitive index of insulin secretion than fasting insulin. Consistently, we found no evidence of hyperplasia of pancreatic islets by histological analysis in Stk25 transgenic vs wild-type mice. Taken together, these data suggest that a compensatory capability of β-cells found in Stk25 transgenic mice at a younger age is lost after a continued high-fat diet challenge. Multiple factors and signalling pathways have been shown to have an impact on decompensation of β-cells and the subsequent progression into diabetes, and in particular, β-cell apoptosis has emerged as a key event (Donath et al. 2005, Bonner-Weir et al. 2010, Poitout et al. 2010, Ashcroft & Rorsman 2012). Indeed, we observed aggravated apoptosis in Stk25 transgenic pancreas, which probably contributed to the lost ability to increase insulin secretion in the context of insulin resistance. Interestingly, MST1 (also known as STK4 or KRS2), another member of the STE20 kinase superfamily, was recently also identified as a critical regulator of apoptotic β-cell death (Ardestani et al. 2014).
The molecular mechanisms that cause pancreatic β-cell damage in the context of obesity are complex and not fully elucidated. In addition to genetic predisposition (O’Rahilly 2009), the combination of excess free fatty acids and glucose (i.e. glucolipotoxicity (Poitout et al. 2010, Kim & Yoon 2011, Leibowitz et al. 2011)) is known to lead to β-cell death by apoptosis and to decreased insulin secretion. Notably, Stk25 transgenic and wild-type mice display comparable levels of body fat and circulating lipids (including free fatty acids, total cholesterol and triacylglycerol) after a dietary challenge (Cansby et al. 2013, Amrutkar et al. 2015b). Moreover, fasting blood glucose levels are similar in Stk25 transgenic and wild-type mice on a high-fat diet and in age-matched lean chow-fed controls (Cansby et al. 2013). Therefore, it is likely that the alterations observed in the pancreas of Stk25 transgenic mice are related to STK25 overexpression, rather than systemic effects through more severe glucolipotoxicity. However, since endogenous STK25 is present in a wide range of different tissues (Pombo et al. 1996, Osada et al. 1997, Nerstedt et al. 2012, Cansby et al. 2013) and Stk25 transgenic mice display global overexpression of the gene (Cansby et al. 2013), this model is not suitable to address whether the pancreatic phenotype is due to a direct cell-autonomous effect of STK25 or secondary to the action of STK25 in other tissues. Interestingly, we failed to detect any impairment of glucose-stimulated insulin secretion in vitro in pancreatic islets isolated from Stk25 transgenic mice, suggesting the potential contribution of systemic factors to regulation of glucose-stimulated insulin release by STK25. Of note, in this study, we observed slightly higher circulating leptin levels in high-fat-fed Stk25 transgenic vs wild-type mice. Leptin is an energy balance-regulating adipokine (Coppari & Bjorbaek 2012) that also is associated with many autoimmune and inflammatory diseases, and higher serum leptin concentrations have previously been connected to inflammatory processes in the pancreas (Kerem et al. 2007). It is therefore possible that increased circulating leptin levels contributed to the more severe pancreatic inflammation observed in Stk25 transgenic vs wild-type mice.
Our previous studies showed that overexpression of STK25 in liver and skeletal muscle cells represses mitochondrial function and β-oxidation, which contributes to increased intrahepatocellular and intramyocellular lipid storage in the respective tissues (Amrutkar et al. 2015b, Chursa et al. 2017). It is known that maintained mitochondrial function in the pancreas is essential to preserve insulin secretion, and impairments in mitochondrial morphology and function have been shown to decrease insulin secretion, presumably through blunted ATP production (Lu et al. 2010). It has also been reported that β-cell apoptosis in obesity is induced via a mitochondria-dependent pathway, which is defined by the loss of mitochondrial transmembrane potential and release of proapoptotic signals to the cytosol (Karaskov et al. 2006, Martinez et al. 2008, Gurzov & Eizirik 2011, Qi & Xia 2012). Unexpectedly, we found increased, rather than decreased, mitochondrial activity in the pancreas of Stk25 transgenic mice when assessed by MitoTracker Red staining, suggesting that altered mitochondrial activity in transgenic pancreas is likely a compensatory response to a higher lipid load rather than a causative factor driving increased lipid accumulation in this organ. Consistent with this observation, increased hepatic mitochondrial oxidation has been reported in patients and rodents with NAFLD (Sunny et al. 2011, Satapati et al. 2012), which is considered to reflect a metabolic adaptation to elevated liver lipid burden to limit further fat deposition. However, it is acknowledged that MitoTracker Red staining is an indirect method to monitor mitochondrial activity, and future studies by directly measuring the mitochondrial oxygen consumption in different tissues are needed to fully understand the role of STK25 in the regulation of mitochondrial bioenergetics.
The alterations in the pancreas of Stk25 transgenic mice are consistent with our previous investigations in liver and skeletal muscle, where STK25 overexpression under conditions of excess dietary fat aggravates lipid deposition, inflammation and fibrosis (Cansby et al. 2013, Amrutkar et al. 2015b, 2016a, Chursa et al. 2017). Taken together, these findings suggest that STK25 increases the susceptibility to ectopic lipid storage and meta-inflammation in the main tissues prone to diabetic damage under metabolic stress, resulting in whole-body glucose intolerance and insulin resistance (Fig. 7). Notably, we have also shown earlier that white adipocytes from subcutaneous fat deposits of high-fat-fed Stk25 transgenic mice are larger than those from high-fat-fed wild-type controls (Cansby et al. 2013), indicating that lipid accumulation in the pancreas, liver and muscle is not a consequence of impaired fat storage capacity in adipose tissue (Fig. 7).
In this study, we characterised the pancreatic phenotype of Stk25 transgenic and wild-type mice challenged with a high-fat diet in order to mimic conditions in high-risk individuals, while chow-fed groups have not been examined, which is a limitation of the study. Notably, our previous investigations have shown that liver and skeletal muscle lipid deposition and whole-body insulin sensitivity are not significantly altered comparing Stk25 transgenic vs wild-type mice fed regular chow diet (Cansby et al. 2013, Amrutkar et al. 2016a, Chursa et al. 2017), suggesting that overexpression of STK25 may lead to significant metabolic alterations in mice only after a dietary challenge.
In summary, the findings in the present study, combined with our previous investigations, reveal that protein kinase STK25 is not only important for regulating peripheral insulin resistance upon chronic exposure to dietary lipids, but it also plays a critical role in β-cell functionality under lipotoxic conditions. Thus, pharmacological manipulation of the STK25 pathway might represent a therapeutic strategy, which combines both regulation of the insulinotropic function and insulin sensitivity in the obese state.
Supplementary data
This is linked to the online version of the paper at http://dx.doi.org/10.1530/JOE-17-0018.
Declaration of interest
M M is a founder and shareholder of ScandiCure AB. The authors declare that there is no other duality of interest associated with this article.
Funding
This work was supported by grants from the Swedish Research Council, the Novo Nordisk Foundation, the Swedish Heart and Lung Foundation, the Diabetes Wellness Network Sweden, the Estonian Research Council, the Swedish Diabetes Foundation, the Royal Society of Arts and Sciences in Gothenburg, the M Bergvalls Foundation, the Wiberg Foundation, the Adlerbert Research Foundation, the I Hultman Foundation, the S and E Goljes Foundation, the West Sweden ALF Program, the F Neubergh Foundation, the I-B and A Lundbergs Research Foundation, and the European Foundation for the Study of Diabetes and Novo Nordisk Partnership for Diabetes Research in Europe.
Author contribution statement
All the authors made substantial contributions to conception and design, acquisition of data, and/or analysis and interpretation of data. All the authors revised the article critically for important intellectual content and approved the final version of the article to be published. M M and E C wrote the manuscript. M M directed the project and is the guarantor of this work.
Acknowledgements
The authors acknowledge the editorial assistance of Rosie Perkins, Wallenberg Laboratory, Department of Molecular and Clinical Medicine, University of Gothenburg, Gothenburg, Sweden. The authors would also like to thank Dr. Thomas Greiner, Wallenberg Laboratory, Department of Molecular and Clinical Medicine, University of Gothenburg, Gothenburg, Sweden, for his valuable comments during the course of the study.
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