Figures
Abstract
The frog skin host-defense peptide esculentin-2CHa (GFSSIFRGVA10KFASKGLGK D20LAKLGVDLVA30CKISKQC) displays antimicrobial, antitumor, and immunomodulatory properties. This study investigated the antidiabetic actions of the peptide and selected analogues. Esculentin-2CHa stimulated insulin secretion from rat BRIN-BD11 clonal pancreatic β-cells at concentrations greater than 0.3 nM without cytotoxicity by a mechanism involving membrane depolarization and increase of intracellular Ca2+. Insulinotropic activity was attenuated by activation of KATP channels, inhibition of voltage-dependent Ca2+ channels and chelation of extracellular Ca2+. The [L21K], [L24K], [D20K, D27K] and [C31S,C37S] analogues were more potent but less effective than esculentin-2CHa whereas the [L28K] and [C31K] analogues were both more potent and produced a significantly (P < 0.001) greater maximum response. Acute administration of [L28K]esculentin-2CHa (75 nmol/kg body weight) to high fat fed mice with obesity and insulin resistance enhanced glucose tolerance and insulin secretion. Twice-daily administration of this dose of [L28K]esculentin-2CHa for 28 days had no significant effect on body weight, food intake, indirect calorimetry or body composition. However, mice exhibited decreased non-fasting plasma glucose (P < 0.05), increased non-fasting plasma insulin (P < 0.05) as well as improved glucose tolerance and insulin secretion (P < 0.01) following both oral and intraperitoneal glucose loads. Impaired responses of isolated islets from high fat fed mice to established insulin secretagogues were restored by [L28K]esculentin-2CHa treatment. Peptide treatment was accompanied by significantly lower plasma and pancreatic glucagon levels and normalization of α-cell mass. Circulating triglyceride concentrations were decreased but plasma cholesterol and LDL concentrations were not significantly affected. The data encourage further investigation of the potential of esculentin-2CHa related peptides for treatment of patients with type 2 diabetes.
Citation: Ojo OO, Srinivasan DK, Owolabi BO, Vasu S, Conlon JM, Flatt PR, et al. (2015) Esculentin-2CHa-Related Peptides Modulate Islet Cell Function and Improve Glucose Tolerance in Mice with Diet-Induced Obesity and Insulin Resistance. PLoS ONE 10(10): e0141549. https://doi.org/10.1371/journal.pone.0141549
Editor: Makoto Kanzaki, Tohoku University, JAPAN
Received: July 13, 2015; Accepted: October 10, 2015; Published: October 29, 2015
Copyright: © 2015 Ojo et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited
Data Availability: All relevant data are within the paper and its Supporting Information files.
Funding: Funding for this study was provided by a project grant from Diabetes UK (https://www.diabetes.org.uk, Grant Number 12/0004457) and an award of a University Vice Chancellor Research Studentship to DKS. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Introduction
Skin secretions of many species of Anura (frogs and toads) represent a valuable source of peptides with therapeutic potential. These peptides, whose primary function is believed to be host-defence, are best known for their antimicrobial properties and there are many examples of components with potent activity against multidrug-resistant pathogenic Gram-positive and Gram-negative bacteria and fungi (reviewed in [1–4]). However, frog skin host-defense peptides are multifunctional and may also display anti-tumor, antiviral, immunomodulatory, and chemoattractive activities (reviewed in [5]). In addition, myotropic peptides produced in the skin, such as those related to mammalian tachykinins, bradykinin and CCK-8, may play a role in deterring ingestion by predators [6]. There are no conserved structural domains in amphibian host-defense peptides that are responsible for biological activity but with few exceptions they are cationic and have the propensity to adopt an amphipathic, α-helical conformation in a membrane-mimetic solvent or in the environment of a phospholipid vesicle [2].
One such host-defense peptide with therapeutic potential is esculentin-2CHa (GFSSIFRGVAKFASKGLGKDLAKLGVDLVACKISKQC), first isolated from norepinephrine-stimulated skin secretions of the Chiricahua leopard frog Lithobates chiricahuensis (Ranidae) [7]. This compound shows potent broad-spectrum antimicrobial properties including activity against clinical isolates of multidrug-resistant strains of Staphylococcus aureus, Acinetobacter baumannii, and Stenotrophomonas maltophilia. The peptide also stimulates the release of the anti-inflammatory cytokine IL-10 by mouse lymphoid cells and displays high cytotoxic potency against human non-small cell lung adenocarcinoma A549 cells but relatively low hemolytic activity against human erythrocytes [8]. Interestingly, such actions on cytokine production by mouse lymphoid cells were also extended to TNF-alpha which may impact on beta cells [8]. Structure-activity studies indicate that removal of the either hydrophobic N-terminal hexapeptide (GFSSIF) or the cyclic C-terminal domain (CKISKQC) and replacement of the Cys31 and Cys37 residues by serine results in appreciable decreases in cytotoxicity against microorganisms and mammalian cells. In contrast, increasing cationicity by substitution of the Asp20 and Asp27 residues by L-Lysine resulted in a modest increase in potency against all microorganisms tested (up to 4-fold) [8].
The current pandemic of type 2 diabetes has necessitated a search for new types of therapeutic agents and naturally occurring incretin peptides that stimulate insulin release in response to high circulating glucose concentration are receiving increasing attention. Several long-acting analogues of the potent incretin GLP-1 are currently in clinical use [9]. A number of frog skin peptides that were first identified on the basis of their ability to inhibit the growth of microorganisms have subsequently been shown to possess the ability to release insulin from the BRIN-BD11 clonal β-cells and isolated mouse islets at low concentrations that are not cytotoxic to the cells and to improve glucose tolerance in mice following acute administration (reviewed in [5, 10]). The high fat fed mouse exhibits obesity, glucose intolerance and insulin resistance and so is a useful model for a preliminary investigation of the therapeutic potential of peptides in treatment of patients with type 2 diabetes [11]. More recently, it has been shown that twice daily treatment of high-fat fed mice for up to 28 days with tigerinin-1R [12], magainin-AM1 [13], and CPF-SE1 [14] results in an improvement in glucose tolerance, insulin sensitivity, and islet β-cell secretory responsiveness.
In the present study, the antidiabetic potential of esculentin-2CHa and selected analogues with increased cationicity (Table 1) was assessed in vitro using BRIN-BD11 cells and isolated mouse islets and in vivo in studies using the high fat fed mouse.
Materials and Methods
Peptide synthesis and purification
Synthetic esculentin-2CHa and its analogues (Table 1) were purchased in crude form GL Biochem Ltd (Shanghai, China) and purified to near homogeneity (> 98% pure) by reversed-phase HLPC on a (2.2 cm x 25 cm) Vydac 218TP1022 (C18) column equilibrated with acetonitrile/water/triflouroacetic acid (21.0/78.9/0.1 v/v) mobile phase at a flow rate of 6 ml/min. The concentration of acetonitrile in the eluting buffer was raised to 56% (v/v) over 60 min. The molecular masses of the peptides were confirmed using MALDI-TOF mass spectrometry.
In vitro insulin-releasing studies
In vitro insulin-releasing effects of esculentin-2CHa and its analogues were assessed using BRIN-BD11 rat clonal β-cells and mouse islets. In the first set of experiments, BRIN-BD11 cells were incubated with the peptides in the concentration range (1 pM– 3 μM) in Krebs-Ringer bicarbonate buffer containing 5.6 mM glucose for 20 min at 37°C as previously described [15–17]. Insulin-releasing effects were also assessed using buffer supplemented with 1.4 and 16.7mm glucose concentrations and with established modulators of insulin release as previously described [15–17]. In a second set of experiments, islets from NIH Swiss mice, isolated by collagenase digestion [18,19], were incubated with a range of concentrations of esculentin-2CHa or its analogues (0.1 nM– 1 μM) for 1 h in Krebs-Ringer bicarbonate (KRB) buffer supplemented with 1.4, 5.6 or 16.7 mM glucose. Following test incubations, aliquots of buffer were retrieved and stored at -20°C for measurement of insulin by radioimmunoassay [20]. In the experiments with BRIN-BD11 cells, the release of lactate dehydrogenase (LDH) was measured as an indicator of the integrity of the plasma membrane using commercially available CytoTox 96 non-radioactive cytotoxicity assay kit (Promega, Madison, WI, USA) according to the manufacturer’s recommended protocol.
Membrane potential studies and intracellular calcium ([Ca2+]i)
Effects of esculentin-2CHa (1 μM) and its analogues on membrane potential and [Ca2+]i in BRIN-BD11 cells over a period of 5 min were assessed using commercially available FLIPR membrane or calcium assay kit (Molecular Devices, USA) as previously described [15]. Data were captured using a Flexstation 3 microplate reader equipped with automatic fluid transfer unit (Molecular Devices, USA).
Laboratory animals
Male National Institutes of Health (NIH) Swiss mice (Harlan Ltd, UK) were housed separately in an air-conditioned room (22 ± 2°C) with relative humidity of 51 ± 5% and a 12-hour light: 12-hour dark cycle and maintained on a high fat diet containing 45% fat, 20% protein and 35% carbohydrate (total energy 19.5 kJ/g, Dietex International Ltd, Witham, UK) for 120 days. Mice maintained on standard rodent diet containing 10% fat, 30% protein and 60% carbohydrates (total energy 12.99 kJ/g) were used as controls. Both groups of animals were allowed food and water ad libitum. All animal experiments were carried out in accordance with the UK Animals (Scientific Procedures) Act 1986 and EU Directive 2010/63EU for animal experiments. The study was approved by University of Ulster Research Ethics Committee.
Acute in vivo studies
For acute in vivo studies, overnight fasted, high fat fed mice (n = 8) received an intraperitoneal injection of glucose alone (18 mmol/kg body weight) or in combination with esculentin-2CHa or its analogues (75 nmol/kg body weight). This peptide dose was selected on the basis of a pilot study that examined acute effects of different doses of esculentin-2CHa on glucose tolerance in lean mice. Blood samples were collected as described previously before injection and at times indicated in the Figures for the measurement of plasma glucose and insulin concentrations.
Longer-term in vivo studies
High-fat fed mice with clearly manifested features of obesity and hyperglycaemia received twice daily injections of either saline vehicle (0.9% (w/v) (high fat fed controls) or [L28K]esculentin-2CHa (75 nmol/kg body weight) for 28 days. This peptide was chosen based on its potent in vitro and acute in vivo actions. Mice (n = 8) fed standard rodent diet and injected with saline were used as lean controls. Energy intake, bodyweight, non-fasting blood glucose and plasma insulin concentrations were monitored every 72 h throughout the duration of the study. At the end of the 28 day treatment period, glucose tolerance (18 mmol/kg body weight, intraperitoneal or oral, overnight fasted) and insulin sensitivity (25 U/kg body weight) were assessed as previously described [12–14]. Indirect calorimetry and energy expenditure in treated and control mice were measured using the Comprehensive Laboratory Animal Monitoring System (CLAMS) metabolic chambers (Columbus Instruments, Columbus, OH, USA). Total body lean and fat mass, bone mineral density and bone mineral content were also measured using DXA scanning (Piximus Densitometer, USA) [21]. Improvement in beta cell function in [L28K]esculentin-2CHa-treated and control mice were evaluated from the insulin secretory responses of islets isolated from these animals to established insulin secretagogues and incretin hormones (16.7 mM glucose, 1 μM GLP-1, 1 μM GIP, 10 mM alanine, 10 mM arginine and 30 mM KCl). Changes in islet morphology were assessed using pancreatic tissues excised from mice treated with [L28K]esculentin-2CHa or saline for 28 days as previously described [12–14].
Biochemical measurements
Pancreatic tissues were homogenized in 20 mM Tris-HCl, 150 mM NaCl, 1 mM EDTA, 1 mM EGTA and 0.5% Triton X 100; pH 7.5 as previously described [14]. Blood samples (approximately 150 μl), collected from the cut tip of the tail vein of unanesthetized mice at intervals indicated in the Figures were used for blood glucose measurements and determination of plasma insulin as previously described [13,14]. Blood glucose was measured using a hand-held Ascencia Contour meter (Bayer Healthcare, UK). Plasma and pancreatic insulin were determined by radioimmunoassay [20]. Plasma and pancreatic glucagon contents were determined by ELISA using commercially available kit (Millipore, MA, USA). Plasma creatinine, alanine transaminase (ALT), aspartic acid transaminase (AST) and alkaline phosphatase (ALP) were measured using commercially available kits (Randox Laboratories, UK) as indicators of renal and liver function. Plasma triglyceride and cholesterol concentrations were measured using an automated clinical chemistry analyser (I-lab 650, and reagents purchased from Instrumentation Laboratory (Warrington, UK). The assay kit for cholesterol was obtained from Randox Laboratories (Antrim, UK). Estimation of LDL cholesterol concentrations was achieved using the Friedewald equation as described previously [22].
Statistical analysis
Results are expressed as mean ± S.E.M. Values were compared using one-way ANOVA followed by Student-Newman-Keuls post hoc test. Area under the curve (AUC) analysis was performed using the trapezoidal rule with baseline correction. P < 0.05 was considered statistically significant.
Results
In vitro insulin releasing effects
The basal rate of insulin secretion from BRIN BD11 cells at 5.6 mM glucose was about 5% of total insulin content of one million cells in 20 min. This was increased by 7.3-fold in the presence of alanine (10mM) (P<0.001; n = 8) (Fig 1A). Esculentin-2CHa produced a significant (P < 0.05) and concentration-dependent stimulation of insulin release at concentrations ≥ 0.03nM. At the highest concentration of 3μM, the peptide produced a near maximum 10.3-fold insulin-secretory response (P < 0.001). All analogues of esculentin-2CHa tested produced a significant (P < 0.05) and concentration-dependent stimulation of insulin release from BRIN-BD11 cells (Fig 1B). The threshold concentration (minimum concentration producing a significant increase in the rate of insulin release) of all analogues, except [D20K,D27K]esculentin-2CHa, was 0.01 nM. Stimulatory effects at 3 μM of [L28K]- and [C31S]-esculentin-2CHa were significantly (P < 0.05) greater than those of the native peptide and the other analogues (Table 2).
Values are mean ± SEM with n = 8. For A, B, D and F, *P < 0.05, **P < 0.01, ***P < 0.001 compared with 5.6mM glucose. For B and D, ΔP < 0.05, ΔΔP < 0.01 compared with native esculentin-2CHa. For C, *P < 0.05, **P < 0.01, ***P < 0.001 compared with 16.7 mM glucose. For E, *P < 0.05, **P < 0.01, ***P < 0.001 compared with the same concentration of glucose alone. ΔP<0.05 compared with esculentin-2CHa at the same glucose concentration. ++P < 0.01, +++P < 0.001 compared with incubation at 5.6 mM glucose for each peptide. For F, ΔΔΔP < 0.001 compared with respective incubation in the absence of the peptide. +P < 0.05, ++P < 0.01, +++P < 0.001 compared with incubation at 5.6 mM glucose in the presence of esculentin-2CHa alone.
The insulinotropic actions of esculentin-2CHa and its analogues were replicated in incubations performed with isolated mouse islets (Fig 1C and 1D). Basal insulin release from islets at 16.7 mM glucose was increased 2.4-fold by GLP-1 (10−6 M). A similar threshold concentration was observed for esculentin-2CHa and its [L21K], [L24K] and [D20K, D27K] analogues at 16.7 mM glucose (Table 2). However, other analogues stimulated insulin secretion from islets at concentrations ≥ 1 nM. The stimulation produced by the highest concentration of esculentin-2CHa (1 μM, 2.7-fold, P < 0.001) was comparable to the insulinotropic effect exhibited by the same concentration (1 μM) of its [L21K] (2.6-fold, P < 0.001), [C31S, C37S] (2.6-fold, P < 0.001) and [D20K,D27K] analogues (1.7-fold, P < 0.001) but was significantly (P < 0.05) higher that the effect observed for [L24K]-esculentin-2CHa (1 μM, 2.3-fold) under the same experimental conditions. The stimulatory effects of the [L28K] (1 μM, 3.4-fold, P < 0.001) and [L31K] (1 μM, 3.3-fold, P < 0.001) analogues on isolated islets were significantly higher when compared with the native peptide (Table 2).
The stimulatory effects of esculentin-2CHa (1 μM) and its substituted analogues on BRIN-BD11 cells increased progressively as the concentration of glucose in the incubation buffer was increased from 1.1 to 16.7mM (Fig 1E). However, the stimulatory action of esculentin-2CHa (Fig 1F) and its analogues were significantly inhibited by diazoxide (300 μM, 52–57%, P < 0.001), verapamil (50 μM, 31–35%, P < 0.001) and by the absence of extracellular calcium (49–55%, P<0.001). No significant release of lactate dehydrogenase (LDH) from BRIN-BD11 cells was observed following incubation with esculentin-2CHa or any analogue tested (Fig 1G).
Effects on membrane potential and intracellular Ca2+ concentration
Membrane potential of BRIN BD11 cells was increased by 5.2-fold (P < 0.001) in the presence of KCl (30 mM, Fig 2A and 2B). Esculentin-2CHa (1 μM) and its analogues also depolarized BRIN-BD11 cells, producing a 2.1-fold (P < 0.001) increase of membrane potential compared with 5.6mM glucose (Table 2). While alanine (10 mM) produced a marked increase (4.6-fold, P < 0.001) in the concentration of intracellular Ca2+, esculentin-2CHa and its analogues elicited only a modest response (1 μM, 1.5-fold, P < 0.05, Fig 2C and 2D, Table 2).
Cells were incubated with esculentin-2CHa (1 μM) or its substituted analogue and data were collected every 1.52 s over a period of 5 min. Values are mean ± SEM with n = 6. *P < 0.05, **P < 0.01, ***P < 0.001 compared with 5.6 mM glucose.
Acute in vivo effects on glucose tolerance and insulin release
Acute in vivo effects of esculentin-2CHa and its analogues were assessed in high fat mice with obesity-diabetes. Intraperitoneal administration of esculentin-2CHa (75 nmol/kg body weight) with glucose (18 mmol/kg body weight) significantly decreased the plasma glucose excursion compared with injection of glucose alone (Fig 3A). Integrated responses, presented as area under the glucose curve, showed that plasma glucose was 33% (P < 0.05) lower in mice injected with esculentin-2CHa (Fig 3B). This was accompanied by a 48% (P < 0.01, Fig 3C and 3D) increase in the integrated insulin response. The plasma glucose response was reduced by 4–52% (P ≤ 0.05) using different analogues of esculentin-2CHa, with the [L28K] and [C31K] peptides producing 52% (P < 0.01) and 40% (P < 0.05) decreases respectively (Table 3). A similar trend was observed for acute effects of the analogues on insulin secretion in high fat fed mice. Plasma insulin response was increased by 10–134% in mice treated with the [L28K] and [C31K] analogues producing stimulating responses that were 2.8- and 2.4-fold greater than that observed with esculentin-2CHa (Table 3).
Values are mean ± SEM with n = 8. *P < 0.05 compared with control
Effects of 28 day administration of [L28K]esculentin-2CHa on body weight, food intake and non-fasting plasma glucose and insulin concentrations
Based on its superior in vitro and acute in vivo effects, [L28K]esculentin-2CHa was selected for longer-term studies using high fat fed mice. These animals exhibited increased body weight, food intake, plasma glucose and insulin concentrations compared with control animals fed a standard diet (Fig 4). Treatment with [L28K]esculentin-2CHa for 28 days did not affect body weight or food intake but resulted in 25% (P < 0.05, Fig 4C) reduction in non-fasting plasma glucose and a 42% (P < 0.05, Fig 4D) increase in non-fasting plasma insulin compared with saline-treated controls.
Values are mean ± SEM with n = 8 mice. *P < 0.05, *** P < 0.001 compared to high fat fed control. All parameters were significantly lower in lean mice than high fat fed control mice (P < 0.05 –P < 0.001).
Effects of 28 day administration of [Lys28]esculentin-2CHa on glucose tolerance and insulin-sensitivity
Treatment of high fat fed mice with [L28K]esculentin-2CHa resulted in significant improvement of intraperitoneal glucose tolerance and glucose-stimulated insulin secretion (P < 0.05, Fig 5A–5D). Area under the curve values (AUC 0–60 min) for glucose and insulin concentrations showed an improvement of 20% (P < 0.05, Fig 5B) and 66% (P < 0.01, Fig 5D) respectively. Similarly, the glycaemic excursion following oral glucose (23%, P < 0.01, Fig 5E and 5F) and the accompanying insulin response (68%, P < 0.001, Fig 5G and 5H) were also improved in mice treated with [L28K]esculentin-2CHa. Treatment with the peptide had no significant effect on insulin sensitivity in high fat fed mice (Fig 5I and 5J).
Insulin sensitivity tests were performed using 25 U/kg body weight of insulin injected intraperitoneally. All tests were conducted following twice-daily treatment of mice with saline or [L28K]esculentin-2CHa (75 nmol/kg body weight) for 28 days. Values are mean ± SEM with n = 8 mice. *P < 0.05, **P < 0.01 and ***P < 0.001 compared with saline-treated lean mice. ΔP < 0.05, ΔΔP < 0.01 compared with high-fat fed control.
Effects of 28 day administration of [L28K]esculentin-2CHa on indirect calorimetry, energy expenditure and body composition in high fat fed mice
Oxygen (O2) consumption, CO2 production and energy expenditure in high fat fed mice increased by 30% (P < 0.001), 22% (P < 0.001) and 27% (P < 0.001) respectively but these parameters together with respiratory exchange ratio were not affected by treatment with [L28K]esculentin-2CHa (S1 Fig). Treatment with [L28K]esculentin-2CHa reversed the loss in bone area but did not affect body fat content and lean body mass in high fat fed mice (S2 Fig). However, saline-treated high fat fed mice exhibited significantly (P < 0.001) reduced bone area (13%, P < 0.001) and increased body fat (2.0-fold, P < 0.001) (S2 Fig) Bone mineral density and bone mineral content were similar in all groups of mice (S2 Fig).
Effects of 28 day administration of [L28K]esculentin-2CHa on pancreatic weight, insulin content and islets insulin secretory responses of isolated islets
Pancreatic weights were similar in all groups of mice (Fig 6A). However, the greater total pancreatic insulin content of high fat fed mice was reversed by treatment with [L28K]esculentin-2CHa (Fig 6B). Compared with lean control mice, secretory responses of islets isolated from high fat fed mice were significantly decreased to 1.4 (27%, P < 0.05), 5.6 (42%, P < 0.05) or 16.7 mM glucose (43%, P < 0.01), GLP-1 (1 μM, 42%, P < 0.05), GIP (1 μM, 40%, P < 0.05), alanine (10 mM, 45%, P < 0.05), arginine (10 mM, 41%, P < 0.05) and KCl (30 mM, 33%, P < 0.05). However, treatment with [L28K]esculentin-2CHa for 28 days restored the insulin-secretory responses to each of these secretagogues (Fig 6C and 6D).
For Fig 6B, ***P < 0.001 compared with lean control, ΔP < 0.01 compared with high-fat control. For Fig 6C, *P < 0.05,**P < 0.01, ***P < 0.001 compared with the response of islets isolated from the same group of mice at 16.7 mM glucose; ΔP < 0.05, ΔΔP < 0.01, ΔΔΔP < 0.001 compared with the respective response of islets isolated from lean control. For Fig 6D, stimulation index refers to fold-increase in insulin secretion from 1.4 mM glucose to 16.7 mM glucose or from 16.7 mM glucose to that observed in the presence of each secretagogue. *P < 0.05, **P < 0.01 compared with the stimulation index of islets isolated from each group of mice at 16.7mM glucose. ΔP < 0.05, ΔΔP < 0.01 compared the stimulation index of lean control.
Effects of 28 day administration of [L28K]esculentin-2CHa on pancreatic and plasma glucagon content, lipid profile and both renal and liver function
The elevated pancreatic and plasma glucagon levels generated by high fat feeding were reduced by 20% (P < 0.05) and 35% (P < 0.05) in [L28K]esculentin-2CHa-treated mice (Fig 7A and 7B). Plasma total cholesterol were similar in all groups while high fat fed mice exhibited reduced plasma HDL cholesterol (23%, P < 0.05) and elevated plasma triglycerides (1.2-fold, P < 0.05) (Fig 7C). Treatment with [L28K]esculentin-2CHa for 28 days had no effect on HDL cholesterol but significantly (P < 0.05) decreased plasma triglycerides. Plasma levels of AST and ALT were similar in all groups of mice, plasma ALP was decreased (43%, P < 0.01) and creatinine increased (140%, P < 0.001) in high fat fed mice compared with lean controls (Fig 7D and 7E). Administration of [L28K]esculentin-2CHa for 28 days resulted in 43% (P < 0.05, Fig 7D) increase in plasma ALP and 40% (P < 0.05, Fig 7E) decrease in plasma creatinine levels.
Mice were treated with twice-daily injections of saline or [L28K]esculentin-2CHa (75 nmol/kg body weight) for 28 days prior to measurement of biochemical parameters. Values are mean ± SEM with n = 8. *P < 0.05, **P < 0.01, ***P < 0.01 compared with lean control. ΔP < 0.05 compared with high-fat control.
Effects of 28 day administration of [L28K]esculentin-2CHa on islet morphology, beta cell and alpha cell area
Islets isolated from saline-treated high fat fed mice were significantly larger than those isolated from lean mice (Fig 8A). The number of islets per mm2 of pancreas as well as beta and alpha cells area were also significantly (P ≤ 0.05) increased in high fat fed mice (Fig 8B–8E). Treatment with [L28K]esculentin-2CHa did not affect the number of islets per mm2 of pancreas but significantly reduced total islet area (44%, P<0.001) as well as beta (43%, P < 0.001) and alpha (48%, P < 0.001) cell areas.
Mice were treated with twice-daily injections of saline or [L28K]esculentin-2CHa (75 nmol/kg body weight) for 28 days prior to excision of pancreatic tissue for immunohistological analysis. Values are mean ± SEM for 8 observations (~120 islets per group). *P < 0.05, **P < 0.01, ***P < 0.001 compared to lean control. ΔΔΔP < 0.001 compared to high fat control.
Discussion
The increasing incidence of type 2 diabetes together with ever mounting challenges posed by associated complications have motivated efforts to discover novel antidiabetic agents with better therapeutic outcomes [23]. The present study provides further evidence for the potentially beneficial actions of the esculentin-2CHa family of peptides and highlights their possible utility in the management of type 2 diabetes. Consistent with observations using several other amphibian host defence peptides [10], esculentin-2CHa stimulates insulin release from BRIN-BD11 cells in a dose-dependent and glucose-responsive manner at concentrations that are non-toxic to the cells. However, magnitude of the effects of the peptide, particularly at the highest concentration tested (3 μM), were appreciably greater than those previously reported for other amphibian host-defence peptides [9]. Indeed, the stimulatory effect of esculetin-2CHa on isolated mouse islets is comparable in magnitude to that of GLP-1 under the same experimental conditions [24,25]. Membrane depolarization and enhanced intracellular Ca2+ concentrations together with the reduced insulin release in the presence of diazoxide, verapamil or Ca2+ chelation suggest that the insulinotropic action of esculentin-2CHa, in common with other but not all previously identified insulinotropic amphibian skin peptides [5,10], may involve the activation of the KATP-dependent pathway of insulin secretion [26]. This is fully supported by initial patch clam experiments evaluating effects of [Arg4]tigerinin-1R in clonal BRIN-BD11 beta cells (R. C. Moffett et al., unpublished observations). This analogue derived from tigerinin-1R isolated from the skin secretions of Hoplobatrachus rugulosus has similar action prolife to esculentin-2CHa. However, effects on other elements of beta cell signal transduction pathways such as glucose metabolism (glycolysis or mitochondrial metabolism), intracellular cyclic AMP generation or activation of phospholipase C should not be ruled out. Indeed, insulin secretion was largely preserved in the presence of diazoxide or verapamil, as well as under Ca2+ free conditions, indicating that almost half of the insulin secretory response induced by esculentin-2CHa is dependent neither on KATP channel closure nor L-type Ca2+ channel activation.
We have demonstrated previously in studies using the amphibian peptides pseudin-2 [15], B2RP [27], alyteserin-2a [28] and tigerinin-1R [29] that site-specific amino acid substitutions that result in increasing cationicity may lead to significant enhancement of their in vitro insulin releasing actions. In this study, such amino acid substitutions resulted in increased net charge and isoelectric point (Table 1) as well as enhanced insulinotropic potency. However, the responses to a 3μM stimulus of all analogues of esculentin-2CHa tested, except the [L28K] and [C31K] peptides, were lower compared with the native peptide.
Consistent with previous studies [11], mice fed a high fat diet exhibited glucose intolerance and insulin resistance. Acute injection with esculentin-2CHa significantly improved both oral and intraperitoneal glucose tolerance and increased insulin secretion. These in vivo actions were greater with the [D28K] and [C31S] analogues while the in vitro insulinotropic actions of the other peptide analogues were not replicated in vivo. The in vivo effects of [L28K] and [C31K]esculentin-2CHa in these animals were more pronounced than those previously reported for other amphibian skin peptides [12–14,30]. Twice-daily administration of [L28K]esculentin-2CHa for 28 days did not affect body weight and food intake but reduced hyperglycaemia and elevated plasma insulin concentrations in the non-fasting state. This was associated with improved glucose tolerance following oral and intraperitoneal glucose administration accompanied by enhanced insulin secretion. These observations are broadly consistent with effects of tigerinin-1R [12], [I10W]-tigerinin-1R [30] and magainin-AM2 [13], suggesting a possible similar spectrum of actions in this animal model of obesity and diabetes. We have previously shown that the antidiabetic effects of magainin-AM2 [13] and [I10W]-tigerinin-1R [30] were accompanied by improvement in insulin sensitivity. However, in the present study, the insulin resistance induced by high fat feeding was not alleviated in mice treated with [L28K]esculentin-2CHa. It is probable, therefore, that the improvement of glucose homeostasis observed in this study is largely due the effects of the peptide on islet cell function. Consistent with this view, the reduced insulin-secretory responses to incretin hormones and other insulin secretagogues observed with islets isolated from saline treated high fat fed mice were reversed by treatment with [L28K]esculentin-2CHa.
Unrestrained hepatic glucose output and elevated glucagon secretion make an important contribution to the development of hyperglycaemia in type 2 diabetes [31]. Interesting, the elevation of pancreatic and plasma glucagon concentrations as well as α-cell area in saline-treated high fat fed mice were normalized by treatment with [L28K]esculentin-2CHa. Although the exact molecular mechanism through which the peptide inhibits α-cell function is not yet known, our results suggest that such effects contribute to the improvement of hyperglycaemia and glucose tolerance. Thus, further studies are required to assess whether [L28K]esculentin-2CHa acts directly on β cells or by indirect effects mediated via enteroendocrine secretions such as GLP-1. Increased islet size accompanying enhanced insulin output and defective β-cell function caused by high fat feeding were also reversed in [L28K]esculentin-2CHa-treated mice. Our preliminary work with analogues of the parent peptide indicate that this may be due to correction of the ratio of beta cell proliferation to apoptosis.
Energy metabolism was not affected by treatment with [L28K]esculentin-2CHa. Similarly, the peptide did not affect adipose tissue deposition, bone mineral content or bone mineral density in high fat fed mice. Bone area and lean body mass were increased in [L28K]esculentin-2CHa-treated mice, but this did not translate to changes in overall body weight. Further studies are required to evaluate long-term impact of [L28K]esculentin-2Cha on circulating cytokines and insulin signalling pathways. Importantly, no adverse effects were observed in mice treated with the peptide, including unchanged circulating concentrations of AST, ALT and ALP together with improved creatinine clearance and lower circulating triglycerides. Although longer term toxicological studies are obviously needed, these observations suggest both benefits and lack of toxicity of [L28K]esculentin-2CHa.
Conclusions
In conclusion, this study has demonstrated the beneficial effects of esculentin-2CHa family of peptides in mice with diet-induced obesity-diabetes. [L28K]esculentin-2CHa exhibited better in vitro insulinotropic potential compared with the native peptide and significantly improved glucose tolerance and enhanced insulin secretion by positive effects on beta cell function in high fat fed mice. These observations together with the previous demonstrated antimicrobial actions [8] encourage further evaluation of the potential of [L28K]esculentin-2CHa as a novel agent for managing patients with type 2 diabetes and associated microbial infections.
Supporting Information
S1 Fig. Effects of [L28K]esculentin-2CHa on O2 consumption (A, B), CO2 production (C, D), respiratory exchange ratio (E, F) and energy expenditure (G, H) in lean and high-fat fed treated with saline or [L28K]esculentin-2CHa (75nmol/kg bw) for 28 days.
Mice were placed in CLAMS metabolic chambers, and O2 consumption or CO2 production were measured for 30s at 15min intervals. RER was calculated by dividing VCO2 by VO2. Energy expenditure was computed using the formula (3.815 + 1.232 x RER) x VO2. Values are means ± SEM for 6 mice. **P<0.01, ***P<0.001 compared with saline-treated lean mice. Shaded bar indicates dark phase.
https://doi.org/10.1371/journal.pone.0141549.s001
(TIF)
S2 Fig. Effects of [L28K]esculentin-2CHa on body composition in normal or high-fat fed mice.
Mice were treated with twice-daily injections of saline or [Lys28]esculentin-2CHa (75nmol/kg body weight) for 28 days prior to DEXA scan (A) and computation of data on lean body mass (B), body fat (C, D), bone mineral density (E), bone mineral content (F) and bone area (G). Values are means ± SEM for 8 mice. *P<0.05, **P<0.01, ***P<0.001compared with lean control. ΔΔΔP<0.01 compared with high fat control.
https://doi.org/10.1371/journal.pone.0141549.s002
(TIF)
Acknowledgments
Funding for this study was provided by a project grant from Diabetes UK (Grant Number 12/0004457) and an award of a University Vice Chancellor Research Studentship to DKS.
Author Contributions
Conceived and designed the experiments: YHAA PRF JMC OOO. Performed the experiments: OOO DKS BOO SV. Analyzed the data: OOO DKS BOO SV. Contributed reagents/materials/analysis tools: JMC YHAA PRF. Wrote the paper: OOO JMC PRF.
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