Your search keyword '"Glucagon-Secreting Cells metabolism"' showing total 32 results

1. Enhanced quantification of α-cell suppression by hyperglycemia using a high-sensitivity glucagon assay.

Author

Dyer RB, Laurenti MC, Christie HE, Mohan S, Egan AM, Dalla Man C, and Vella A

Subjects

Humans, Male, Immunoassay methods, Glucose metabolism, Female, Adult, Diabetes Mellitus, Type 2 metabolism, Middle Aged, Blood Glucose metabolism, Glucagon metabolism, Glucagon blood, Glucagon-Secreting Cells metabolism, Hyperglycemia metabolism

Abstract

Accurate measurement of glucagon concentrations in a variety of conditions is necessary for subsequent estimation of glucagon secretion. Glucagon arises in the α-cell as a product of proglucagon processing. Modern two-site immunoassays have overcome prior problems with glucagon measurement caused by cross-reactivity with other proglucagon-derived fragments. However, in response to hyperglycemia, glucagon concentrations can fall below the limit of quantification of commercial immunoassays. This has implications for the characterization of α-cell function in health, in prediabetes, and in type 2 diabetes. An increase in the sensitivity of glucagon measurement was achieved by ethanol precipitation and concentration of the sample before measurement. Concentrating the sample sixfold enabled a decrease in the level of quantitation from 1.7 to 0.3 pmol/L with acceptable precision. To establish whether this enhanced high-sensitivity glucagon assay enhances the characterization of α-cell function in health and disease, we then estimated glucagon secretion rate (GSR) in four subjects. We subsequently used the relationship of GSR to glucose concentrations to characterize the α-cell response to glucose and demonstrate improved characterization of α-cell dysfunction in vivo. NEW & NOTEWORTHY We describe a method that lowers the limit of quantification of a glucagon immunoassay thereby enhancing the ability to differentiate between normal and abnormal α-cell responsiveness to glucagon.

Published

2025

2. Evaluating glucose-dependent insulinotropic polypeptide and glucagon as key regulators of insulin secretion in the pancreatic islet.

Author

Lewandowski SL, El K, and Campbell JE

Subjects

Animals, Humans, Glucagon-Like Peptide 1 metabolism, Glucagon-Secreting Cells metabolism, Incretins metabolism, Insulin metabolism, Insulin-Secreting Cells metabolism, Gastric Inhibitory Polypeptide metabolism, Glucagon metabolism, Insulin Secretion physiology, Islets of Langerhans metabolism, Islets of Langerhans drug effects

Abstract

The incretin axis is an essential component of postprandial insulin secretion and glucose homeostasis. There are two incretin hormones, glucagon-like peptide 1 (GLP-1) and glucose-dependent insulinotropic polypeptide (GIP), which exert multiple actions throughout the body. A key cellular target for the incretins are pancreatic β-cells, where they potentiate nutrient-stimulated insulin secretion. This feature of incretins has made this system an attractive target for therapeutic interventions aimed at controlling glycemia. Here, we discuss the role of GIP in both β-cells and α-cells within the islet, to stimulate insulin and glucagon secretion, respectively. Moreover, we discuss how glucagon secretion from α-cells has important insulinotropic actions in β-cells through an axis termed α- to β-cell communication. These recent advances have elevated the potential of GIP and glucagon as a therapeutic targets, coinciding with emerging compounds that pharmacologically leverage the actions of these two peptides in the context of diabetes and obesity.

Published

2024

3. Zinc-chelating BET bromodomain inhibitors equally target islet endocrine cell types.

Author

Jones Lipinski RA, Stancill JS, Nuñez R, Wynia-Smith SL, Sprague DJ, Nord JA, Bird A, Corbett JA, and Smith BC

Subjects

Animals, Humans, Male, Mice, Azepines pharmacology, Azepines chemistry, Glucagon-Secreting Cells drug effects, Glucagon-Secreting Cells metabolism, Mice, Inbred C57BL, Nuclear Proteins, Transcription Factors metabolism, Transcription Factors antagonists & inhibitors, Triazoles pharmacology, Triazoles chemistry, Bromodomain Containing Proteins antagonists & inhibitors, Bromodomain Containing Proteins chemistry, Chelating Agents pharmacology, Insulin-Secreting Cells drug effects, Insulin-Secreting Cells metabolism, Zinc chemistry, Zinc pharmacology, Zinc metabolism

Abstract

Inhibition of the bromodomain and extraterminal domain (BET) protein family is a potential strategy to prevent and treat diabetes; however, the clinical use of BET bromodomain inhibitors (BETis) is associated with adverse effects. Here, we explore a strategy for targeting BETis to β cells by exploiting the high-zinc (Zn 2+ ) concentration in β cells relative to other cell types. We report the synthesis of a novel, Zn 2+ -chelating derivative of the pan-BETi (+)-JQ1, (+)-JQ1-DPA, in which (+)-JQ1 was conjugated to dipicolyl amine (DPA). As controls, we synthesized (+)-JQ1-DBA, a non-Zn 2+ -chelating derivative, and (-)-JQ1-DPA, an inactive enantiomer that chelates Zn 2+ . Molecular modeling and biophysical assays showed that (+)-JQ1-DPA and (+)-JQ1-DBA retain potent binding to BET bromodomains in vitro. Cellular assays demonstrated (+)-JQ1-DPA attenuated NF-ĸB target gene expression in β cells stimulated with the proinflammatory cytokine interleukin 1β. To assess β-cell selectivity, we isolated islets from a mouse model that expresses green fluorescent protein in insulin-positive β cells and mTomato in insulin-negative cells (non-β cells). Surprisingly, Zn 2+ chelation did not confer β-cell selectivity as (+)-JQ1-DPA was equally effective in both β and α cells; however, (+)-JQ1-DPA was less effective in macrophages, a nonendocrine islet cell type. Intriguingly, the non-Zn 2+ -chelating derivative (+)-JQ1-DBA displayed the opposite selectivity, with greater effect in macrophages compared with (+)-JQ1-DPA, suggesting potential as a macrophage-targeting molecule. These findings suggest that Zn 2+ -chelating small molecules confer endocrine cell selectivity rather than β-cell selectivity in pancreatic islets and provide valuable insights and techniques to assess Zn 2+ chelation as an approach to selectively target small molecules to pancreatic β cells. NEW & NOTEWORTHY Inhibition of BET bromodomains is a novel potential strategy to prevent and treat diabetes mellitus. However, BET inhibitors have negative side effects. We synthesized a BET inhibitor expected to exploit the high zinc concentration in β cells to accumulate in β cells. We show our inhibitor targeted pancreatic endocrine cells; however, it was less effective in immune cells. A control inhibitor showed the opposite effect. These findings help us understand how to target specific cells in diabetes treatment.

Published

2024

4. Unveiling cell subpopulations in T1D mouse islets using single-cell RNA sequencing.

Author

Yang H, Luo J, Liu X, Luo Y, Lai X, and Zou F

Subjects

Animals, Mice, Diabetes Mellitus, Experimental genetics, Diabetes Mellitus, Experimental pathology, Glucagon-Secreting Cells metabolism, Female, RNA-Seq methods, Mice, Inbred C57BL, Diabetes Mellitus, Type 1 genetics, Single-Cell Analysis methods, Islets of Langerhans metabolism, Islets of Langerhans cytology, Insulin-Secreting Cells metabolism, Sequence Analysis, RNA methods

Abstract

Type 1 diabetes (T1D) is an autoimmune disease characterized by the destruction of beta cells by immune cells. The interactions among cells within the islets may be closely linked to the pathogenesis of T1D. In this study, we used single-cell RNA sequencing (scRNA-Seq) to analyze the cellular heterogeneity within the islets of a T1D mouse model. We established a T1D mouse model induced by streptozotocin and identified cell subpopulations using scRNA-Seq technology. Our results revealed 11 major cell types in the pancreatic islets of T1D mice, with heterogeneity observed in the alpha and beta cell subgroups, which may play a crucial role in the progression of T1D. Flow cytometry further confirmed a mature alpha and beta cell reduction in T1D mice. Overall, our scRNA-Seq analysis provided insights into the cellular heterogeneity of T1D islet tissue and highlighted the potential importance of alpha and beta cells in developing T1D. NEW & NOTEWORTHY In this study, we created a comprehensive single-cell atlas of pancreatic islets in a T1D mouse model using scRNA-Seq and identified 11 major cell types in the islets, highlighting the role of alpha and beta cells in T1D. This study revealed a significant reduction in the maturity alpha and beta cells in T1D mice through flow cytometry. It also demonstrated the heterogeneity of alpha and beta cells, potentially crucial for T1D progression. Overall, our scRNA-Seq analysis provided new insights for understanding and treating T1D by studying cell subtype changes and functions.

Published

2024

5. The role of preproglucagon peptides in regulating β-cell morphology and responses to streptozotocin-induced diabetes.

Author

Arble DM, Hutch CR, Hafner H, Stelmak D, Leix K, Sorrell J, Pressler JW, Gregg B, and Sandoval DA

Subjects

Mice, Animals, Proglucagon genetics, Proglucagon metabolism, Streptozocin, Insulin metabolism, Glucose pharmacology, Mice, Knockout, Blood Glucose metabolism, Diabetes Mellitus, Experimental metabolism, Hyperglycemia, Glucagon-Secreting Cells metabolism

Abstract

Insulin secretion from β-cells is tightly regulated by local signaling from preproglucagon ( Gcg ) products from neighboring α-cells. Physiological paracrine signaling within the microenvironment of the β-cell is altered after metabolic stress, such as high-fat diet or the β-cell toxin, streptozotocin (STZ). Here, we examined the role and source of Gcg peptides in β-cell function and in response to STZ-induced hyperglycemia. We used whole body Gcg null (Gcg Null ) mice and mice with Gcg expression either specifically within the pancreas (Gcg ΔPanc ) or the intestine (Gcg ΔIntest ). With lower doses of STZ exposure, insulin levels were greater and glucose levels were lower in Gcg Null mice compared with wild-type mice. When Gcg was functional only in the intestine, plasma glucagon-like peptide-1 (GLP-1) levels were fully restored but these mice did not have any additional protection from STZ-induced diabetes. Pancreatic Gcg reactivation normalized the hyperglycemic response to STZ. In animals not treated with STZ, Gcg Null mice had increased pancreas mass via both α- and β-cell hyperplasia and reactivation of Gcg in the intestine normalized β- but not α-cell mass, whereas pancreatic reactivation normalized both β- and α-cell mass. Gcg Null and Gcg ΔIntest mice maintained higher β-cell mass after treatment with STZ compared with control and Gcg ΔPanc mice. Although in vivo insulin response to glucose was normal, global lack of Gcg impaired glucose-stimulated insulin secretion in isolated islets. Congenital replacement of Gcg either in the pancreas or intestine normalized glucose-stimulated insulin secretion. Interestingly, mice that had intestinal Gcg reactivated in adulthood had impaired insulin response to KCl. We surmise that the expansion of β-cell mass in the Gcg Null mice compensated for decreased individual β-cell insulin secretion, which is sufficient to normalize glucose under physiological conditions and conferred some protection after STZ-induced diabetes. NEW & NOTEWORTHY We examined the role of Gcg on β-cell function under normal and high glucose conditions. GcgNull mice had decreased glucose-stimulated insulin secretion, increased β-cell mass, and partial protection against STZ-induced hyperglycemia. Expression of Gcg within the pancreas normalized these endpoints. Intestinal expression of Gcg only normalized β-cell mass and glucose-stimulated insulin secretion. Increased β-cell mass in GcgNull mice likely compensated for decreased insulin secretion normalizing physiological glucose levels and conferring some protection after STZ-induced diabetes.

Published

2023

6. Human pancreatic capillaries and nerve fibers persist in type 1 diabetes despite beta cell loss.

Author

Richardson TM, Saunders DC, Haliyur R, Shrestha S, Cartailler JP, Reinert RB, Petronglo J, Bottino R, Aramandla R, Bradley AM, Jenkins R, Phillips S, Kang H, Caicedo A, Powers AC, and Brissova M

Subjects

Humans, Mice, Animals, Glucagon metabolism, Capillaries metabolism, Nerve Fibers metabolism, Diabetes Mellitus, Type 1 metabolism, Islets of Langerhans metabolism, Glucagon-Secreting Cells metabolism, Diabetes Mellitus, Type 2 metabolism

Abstract

The autonomic nervous system regulates pancreatic function. Islet capillaries are essential for the extension of axonal projections into islets, and both of these structures are important for appropriate islet hormone secretion. Because beta cells provide important paracrine cues for islet glucagon secretion and neurovascular development, we postulated that beta cell loss in type 1 diabetes (T1D) would lead to a decline in intraislet capillaries and reduction of islet innervation, possibly contributing to abnormal glucagon secretion. To define morphological characteristics of capillaries and nerve fibers in islets and acinar tissue compartments, we analyzed neurovascular assembly across the largest cohort of T1D and normal individuals studied thus far. Because innervation has been studied extensively in rodent models of T1D, we also compared the neurovascular architecture between mouse and human pancreas and assembled transcriptomic profiles of molecules guiding islet angiogenesis and neuronal development. We found striking interspecies differences in islet neurovascular assembly but relatively modest differences at transcriptome level, suggesting that posttranscriptional regulation may be involved in this process. To determine whether islet neurovascular arrangement is altered after beta cell loss in T1D, we compared pancreatic tissues from non-diabetic, recent-onset T1D (<10-yr duration), and longstanding T1D (>10-yr duration) donors. Recent-onset T1D showed greater islet and acinar capillary density compared to non-diabetic and longstanding T1D donors. Both recent-onset and longstanding T1D had greater islet nerve fiber density compared to non-diabetic donors. We did not detect changes in sympathetic axons in either T1D cohort. Additionally, nerve fibers overlapped with extracellular matrix (ECM), supporting its role in the formation and function of axonal processes. These results indicate that pancreatic capillaries and nerve fibers persist in T1D despite beta cell loss, suggesting that alpha cell secretory changes may be decoupled from neurovascular components. NEW & NOTEWORTHY Defining the neurovascular architecture in the pancreas of individuals with type 1 diabetes (T1D) is crucial to understanding the mechanisms of dysregulated glucagon secretion. In the largest T1D cohort of biobanked tissues analyzed to date, we found that pancreatic capillaries and nerve fibers persist in human T1D despite beta cell loss, suggesting that alpha cell secretory changes may be decoupled from neurovascular components. Because innervation has been studied extensively in rodent T1D models, our studies also provide the first rigorous direct comparisons of neurovascular assembly in mouse and human, indicating dramatic interspecies differences.

Published

2023

7. Arginine-induced glucagon secretion and glucagon-induced enhancement of amino acid catabolism are not influenced by ambient glucose levels in mice.

Author

Maruszczak K, Rasmussen C, Ceutz FR, Ørgaard A, Elmelund E, Richter MM, Holst JJ, Winther-Sørensen M, and Wewer Albrechtsen NJ

Subjects

Amino Acids biosynthesis, Animals, Glucose metabolism, Insulin, Mice, Urea, Arginine metabolism, Blood Glucose, Glucagon metabolism, Glucagon-Secreting Cells metabolism

Abstract

Amino acids stimulate the secretion of glucagon, and glucagon receptor signaling regulates amino acid catabolism via ureagenesis, together constituting the liver-α cell axis. Impairment of the liver-α cell axis is observed in metabolic diseases such as diabetes. It is, however, unknown whether glucose affects the liver-α cell axis. We investigated the role of glucose on the liver-α cell axis in vivo and ex vivo. The isolated perfused mouse pancreas was used to evaluate the direct effect of low (3.5 mmol/L) and high (15 mmol/L) glucose levels on amino acid (10 mmol/L arginine)-induced glucagon secretion. High glucose levels alone lowered glucagon secretion, but the amino acid-induced glucagon responses were similar in high and low glucose conditions ( P = 0.38). The direct effect of glucose on glucagon and amino acid-induced ureagenesis was assessed using isolated perfused mouse livers stimulated with a mixture of amino acids (Vamin R , 10 mmol/L) and glucagon (10 nmol/L) during high and low glucose conditions. Urea production increased robustly but was independent of glucose levels ( P = 0.95). To investigate the whole body effects of glucose on the liver-α cell axis, four groups of mice received intraperitoneal injections of glucose-Vamin (2 g/kg, + 3.5 µmol/g, respectively, G/V), saline-Vamin (S/V), glucose-saline (G/S), or saline-saline (S/S). Blood glucose did not differ significantly between G/S and G/V groups. Levels of glucagon and amino acids were similar in the G/V and S/V groups ( P = 0.28). Amino acids may overrule the inhibitory effect of glucose on glucagon secretion and the liver-α cell axis may operate independently of glucose in mice. NEW & NOTEWORTHY Glucagon is an essential regulator of our metabolism. Recent evidence suggests that the physiological actions of glucagon reside in amino acid catabolism in the so-called liver-α cell axis, in which amino acids stimulate glucagon secretion and glucagon enhances hepatic amino acid catabolism. Here, it is demonstrated that this feedback system is independent of glycemia possibly explaining why hyperglycemia in diabetes may not suppress α cell secretion.

Published

2022

8. Alanine, arginine, cysteine, and proline, but not glutamine, are substrates for, and acute mediators of, the liver-α-cell axis in female mice.

Author

Galsgaard KD, Jepsen SL, Kjeldsen SAS, Pedersen J, Wewer Albrechtsen NJ, and Holst JJ

Subjects

Alanine metabolism, Animals, Arginine metabolism, Cysteine metabolism, Female, Glucagon-Secreting Cells drug effects, Glutamine metabolism, In Vitro Techniques, Insulin metabolism, Mice, Proline metabolism, Receptors, Glucagon antagonists & inhibitors, Receptors, Glucagon metabolism, Amino Acids metabolism, Blood Glucose metabolism, Glucagon metabolism, Glucagon-Secreting Cells metabolism, Liver metabolism

Abstract

The aim of this study was to identify the amino acids that stimulate glucagon secretion in mice and whose metabolism depends on glucagon receptor signaling. Pancreata of female C57BL/6JRj mice were perfused with 19 individual amino acids and pyruvate (at 10 mM), and secretion of glucagon was assessed using a specific glucagon radioimmunoassay. Separately, a glucagon receptor antagonist (GRA; 25-2648, 100 mg/kg) or vehicle was administered to female C57BL/6JRj mice 3 h before an intraperitoneal injection of four different isomolar amino acid mixtures (in total 7 µmol/g body wt) as follows: mixture 1 contained alanine, arginine, cysteine, and proline; mixture 2 contained aspartate, glutamate, histidine, and lysine; mixture 3 contained citrulline, methionine, serine, and threonine; and mixture 4 contained glutamine, leucine, isoleucine, and valine. Blood glucose, plasma glucagon, amino acid, and insulin concentrations were measured using well-characterized methodologies. Alanine ( P = 0.03), arginine ( P < 0.0001), cysteine ( P = 0.01), glycine ( P = 0.02), lysine ( P = 0.02), and proline ( P = 0.03), but not glutamine ( P = 0.9), stimulated glucagon secretion from the perfused mouse pancreas. However, when the four isomolar amino acid mixtures were administered in vivo, the four mixtures elicited similar glucagon responses ( P > 0.5). Plasma concentrations of total amino acids in vivo were higher after administration of GRA when mixture 1 ( P = 0.004) or mixture 3 ( P = 0.04) were injected. Our data suggest that alanine, arginine, cysteine, and proline, but not glutamine, are involved in the acute regulation of the liver-α-cell axis in female mice, as they all increased glucagon secretion and their disappearance rate was altered by GRA.

Published

2020

9. Glucose-mediated inhibition of calcium-activated potassium channels limits α-cell calcium influx and glucagon secretion.

Author

Dickerson MT, Dadi PK, Altman MK, Verlage KR, Thorson AS, Jordan KL, Vierra NC, Amarnath G, and Jacobson DA

Subjects

Alkanes pharmacology, Animals, Apamin pharmacology, Calcium Channels, L-Type metabolism, Calcium Channels, P-Type metabolism, Calcium Channels, Q-Type metabolism, Endoplasmic Reticulum metabolism, Mice, Mice, Transgenic, Patch-Clamp Techniques, Peptides pharmacology, Potassium Channel Blockers pharmacology, Potassium Channels, Calcium-Activated antagonists & inhibitors, Pyrazoles pharmacology, Quinolinium Compounds pharmacology, Calcium metabolism, Calcium Channels metabolism, Glucagon metabolism, Glucagon-Secreting Cells metabolism, Glucose metabolism, Potassium Channels, Calcium-Activated metabolism

Abstract

Pancreatic α-cells exhibit oscillations in cytosolic Ca 2+ (Ca 2+ c ), which control pulsatile glucagon (GCG) secretion. However, the mechanisms that modulate α-cell Ca 2+ c oscillations have not been elucidated. As β-cell Ca 2+ c oscillations are regulated in part by Ca 2+ -activated K + (K slow ) currents, this work investigated the role of K slow in α-cell Ca 2+ handling and GCG secretion. α-Cells displayed K slow currents that were dependent on Ca 2+ influx through L- and P/Q-type voltage-dependent Ca 2+ channels (VDCCs) as well as Ca 2+ released from endoplasmic reticulum stores. α-Cell K slow was decreased by small-conductance Ca 2+ -activated K + (SK) channel inhibitors apamin and UCL 1684, large-conductance Ca 2+ -activated K + (BK) channel inhibitor iberiotoxin (IbTx), and intermediate-conductance Ca 2+ -activated K + (IK) channel inhibitor TRAM 34. Moreover, partial inhibition of α-cell K slow with apamin depolarized membrane potential ( V m ) (3.8 ± 0.7 mV) and reduced action potential (AP) amplitude (10.4 ± 1.9 mV). Although apamin transiently increased Ca 2+ influx into α-cells at low glucose (42.9 ± 10.6%), sustained SK (38.5 ± 10.4%) or BK channel inhibition (31.0 ± 11.7%) decreased α-cell Ca 2+ influx. Total α-cell Ca 2+ c was similarly reduced (28.3 ± 11.1%) following prolonged treatment with high glucose, but it was not decreased further by SK or BK channel inhibition. Consistent with reduced α-cell Ca 2+ c following prolonged K slow inhibition, apamin decreased GCG secretion from mouse (20.4 ± 4.2%) and human (27.7 ± 13.1%) islets at low glucose. These data demonstrate that K slow activation provides a hyperpolarizing influence on α-cell V m that sustains Ca 2+ entry during hypoglycemic conditions, presumably by preventing voltage-dependent inactivation of P/Q-type VDCCs. Thus, when α-cell Ca 2+ c is elevated during secretagogue stimulation, K slow activation helps to preserve GCG secretion.

Published

2019

10. Hyperglucagonemia correlates with plasma levels of non-branched-chain amino acids in patients with liver disease independent of type 2 diabetes.

Author

Wewer Albrechtsen NJ, Junker AE, Christensen M, Hædersdal S, Wibrand F, Lund AM, Galsgaard KD, Holst JJ, Knop FK, and Vilsbøll T

Subjects

Adult, Aged, Biomarkers blood, Body Mass Index, Case-Control Studies, Cholesterol blood, Diabetes Mellitus, Type 2 diagnosis, Diabetes Mellitus, Type 2 physiopathology, Fasting blood, Female, Glycated Hemoglobin metabolism, Humans, Liver pathology, Male, Middle Aged, Non-alcoholic Fatty Liver Disease diagnosis, Non-alcoholic Fatty Liver Disease physiopathology, Up-Regulation, Amino Acids blood, Diabetes Mellitus, Type 2 blood, Glucagon blood, Glucagon-Secreting Cells metabolism, Insulin Resistance, Liver metabolism, Non-alcoholic Fatty Liver Disease blood

Abstract

Patients with type 2 diabetes (T2D) and patients with nonalcoholic fatty liver disease (NAFLD) frequently exhibit elevated plasma concentrations of glucagon (hyperglucagonemia). Hyperglucagonemia and α-cell hyperplasia may result from elevated levels of plasma amino acids when glucagon's action on hepatic amino acid metabolism is disrupted. We therefore measured plasma levels of glucagon and individual amino acids in patients with and without biopsy-verified NAFLD and with and without type T2D. Fasting levels of amino acids and glucagon in plasma were measured, using validated ELISAs and high-performance liquid chromatography, in obese, middle-aged individuals with I) normal glucose tolerance (NGT) and NAFLD, II) T2D and NAFLD, III) T2D without liver disease, and IV) NGT and no liver disease. Elevated levels of total amino acids were observed in participants with NAFLD and NGT compared with NGT controls (1,310 ± 235 µM vs. 937 ± 281 µM, P = 0.03) and in T2D and NAFLD compared with T2D without liver disease (1,354 ± 329 µM vs. 511 ± 235 µM, P < 0.0001). Particularly amino acids with known glucagonotropic effects (e.g., glutamine) were increased. Plasma levels of total amino acids correlated to plasma levels of glucagon also when adjusting for body mass index (BMI), glycated hemoglobin (Hb A1c ), and cholesterol levels (β = 0.013 ± 0.007, P = 0.024). Elevated plasma levels of total amino acids associate with hyperglucagonemia in NAFLD patients independently of glycemic control, BMI or cholesterol - supporting the potential importance of a "liver-α-cell axis" in which glucagon regulates hepatic amino acid metabolism. Fasting hyperglucagonemia as seen in T2D may therefore represent impaired hepatic glucagon action with increasing amino acids levels. NEW & NOTEWORTHY Hypersecretion of glucagon (hyperglucagonemia) has been suggested to be linked to type 2 diabetes. Here, we show that levels of amino acids correlate with levels of glucagon. Hyperglucagonemia may depend on hepatic steatosis rather than type 2 diabetes.

Published

2018

11. Dynamics of glucagon secretion in mice and rats revealed using a validated sandwich ELISA for small sample volumes.

Author

Wewer Albrechtsen NJ, Kuhre RE, Windeløv JA, Ørgaard A, Deacon CF, Kissow H, Hartmann B, and Holst JJ

Subjects

Anesthetics, Dissociative pharmacology, Animals, Arginine pharmacology, Chromatography, Gel, Enzyme-Linked Immunosorbent Assay, Female, Glucagon analysis, Glucagon drug effects, Glucagon-Secreting Cells drug effects, Glucose pharmacology, Hypnotics and Sedatives pharmacology, Ketamine pharmacology, Male, Mannitol pharmacology, Mice, Mice, Inbred C57BL, Rats, Rats, Wistar, Sweetening Agents pharmacology, Xylazine pharmacology, Glucagon metabolism, Glucagon-Secreting Cells metabolism

Abstract

Glucagon is a metabolically important hormone, but many aspects of its physiology remain obscure, because glucagon secretion is difficult to measure in mice and rats due to methodological inadequacies. Here, we introduce and validate a low-volume, enzyme-linked immunosorbent glucagon assay according to current analytical guidelines, including tests of sensitivity, specificity, and accuracy, and compare it, using the Bland-Altman algorithm and size-exclusion chromatography, with three other widely cited assays. After demonstrating adequate performance of the assay, we measured glucagon secretion in response to intravenous glucose and arginine in anesthetized mice (isoflurane) and rats (Hypnorm/midazolam). Glucose caused a long-lasting suppression to very low values (1-2 pmol/l) within 2 min in both species. Arginine stimulated secretion 8- to 10-fold in both species, peaking at 1-2 min and returning to basal levels at 6 min (mice) and 12 min (rats). d-Mannitol (osmotic control) was without effect. Ketamine/xylazine anesthesia in mice strongly attenuated (P < 0.01) α-cell responses. Chromatography of pooled plasma samples confirmed the accuracy of the assay. In conclusion, dynamic analysis of glucagon secretion in rats and mice with the novel accurate sandwich enzyme-linked immunosorbent assay revealed extremely rapid and short-lived responses to arginine and rapid and profound suppression by glucose., (Copyright © 2016 the American Physiological Society.)

Published

2016

12. Paracrine regulation of glucagon secretion: the β/α/δ model.

Author

Watts M, Ha J, Kimchi O, and Sherman A

Subjects

Humans, Models, Theoretical, Paracrine Communication, Calcium metabolism, Glucagon metabolism, Glucagon-Secreting Cells metabolism, Glucose metabolism, Insulin metabolism, Insulin-Secreting Cells metabolism, Somatostatin metabolism, Somatostatin-Secreting Cells metabolism

Abstract

The regulation of glucagon secretion in the pancreatic α-cell is not well understood. It has been proposed that glucose suppresses glucagon secretion either directly through an intrinsic mechanism within the α-cell or indirectly through an extrinsic mechanism. Previously, we described a mathematical model for isolated pancreatic α-cells and used it to investigate possible intrinsic mechanisms of regulating glucagon secretion. We demonstrated that glucose can suppress glucagon secretion through both ATP-dependent potassium channels (K ATP ) and a store-operated current (SOC). We have now developed an islet model that combines previously published mathematical models of α- and β-cells with a new model of δ-cells and use it to explore the effects of insulin and somatostatin on glucagon secretion. We show that the model can reproduce experimental observations that the inhibitory effect of glucose remains even when paracrine modulators are no longer acting on the α-cell. We demonstrate how paracrine interactions can either synchronize α- and δ-cells to produce pulsatile oscillations in glucagon and somatostatin secretion or fail to do so. The model can also account for the paradoxical observation that glucagon can be out of phase with insulin, whereas α-cell calcium is in phase with insulin. We conclude that both paracrine interactions and the α-cell's intrinsic mechanisms are needed to explain the response of glucagon secretion to glucose.

Published

2016

13. Short-term sleep deprivation with nocturnal light exposure alters time-dependent glucagon-like peptide-1 and insulin secretion in male volunteers.

Author

Gil-Lozano M, Hunter PM, Behan LA, Gladanac B, Casper RF, and Brubaker PL

Subjects

Adolescent, Adult, CLOCK Proteins genetics, Cells, Cultured, Circadian Rhythm physiology, Glucagon-Secreting Cells radiation effects, Healthy Volunteers, Humans, Insulin Secretion, Insulin-Secreting Cells radiation effects, Light, Male, Metabolic Networks and Pathways genetics, Metabolic Networks and Pathways radiation effects, Time Factors, Young Adult, Glucagon-Like Peptide 1 metabolism, Glucagon-Secreting Cells metabolism, Insulin metabolism, Insulin-Secreting Cells metabolism, Sleep Deprivation metabolism

Abstract

The intestinal L cell is the principal source of glucagon-like peptide-1 (GLP-1), a major determinant of insulin release. Because GLP-1 secretion is regulated in a circadian manner in rodents, we investigated whether the activity of the human L cell is also time sensitive. Rhythmic fluctuations in the mRNA levels of canonical clock genes were found in the human NCI-H716 L cell model, which also showed a time-dependent pattern in their response to well-established secretagogues. A diurnal variation in GLP-1 responses to identical meals (850 kcal), served 12 h apart in the normal dark (2300) and light (1100) periods, was also observed in male volunteers maintained under standard sleep and light conditions. These findings suggest the existence of a daily pattern of activity in the human L cell. Moreover, we separately tested the short-term effects of sleep deprivation and nocturnal light exposure on basal and postprandial GLP-1, insulin, and glucose levels in the same volunteers. Sleep deprivation with nocturnal light exposure disrupted the melatonin and cortisol profiles and increased insulin resistance. Moreover, it also induced profound derangements in GLP-1 and insulin responses such that postprandial GLP-1 and insulin levels were markedly elevated and the normal variation in GLP-1 responses was abrogated. These alterations were not observed in sleep-deprived participants maintained under dark conditions, indicating a direct effect of light on the mechanisms that regulate glucose homeostasis. Accordingly, the metabolic abnormalities known to occur in shift workers may be related to the effects of irregular light-dark cycles on these glucoregulatory pathways., (Copyright © 2016 the American Physiological Society.)

Published

2016

14. Physiology of proglucagon peptides: role of glucagon and GLP-1 in health and disease.

Author

Sandoval DA and D'Alessio DA

Subjects

Animals, Diabetes Mellitus metabolism, Diabetes Mellitus physiopathology, Enteroendocrine Cells metabolism, Gene Expression Regulation, Glucagon genetics, Glucagon-Like Peptide 1 genetics, Glucagon-Secreting Cells metabolism, Homeostasis, Humans, Blood Glucose metabolism, Energy Metabolism, Glucagon metabolism, Glucagon-Like Peptide 1 metabolism, Signal Transduction

Abstract

The preproglucagon gene (Gcg) is expressed by specific enteroendocrine cells (L-cells) of the intestinal mucosa, pancreatic islet α-cells, and a discrete set of neurons within the nucleus of the solitary tract. Gcg encodes multiple peptides including glucagon, glucagon-like peptide-1, glucagon-like peptide-2, oxyntomodulin, and glicentin. Of these, glucagon and GLP-1 have received the most attention because of important roles in glucose metabolism, involvement in diabetes and other disorders, and application to therapeutics. The generally accepted model is that GLP-1 improves glucose homeostasis indirectly via stimulation of nutrient-induced insulin release and by reducing glucagon secretion. Yet the body of literature surrounding GLP-1 physiology reveals an incompletely understood and complex system that includes peripheral and central GLP-1 actions to regulate energy and glucose homeostasis. On the other hand, glucagon is established principally as a counterregulatory hormone, increasing in response to physiological challenges that threaten adequate blood glucose levels and driving glucose production to restore euglycemia. However, there also exists a potential role for glucagon in regulating energy expenditure that has recently been suggested in pharmacological studies. It is also becoming apparent that there is cross-talk between the proglucagon derived-peptides, e.g., GLP-1 inhibits glucagon secretion, and some additive or synergistic pharmacological interaction between GLP-1 and glucagon, e.g., dual glucagon/GLP-1 agonists cause more weight loss than single agonists. In this review, we discuss the physiological functions of both glucagon and GLP-1 by comparing and contrasting how these peptides function, variably in concert and opposition, to regulate glucose and energy homeostasis., (Copyright © 2015 the American Physiological Society.)

Published

2015

15. Somatostatin and insulin mediate glucose-inhibited glucagon secretion in the pancreatic α-cell by lowering cAMP.

Author

Elliott AD, Ustione A, and Piston DW

Subjects

Animals, Cyclic AMP analysis, Cyclic AMP metabolism, Cyclic AMP-Dependent Protein Kinases metabolism, Flow Cytometry, Humans, Islets of Langerhans cytology, Male, Mice, Mice, Inbred C57BL, Microscopy, Confocal, Signal Transduction physiology, Glucagon metabolism, Glucagon-Secreting Cells metabolism, Glucose metabolism, Insulin metabolism, Islets of Langerhans metabolism, Somatostatin pharmacology

Abstract

The dysregulation of glucose-inhibited glucagon secretion from the pancreatic islet α-cell is a critical component of diabetes pathology and metabolic disease. We show a previously uncharacterized [Ca(2+)]i-independent mechanism of glucagon suppression in human and murine pancreatic islets whereby cAMP and PKA signaling are decreased. This decrease is driven by the combination of somatostatin, which inhibits adenylyl cyclase production of cAMP via the Gαi subunit of the SSTR2, and insulin, which acts via its receptor to activate phosphodiesterase 3B and degrade cytosolic cAMP. Our data indicate that both somatostatin and insulin signaling are required to suppress cAMP/PKA and glucagon secretion from both human and murine α-cells, and the combination of these two signaling mechanisms is sufficient to reduce glucagon secretion from isolated α-cells as well as islets. Thus, we conclude that somatostatin and insulin together are critical paracrine mediators of glucose-inhibited glucagon secretion and function by lowering cAMP/PKA signaling with increasing glucose., (Copyright © 2015 the American Physiological Society.)

Published

2015

16. Interleukin-6 amplifies glucagon secretion: coordinated control via the brain and pancreas.

Author

Barnes TM, Otero YF, Elliott AD, Locke AD, Malabanan CM, Coldren AG, Brissova M, Piston DW, and McGuinness OP

Subjects

Animals, Brain drug effects, Epinephrine pharmacology, Glucagon drug effects, Glucose Clamp Technique, Hypoglycemia metabolism, Interleukin-6 metabolism, Islets of Langerhans metabolism, Lipopolysaccharides pharmacology, Mice, Mice, Inbred C57BL, Mice, Knockout, Stress, Physiological, Sympathomimetics pharmacology, Brain metabolism, Glucagon metabolism, Glucagon-Secreting Cells metabolism, Interleukin-6 genetics

Abstract

Inappropriate glucagon secretion contributes to hyperglycemia in inflammatory disease. Previous work implicates the proinflammatory cytokine interleukin-6 (IL-6) in glucagon secretion. IL-6-KO mice have a blunted glucagon response to lipopolysaccharide (LPS) that is restored by intravenous replacement of IL-6. Given that IL-6 has previously been demonstrated to have a transcriptional (i.e., slow) effect on glucagon secretion from islets, we hypothesized that the rapid increase in glucagon following LPS occurred by a faster mechanism, such as by action within the brain. Using chronically catheterized conscious mice, we have demonstrated that central IL-6 stimulates glucagon secretion uniquely in the presence of an accompanying stressor (hypoglycemia or LPS). Contrary to our hypothesis, however, we found that IL-6 amplifies glucagon secretion in two ways; IL-6 not only stimulates glucagon secretion via the brain but also by direct action on islets. Interestingly, IL-6 augments glucagon secretion from both sites only in the presence of an accompanying stressor (such as epinephrine). Given that both adrenergic tone and plasma IL-6 are elevated in multiple inflammatory diseases, the interactions of the IL-6 and catecholaminergic signaling pathways in regulating GCG secretion may contribute to our present understanding of these diseases., (Copyright © 2014 the American Physiological Society.)

Published

2014

17. Composition and function of macroencapsulated human embryonic stem cell-derived implants: comparison with clinical human islet cell grafts.

Author

Motté E, Szepessy E, Suenens K, Stangé G, Bomans M, Jacobs-Tulleneers-Thevissen D, Ling Z, Kroon E, and Pipeleers D

Subjects

Animals, C-Peptide blood, C-Peptide metabolism, Cell Differentiation, Cell Line, Cells, Immobilized cytology, Cells, Immobilized metabolism, Crosses, Genetic, Diabetes Mellitus, Type 1 blood, Diabetes Mellitus, Type 1 metabolism, Diabetes Mellitus, Type 1 pathology, Embryonic Stem Cells cytology, Embryonic Stem Cells metabolism, Glucagon-Secreting Cells cytology, Glucagon-Secreting Cells metabolism, Humans, Insulin-Secreting Cells cytology, Insulin-Secreting Cells metabolism, Kidney, Membranes, Mice, Inbred NOD, Mice, SCID, Proinsulin blood, Proinsulin metabolism, Subcutaneous Tissue, Tissue Scaffolds adverse effects, Cells, Immobilized transplantation, Diabetes Mellitus, Type 1 surgery, Embryonic Stem Cells transplantation, Implants, Experimental adverse effects, Islets of Langerhans Transplantation adverse effects, Transplantation, Heterologous adverse effects, Transplantation, Heterotopic adverse effects

Abstract

β-Cells generated from large-scale sources can overcome current shortages in clinical islet cell grafts provided that they adequately respond to metabolic variations. Pancreatic (non)endocrine cells can develop from human embryonic stem (huES) cells following in vitro derivation to pancreatic endoderm (PE) that is subsequently implanted in immune-incompetent mice for further differentiation. Encapsulation of PE increases the proportion of endocrine cells in subcutaneous implants, with enrichment in β-cells when they are placed in TheraCyte-macrodevices and predominantly α-cells when they are alginate-microencapsulated. At posttransplant (PT) weeks 20-30, macroencapsulated huES implants presented higher glucose-responsive plasma C-peptide levels and a lower proinsulin-over-C-peptide ratio than human islet cell implants under the kidney capsule. Their ex vivo analysis showed the presence of single-hormone-positive α- and β-cells that exhibited rapid secretory responses to increasing and decreasing glucose concentrations, similar to isolated human islet cells. However, their insulin secretory amplitude was lower, which was attributed in part to a lower cellular hormone content; it was associated with a lower glucose-induced insulin biosynthesis, but not with lower glucagon-induced stimulation, which together is compatible with an immature functional state of the huES-derived β-cells at PT weeks 20-30. These data support the therapeutic potential of macroencapsulated huES implants but indicate the need for further functional analysis. Their comparison with clinical-grade human islet cell grafts sets references for future development and clinical translation., (Copyright © 2014 the American Physiological Society.)

Published

2014

18. Neuronostatin inhibits glucose-stimulated insulin secretion via direct action on the pancreatic α-cell.

Author

Salvatori AS, Elrick MM, Samson WK, Corbett JA, and Yosten GL

Subjects

Animals, Area Under Curve, Blood Glucose metabolism, Blotting, Western, Bradykinin pharmacology, Cell Line, Cyclic AMP metabolism, Cyclic AMP-Dependent Protein Kinases metabolism, Electrophoresis, Polyacrylamide Gel, Glucagon-Secreting Cells drug effects, Injections, Intraperitoneal, Inositol 1,4,5-Trisphosphate metabolism, Insulin blood, Islets of Langerhans drug effects, Islets of Langerhans metabolism, Male, Peptide Fragments administration & dosage, Rats, Rats, Sprague-Dawley, Real-Time Polymerase Chain Reaction, Somatostatin administration & dosage, Glucagon-Secreting Cells metabolism, Glucose antagonists & inhibitors, Glucose pharmacology, Insulin metabolism, Peptide Fragments pharmacology, Somatostatin pharmacology

Abstract

Neuronostatin is a recently described peptide hormone encoded by the somatostatin gene. We previously showed that intraperitoneal injection of neuronostatin into mice resulted in c-Jun accumulation in pancreatic islets in a pattern consistent with the activation of glucagon-producing α-cells. We therefore hypothesized that neuronostatin could influence glucose homeostasis via a direct effect on the α-cell. Neuronostatin enhanced low-glucose-induced glucagon release in isolated rat islets and in the immortalized α-cell line αTC1-9. Furthermore, incubation with neuronostatin led to an increase in transcription of glucagon mRNA, as determined by RT-PCR. Neuronostatin also inhibited glucose-stimulated insulin secretion from isolated islets. However, neuronostatin did not alter insulin release from the β-cell line INS 832/13, indicating that the effect of neuronostatin on insulin secretion may be secondary to a direct action on the α-cell. In agreement with our in vitro data, intra-arterial infusion of neuronostatin in male rats delayed glucose disposal and inhibited insulin release during a glucose challenge. These studies suggest that neuronostatin participates in maintaining glucose homeostasis through cell-cell interactions between α-cells and β-cells in the endocrine pancreas, leading to attenuation in insulin secretion., (Copyright © 2014 the American Physiological Society.)

Published

2014

19. Partial ablation of leptin signaling in mouse pancreatic α-cells does not alter either glucose or lipid homeostasis.

Author

Tudurí E, Denroche HC, Kara JA, Asadi A, Fox JK, and Kieffer TJ

Subjects

Animals, Cells, Cultured, Diabetes Mellitus, Experimental drug therapy, Diabetes Mellitus, Experimental genetics, Diabetes Mellitus, Experimental metabolism, Diabetes Mellitus, Type 1 drug therapy, Diabetes Mellitus, Type 1 genetics, Diabetes Mellitus, Type 1 metabolism, Female, Homeostasis genetics, Leptin therapeutic use, Mice, Mice, Inbred C57BL, Mice, Transgenic, Receptors, Leptin metabolism, Signal Transduction genetics, Gene Deletion, Glucagon-Secreting Cells metabolism, Glucose metabolism, Leptin metabolism, Lipid Metabolism genetics, Receptors, Leptin genetics

Abstract

The role of glucagon in the pathological condition of diabetes is gaining interest, and it has been recently reported that its action is essential for hyperglycemia to occur. Glucagon levels, which are elevated in some diabetic models, are reduced following leptin therapy. Likewise, hyperglycemia is corrected in type 1 diabetic mice treated with leptin, although the mechanisms have not been fully determined. A direct inhibitory effect of leptin on mouse and human α-cells has been demonstrated at the levels of electrical activity, calcium signaling, and glucagon secretion. In the present study we employed the Cre-loxP strategy to generate Lepr(flox/flox) Gcg-cre mice, which specifically lack leptin receptors in glucagon-secreting α-cells, to determine whether leptin resistance in α-cells contributes to hyperglucagonemia, and also whether leptin action in α-cells is required to improve glycemia in type 1 diabetes with leptin therapy. Immunohistochemical analysis of pancreas sections revealed Cre-mediated recombination in ∼ 43% of the α-cells. We observed that in vivo Lepr(flox/flox) Gcg-cre mice display normal glucose and lipid homeostasis. In addition, leptin administration in streptozotocin-induced diabetic Lepr(flox/flox) Gcg-cre mice restored euglycemia similarly to control mice. These findings suggest that loss of leptin receptor signaling in close to one-half of α-cells does not alter glucose metabolism in vivo, nor is it sufficient to prevent the therapeutic action of leptin in type 1 diabetes.

Published

2014

20. Long-term ketogenic diet causes glucose intolerance and reduced β- and α-cell mass but no weight loss in mice.

Author

Ellenbroek JH, van Dijck L, Töns HA, Rabelink TJ, Carlotti F, Ballieux BE, and de Koning EJ

Subjects

Animals, Biomarkers blood, Chemokine CCL2 blood, Diet, Carbohydrate-Restricted adverse effects, Glucagon-Secreting Cells metabolism, Glucose Intolerance metabolism, Glucose Intolerance pathology, Inflammation blood, Insulin blood, Insulin-Secreting Cells metabolism, Interleukin-1beta blood, Interleukin-6 blood, Mice, Triglycerides blood, Diet, Ketogenic adverse effects, Glucagon-Secreting Cells pathology, Glucose Intolerance etiology, Insulin-Secreting Cells pathology, Weight Loss

Abstract

High-fat, low-carbohydrate ketogenic diets (KD) are used for weight loss and for treatment of refractory epilepsy. Recently, short-time studies in rodents have shown that, besides their beneficial effect on body weight, KD lead to glucose intolerance and insulin resistance. However, the long-term effects on pancreatic endocrine cells are unknown. In this study we investigate the effects of long-term KD on glucose tolerance and β- and α-cell mass in mice. Despite an initial weight loss, KD did not result in weight loss after 22 wk. Plasma markers associated with dyslipidemia and inflammation (cholesterol, triglycerides, leptin, monocyte chemotactic protein-1, IL-1β, and IL-6) were increased, and KD-fed mice showed signs of hepatic steatosis after 22 wk of diet. Long-term KD resulted in glucose intolerance that was associated with insufficient insulin secretion from β-cells. After 22 wk, insulin-stimulated glucose uptake was reduced. A reduction in β-cell mass was observed in KD-fed mice together with an increased number of smaller islets. Also α-cell mass was markedly decreased, resulting in a lower α- to β-cell ratio. Our data show that long-term KD causes dyslipidemia, a proinflammatory state, signs of hepatic steatosis, glucose intolerance, and a reduction in β- and α-cell mass, but no weight loss. This indicates that long-term high-fat, low-carbohydrate KD lead to features that are also associated with the metabolic syndrome and an increased risk for type 2 diabetes in humans.

Published

2014

21. Increased amino acid supply potentiates glucose-stimulated insulin secretion but does not increase β-cell mass in fetal sheep.

Author

Gadhia MM, Maliszewski AM, O'Meara MC, Thorn SR, Lavezzi JR, Limesand SW, Hay WW Jr, Brown LD, and Rozance PJ

Subjects

Amino Acids administration & dosage, Amino Acids, Branched-Chain administration & dosage, Amino Acids, Branched-Chain metabolism, Animals, Animals, Inbred Strains, Arginine administration & dosage, Arginine metabolism, Electrolytes administration & dosage, Female, Fetal Weight, Glucagon blood, Glucagon metabolism, Glucagon-Secreting Cells cytology, Glucagon-Secreting Cells metabolism, Glucose administration & dosage, Infusions, Intravenous, Insulin blood, Insulin Resistance, Insulin Secretion, Insulin-Secreting Cells cytology, Organ Size, Pancreas blood supply, Pancreas cytology, Pancreas metabolism, Pregnancy, Random Allocation, Sheep, Domestic, Solutions administration & dosage, Amino Acids metabolism, Glucose metabolism, Insulin metabolism, Insulin-Secreting Cells metabolism, Pancreas embryology

Abstract

Amino acids and glucose acutely stimulate fetal insulin secretion. In isolated adult pancreatic islets, amino acids potentiate glucose-stimulated insulin secretion (GSIS), but whether amino acids have this same effect in the fetus is unknown. Therefore, we tested the effects of increased fetal amino acid supply on GSIS and morphology of the pancreas. We hypothesized that increasing fetal amino acid supply would potentiate GSIS. Singleton fetal sheep received a direct intravenous infusion of an amino acid mixture (AA) or saline (CON) for 10-14 days during late gestation to target a 25-50% increase in fetal branched-chain amino acids (BCAA). Early-phase GSIS increased 150% in the AA group (P < 0.01), and this difference was sustained for the duration of the hyperglycemic clamp (105 min) (P < 0.05). Glucose-potentiated arginine-stimulated insulin secretion (ASIS), pancreatic insulin content, and pancreatic glucagon content were similar between groups. β-Cell mass and area were unchanged between groups. Baseline and arginine-stimulated glucagon concentrations were increased in the AA group (P < 0.05). Pancreatic α-cell mass and area were unchanged. Fetal and pancreatic weights were similar. We conclude that a sustained increase of amino acid supply to the normally growing late-gestation fetus potentiated fetal GSIS but did not affect the morphology or insulin content of the pancreas. We speculate that increased β-cell responsiveness (insulin secretion) following increased amino acid supply may be due to increased generation of secondary messengers in the β-cell. This may be enhanced by the paracrine action of glucagon on the β-cell.

Published

2013

22. Glucose metabolism is altered after loss of L cells and α-cells but not influenced by loss of K cells.

Author

Pedersen J, Ugleholdt RK, Jørgensen SM, Windeløv JA, Grunddal KV, Schwartz TW, Füchtbauer EM, Poulsen SS, Holst PJ, and Holst JJ

Subjects

Animals, Apoptosis genetics, Apoptosis physiology, Diphtheria Toxin genetics, Enteroendocrine Cells classification, Enteroendocrine Cells metabolism, Female, Gastric Inhibitory Polypeptide metabolism, Gene Knockdown Techniques, Genes, Transgenic, Suicide genetics, Glucagon-Secreting Cells metabolism, Male, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Mice, Transgenic, Organ Specificity genetics, Enteroendocrine Cells physiology, Glucagon-Secreting Cells physiology, Glucose metabolism

Abstract

The enteroendocrine K and L cells are responsible for secretion of glucose-dependent insulinotropic polypeptide (GIP) and glucagon like-peptide 1 (GLP-1), whereas pancreatic α-cells are responsible for secretion of glucagon. In rodents and humans, dysregulation of the secretion of GIP, GLP-1, and glucagon is associated with impaired regulation of metabolism. This study evaluates the consequences of acute removal of Gip- or Gcg-expressing cells on glucose metabolism. Generation of the two diphtheria toxin receptor cellular knockout mice, TgN(GIP.DTR) and TgN(GCG.DTR), allowed us to study effects of acute ablation of K and L cells and α-cells. Diphtheria toxin administration reduced the expression of Gip and content of GIP in the proximal jejunum in TgN(GIP.DTR) and expression of Gcg and content of proglucagon-derived peptides in both proximal jejunum and terminal ileum as well as content of glucagon in pancreas in TgN(GCG.DTR) compared with wild-type mice. GIP response to oral glucose was attenuated following K cell loss, but oral and intraperitoneal glucose tolerances were unaffected. Intraperitoneal glucose tolerance was impaired following combined L cell and α-cell loss and normal following α-cell loss. Oral glucose tolerance was improved following L cell and α-cell loss and supernormal following α-cell loss. We present two mouse models that allow studies of the effects of K cell or L cell and α-cell loss as well as isolated α-cell loss. Our findings show that intraperitoneal glucose tolerance is dependent on an intact L cell mass and underscore the diabetogenic effects of α-cell signaling. Furthermore, the results suggest that K cells are less involved in acute regulation of mouse glucose metabolism than L cells and α-cells.

Published

2013

23. SSTR2 is the functionally dominant somatostatin receptor in human pancreatic β- and α-cells.

Author

Kailey B, van de Bunt M, Cheley S, Johnson PR, MacDonald PE, Gloyn AL, Rorsman P, and Braun M

Subjects

Calcium Signaling drug effects, Cells, Cultured, Exocytosis drug effects, G Protein-Coupled Inwardly-Rectifying Potassium Channels antagonists & inhibitors, G Protein-Coupled Inwardly-Rectifying Potassium Channels genetics, G Protein-Coupled Inwardly-Rectifying Potassium Channels metabolism, Gene Expression Regulation, Glucagon-Secreting Cells cytology, Glucagon-Secreting Cells drug effects, Humans, Immunohistochemistry, Insulin-Secreting Cells cytology, Insulin-Secreting Cells drug effects, Islets of Langerhans cytology, Islets of Langerhans drug effects, Islets of Langerhans metabolism, Kinetics, Membrane Potentials drug effects, Patch-Clamp Techniques, Potassium Channel Blockers pharmacology, Protein Isoforms agonists, Protein Isoforms genetics, Protein Isoforms metabolism, Protein Subunits genetics, Protein Subunits metabolism, RNA, Messenger metabolism, Receptors, Somatostatin agonists, Receptors, Somatostatin genetics, Recombinant Proteins agonists, Recombinant Proteins metabolism, Somatostatin agonists, Glucagon-Secreting Cells metabolism, Insulin-Secreting Cells metabolism, Receptors, Somatostatin metabolism, Somatostatin metabolism

Abstract

Somatostatin-14 (SST) inhibits insulin and glucagon secretion by activating G protein-coupled somatostatin receptors (SSTRs), of which five isoforms exist (SSTR1-5). In mice, the effects on pancreatic β-cells are mediated by SSTR5, whereas α-cells express SSTR2. In both cell types, SSTR activation results in membrane hyperpolarization and suppression of exocytosis. Here, we examined the mechanisms by which SST inhibits secretion from human β- and α-cells and the SSTR isoforms mediating these effects. Quantitative PCR revealed high expression of SSTR2, with lower levels of SSTR1, SSTR3, and SSTR5, in human islets. Immunohistochemistry showed expression of SSTR2 in both β- and α-cells. SST application hyperpolarized human β-cells and inhibited action potential firing. The membrane hyperpolarization was unaffected by tolbutamide but antagonized by tertiapin-Q, a blocker of G protein-gated inwardly rectifying K⁺ channels (GIRK). The effect of SST was mimicked by an SSTR2-selective agonist, whereas a SSTR5 agonist was marginally effective. SST strongly (>70%) reduced depolarization-evoked exocytosis in both β- and α-cells. A slightly weaker inhibition was observed in both cell types after SSTR2 activation. SSTR3- and SSTR1-selective agonists moderately reduced the exocytotic responses in β- and α-cells, respectively, whereas SSTR4- and SSTR5-specific agonists were ineffective. SST also reduced voltage-gated P/Q-type Ca²⁺ currents in β-cells, but normalization of Ca²⁺ influx to control levels by prolonged depolarizations only partially restored exocytosis. We conclude that SST inhibits secretion from both human β- and α-cells by activating GIRK and suppressing electrical activity, reducing P/Q-type Ca²⁺ currents, and directly inhibiting exocytosis. These effects are mediated predominantly by SSTR2 in both cell types.

Published

2012

24. Evidence for an interaction of neuronostatin with the orphan G protein-coupled receptor, GPR107.

Author

Yosten GL, Redlinger LJ, and Samson WK

Subjects

Animals, Blood Pressure drug effects, Blood Pressure physiology, Cardiovascular Physiological Phenomena, Cell Line, Cell Line, Tumor, Cells, Cultured, Glucagon-Secreting Cells metabolism, Glucagon-Secreting Cells pathology, Humans, Hypothalamus metabolism, Hypothalamus pathology, Male, Mice, Myocardium metabolism, Myocardium pathology, RNA, Small Interfering pharmacology, Rats, Stomach Neoplasms metabolism, Stomach Neoplasms pathology, Peptide Fragments metabolism, Peptide Hormones metabolism, Receptors, G-Protein-Coupled metabolism, Somatostatin metabolism

Abstract

Neuronostatin, derived from the somatostatin preprohormone, is a recently described peptide that is produced by several tissues involved in cardiovascular regulation and metabolism, including the hypothalamus. Injection of neuronostatin into the lateral cerebroventricle led to a dose-related increase in mean arterial pressure (MAP) in rats. Any attempt to inhibit the production of neuronostatin would alter somatostatin production as well, making determination of the physiological relevance of the peptide's pharmacologic effects by compromise of production approaches impossible. Therefore, we employed an alternative approach to identify and compromise the production of the neuronostatin receptor. Because neuronostatin was shown to signal via a PKA-dependent mechanism, we hypothesized that the neuronostatin receptor was a G protein-coupled receptor (GPCR), in particular, one of the orphan GPCRs for which the ligand is unknown. Therefore, we screened neuronostatin-responsive tissues, including hypothalamus, heart, pancreatic α-cells, and the gastric tumor cell line KATOIII, for expression of orphan GPCRs. Four orphan GPCRs were expressed by all cell types, including GPR56 and GPR107. Knockdown of GPR107, but not GPR56 or GPR146, led to a loss of responsiveness to neuronostatin by KATOIII cells. Rats injected with siRNA directed against GPR107 (2 μg/day for 2 days) into the lateral cerebroventricle did not exhibit an increase in MAP in response to neuronostatin treatment. Rats with compromised GPR107 expression also displayed blunted reactivity in a baroreflex sensitivity test, indicating that GPR107 and neuronostatin may be important regulators of cardiovascular function. Thus, GPR107 is a promising candidate receptor for neuronostatin, and neuronostatin, interacting with GPR107, may play an important role in the central control of cardiovascular function.

Published

2012

25. Activin B regulates islet composition and islet mass but not whole body glucose homeostasis or insulin sensitivity.

Author

Bonomi L, Brown M, Ungerleider N, Muse M, Matzuk MM, and Schneyer A

Subjects

Activins genetics, Aging blood, Animals, Blood Glucose analysis, Cell Count, Follistatin metabolism, Glucagon-Secreting Cells cytology, Glucagon-Secreting Cells metabolism, Inhibin-beta Subunits genetics, Insulin blood, Insulin Secretion, Islets of Langerhans metabolism, Male, Mice, Mice, 129 Strain, Mice, Inbred C57BL, Mice, Knockout, Myostatin metabolism, Organ Size, Tissue Culture Techniques, Activins metabolism, Aging metabolism, Homeostasis, Inhibin-beta Subunits metabolism, Insulin metabolism, Insulin Resistance, Islets of Langerhans cytology

Abstract

Based on the phenotype of the activin-like kinase-7 (ALK7)-null mouse, activins A and B have been proposed to play distinct roles in regulating pancreatic islet function and glucose homeostasis, with activin A acting to enhance islet function and insulin release while activin B antagonizes these actions. We therefore hypothesized that islets from activin B-null (BBKO) mice would have enhanced glucose-stimulated insulin secretion. In addition, we hypothesized that this enhanced islet function would translate into increased whole body glucose tolerance. We tested these hypotheses by analyzing glucose homeostasis, insulin secretion, and islet function in BBKO mice. No differences were observed in fasting glucose or insulin levels, glucose tolerance, or insulin sensitivity compared with weight-matched young or older males. Similarly, there were no significant differences in insulin secretion comparing islets from WT or BBKO males at either age. However, BBKO islets were more sensitive to activin A, myostatin (MSTN), and follistatin (FST) treatments, so that activin A and FST inhibited and MSTN enhanced glucose stimulated insulin secretion. While mean islet area and the distribution of islet areas were not different between the genotypes, islet mass, islet number, and the proportion of α-cells/islet were significantly reduced in BBKO islets. These results indicate that activin B does not antagonize activin A to influence whole body glucose homeostasis or β-cell function but does influence islet mass and proportion of α-cells/islet. Therefore, loss of activin B signaling alone does not account for the ALK7-null phenotype, but activin B may have important roles in modulating islet mass, islet number, and the cellular composition of islets.

Published

2012

26. Maternal obesity accelerates fetal pancreatic beta-cell but not alpha-cell development in sheep: prenatal consequences.

Author

Ford SP, Zhang L, Zhu M, Miller MM, Smith DT, Hess BW, Moss GE, Nathanielsz PW, and Nijland MJ

Subjects

Animals, Animals, Newborn, Blood Glucose metabolism, Cell Proliferation, Disease Models, Animal, Female, Fetal Development, Fetus pathology, Gestational Age, Glucagon-Secreting Cells metabolism, Hydrocortisone blood, Insulin blood, Insulin-Secreting Cells metabolism, Mitosis, Obesity metabolism, Obesity pathology, Pancreas embryology, Pancreas metabolism, Pregnancy, Prenatal Exposure Delayed Effects, Sheep, Up-Regulation, Glucagon-Secreting Cells pathology, Insulin Resistance, Insulin-Secreting Cells pathology, Maternal Nutritional Physiological Phenomena, Obesity physiopathology, Pancreas pathology

Abstract

Maternal obesity affects offspring weight, body composition, and organ function, increasing diabetes and metabolic syndrome risk. We determined effects of maternal obesity and a high-energy diet on fetal pancreatic development. Sixty days prior to breeding, ewes were assigned to control [100% of National Research Council (NRC) recommendations] or obesogenic (OB; 150% NRC) diets. At 75 days gestation, OB ewes exhibited elevated insulin-to-glucose ratios at rest and during a glucose tolerance test, demonstrating insulin resistance compared with control ewes. In fetal studies, ewes ate their respective diets from 60 days before to 75 days after conception when animals were euthanized under general anesthesia. OB and control ewes increased in body weight by approximately 43% and approximately 6%, respectively, from diet initiation until necropsy. Although all organs were heavier in fetuses from OB ewes, only pancreatic weight increased as a percentage of fetal weight. Blood glucose, insulin, and cortisol were elevated in OB ewes and fetuses on day 75. Insulin-positive cells per unit pancreatic area were 50% greater in fetuses from OB ewes as a result of increased beta-cell mitoses rather than decreased programmed cell death. Lambs of OB ewes were born earlier but weighed the same as control lambs; however, their crown-to-rump length was reduced, and their fat mass was increased. We conclude that increased systemic insulin in fetuses from OB ewes results from increased glucose exposure and/or cortisol-induced accelerated fetal beta-cell maturation and may contribute to premature beta-cell function loss and predisposition to obesity and metabolic disease in offspring.

Published

2009

27. Epac is involved in cAMP-stimulated proglucagon expression and hormone production but not hormone secretion in pancreatic alpha- and intestinal L-cell lines.

Author

Islam D, Zhang N, Wang P, Li H, Brubaker PL, Gaisano HY, Wang Q, and Jin T

Subjects

Blotting, Northern, Blotting, Western, Cell Line, Colforsin pharmacology, Cyclic AMP-Dependent Protein Kinases metabolism, Glucagon-Like Peptide 1 biosynthesis, Glucagon-Like Peptide 1 metabolism, Guanine Nucleotide Exchange Factors genetics, Guanine Nucleotide Exchange Factors metabolism, Humans, Immunohistochemistry, Proglucagon genetics, RNA, Messenger biosynthesis, RNA, Messenger genetics, Reverse Transcriptase Polymerase Chain Reaction, Signal Transduction, Transfection, Cyclic AMP metabolism, Enteroendocrine Cells metabolism, Glucagon-Secreting Cells metabolism, Guanine Nucleotide Exchange Factors biosynthesis, Proglucagon biosynthesis

Abstract

Both Epac and PKA are effectors of the second messenger cAMP. Utilizing an exchange protein directly activated by cAMP (Epac) pathway-specific cAMP analog (ESCA), we previously reported that Epac signaling regulates proglucagon gene (gcg) expression in the glucagon-like peptide-1 (GLP-1)-producing intestinal endocrine L-cell lines GLUTag and STC-1. We now show that Epac-2 is also expressed in glucagon-producing pancreatic alpha-cell lines, including PKA-deficient InR1-G9 cells, and that ESCA stimulates gcg promoter and mRNA expression in the InR1-G9 cells. Using a dominant-negative Epac-2 expression plasmid (Epac-2DN), we found that Epac inhibition attenuated forskolin-stimulated gcg promoter expression in the PKA-active STC-1 cell line and blocked forskolin-stimulated gcg promoter expression in the InR1-G9 cells. Consistently, ESCA was shown to stimulate glucagon and GLP-1 production in the InR1-G9 and GLUTag cell lines, respectively. Surprisingly, ESCA treatment did not show a notable stimulation of glucagon or GLP-1 secretion from these two cell lines. This is in contrast to its ability to stimulate insulin secretion from the pancreatic INS-1 beta-cell line. Our findings suggest that Epac is selectively involved in peptide hormone secretion in pancreatic and intestinal endocrine cells and that distinct signaling cascades are involved in stimulating production vs. secretion of glucagon and GLP-1 in response to cAMP elevation.

Published

2009

28. Cyclic AMP accelerates calcium waves in pancreatic acinar cells.

Author

Shah AU, Grant WM, Latif SU, Mannan ZM, Park AJ, and Husain SZ

Subjects

Animals, Cells, Cultured, Rats, Rats, Sprague-Dawley, Calcium metabolism, Calcium Signaling drug effects, Calcium Signaling physiology, Cyclic AMP administration & dosage, Glucagon-Secreting Cells drug effects, Glucagon-Secreting Cells metabolism

Abstract

Cytosolic Ca(2+) (Ca(i)(2+)) flux within the pancreatic acinar cell is important both physiologically and pathologically. We examined the role of cAMP in shaping the apical-to-basal Ca(2+) wave generated by the Ca(2+)-activating agonist carbachol. We hypothesized that cAMP modulates intra-acinar Ca(2+) channel opening by affecting either cAMP-dependent protein kinase (PKA) or exchange protein directly activated by cAMP (Epac). Isolated pancreatic acinar cells from rats were stimulated with carbachol (1 muM) with or without vasoactive intestinal polypeptide (VIP) or 8-bromo-cAMP (8-Br-cAMP), and then Ca(i)(2+) was monitored by confocal laser-scanning microscopy. The apical-to-basal carbachol (1 muM)-stimulated Ca(2+) wave was 8.63 +/- 0.68 microm/s; it increased to 19.66 +/- 2.22 microm/s (*P < 0.0005) with VIP (100 nM), and similar increases were observed with 8-Br-cAMP (100 microM). The Ca(2+) rise time after carbachol stimulation was reduced in both regions but to a greater degree in the basal. Lag time and maximal Ca(2+) elevation were not significantly affected by cAMP. The effect of cAMP on Ca(2+) waves also did not appear to depend on extracellular Ca(2+). However, the ryanodine receptor (RyR) inhibitor dantrolene (100 microM) reduced the cAMP-enhancement of wave speed. It was also reduced by the PKA inhibitor PKI (1 microM). 8-(4-chloro-phenylthio)-2'-O-Me-cAMP, a specific agonist of Epac, caused a similar increase as 8-Br-cAMP or VIP. These data suggest that cAMP accelerates the speed of the Ca(2+) wave in pancreatic acinar cells. A likely target of this modulation is the RyR, and these effects are mediated independently by PKA and Epac pathways.

Published

2008

29. Inhibition of Ca2+ signaling and glucagon secretion in mouse pancreatic alpha-cells by extracellular ATP and purinergic receptors.

Author

Tudurí E, Filiputti E, Carneiro EM, and Quesada I

Subjects

Adenosine pharmacology, Adenosine Triphosphate analogs & derivatives, Animals, Extracellular Space drug effects, Extracellular Space physiology, Glucose pharmacology, Immunohistochemistry, In Vitro Techniques, Mice, Microscopy, Confocal, Paracrine Communication drug effects, Paracrine Communication physiology, Receptor, Adenosine A1 drug effects, Receptor, Adenosine A2A drug effects, Receptors, Purinergic drug effects, Receptors, Purinergic P2 drug effects, Receptors, Purinergic P2Y1, Adenosine Triphosphate pharmacology, Calcium Signaling drug effects, Glucagon metabolism, Glucagon-Secreting Cells drug effects, Glucagon-Secreting Cells metabolism, Receptors, Purinergic physiology

Abstract

Glucagon secreted from pancreatic alpha-cells plays a critical role in glycemia, mainly by hepatic glucose mobilization. In diabetic patients, an impaired control of glucagon release can worsen glucose homeostasis. Despite its importance, the mechanisms that regulate its secretion are still poorly understood. Since alpha-cells are particularly sensitive to neural and paracrine factors, in this report we studied the role of purinergic receptors and extracellular ATP, which can be released from nerve terminals and beta-cell secretory granules. Using immunocytochemistry, we identified in alpha-cells the P2 receptor subtype P2Y1, as well as the P1 receptors A1 and A2A. In contrast, only P2Y1 and A1 receptors were localized in beta-cells. To analyze the role of purinergic receptors in alpha-cell function, we studied their participation in Ca2+ signaling. At low glucose concentrations, mouse alpha-cells exhibited the characteristic oscillatory Ca2+ signals that lead to secretion. Application of ATP (1-10 microM) abolished these oscillations or reduced their frequency in alpha-cells within intact islets and isolated in culture. ATPgammaS, a nonhydrolyzable ATP derivative, indicated that the ATP effect was mainly direct rather than through ATP-hydrolytic products. Additionally, adenosine (1-10 microM) was also found to reduce Ca2+ signals. ATP-mediated inhibition of Ca2+ signaling was accompanied by a decrease in glucagon release from intact islets in contrast to the adenosine effect. Using pharmacological agonists, we found that only P2Y1 and A2A were likely involved in the inhibitory effect on Ca2+ signaling. All these findings indicate that extracellular ATP and purinergic stimulation are effective regulators of the alpha-cell function.

Published

2008

30. Downstream regulatory element antagonistic modulator regulates islet prodynorphin expression.

Author

Jacobson DA, Cho J, Landa LR Jr, Tamarina NA, Roe MW, Buxbaum JD, and Philipson LH

Subjects

3,4-Dichloro-N-methyl-N-(2-(1-pyrrolidinyl)-cyclohexyl)-benzeneacetamide, (trans)-Isomer pharmacology, Animals, Calcium metabolism, Cell Line, Cell Nucleus metabolism, DNA metabolism, Dynorphins pharmacology, Electrophoretic Mobility Shift Assay, Glucagon metabolism, Glucagon-Secreting Cells chemistry, Glucagon-Secreting Cells drug effects, Glucagon-Secreting Cells metabolism, Glucose pharmacology, Humans, Insulin-Secreting Cells drug effects, Insulin-Secreting Cells metabolism, Islets of Langerhans drug effects, Kv Channel-Interacting Proteins genetics, Mice, Mice, Inbred C57BL, Mice, Knockout, Naltrexone analogs & derivatives, Naltrexone pharmacology, Protein Binding physiology, Receptors, Opioid, kappa analysis, Receptors, Opioid, kappa antagonists & inhibitors, Repressor Proteins genetics, Enkephalins genetics, Gene Expression Regulation, Islets of Langerhans metabolism, Kv Channel-Interacting Proteins metabolism, Protein Precursors genetics, Repressor Proteins metabolism

Abstract

Calcium-binding proteins regulate transcription and secretion of pancreatic islet hormones. Here, we demonstrate neuroendocrine expression of the calcium-binding downstream regulatory element antagonistic modulator (DREAM) and its role in glucose-dependent regulation of prodynorphin (PDN) expression. DREAM is distributed throughout beta- and alpha-cells in both the nucleus and cytoplasm. As DREAM regulates neuronal dynorphin expression, we determined whether this pathway is affected in DREAM(-/-) islets. Under low glucose conditions, with intracellular calcium concentrations of <100 nM, DREAM(-/-) islets had an 80% increase in PDN message compared with controls. Accordingly, DREAM interacts with the PDN promoter downstream regulatory element (DRE) under low calcium (<100 nM) conditions, inhibiting PDN transcription in beta-cells. Furthermore, beta-cells treated with high glucose (20 mM) show increased cytoplasmic calcium (approximately 200 nM), which eliminates DREAM's interaction with the DRE, causing increased PDN promoter activity. As PDN is cleaved into dynorphin peptides, which stimulate kappa-opioid receptors expressed predominantly in alpha-cells of the islet, we determined the role of dynorphin A-(1-17) in glucagon secretion from the alpha-cell. Stimulation with dynorphin A-(1-17) caused alpha-cell calcium fluctuations and a significant increase in glucagon release. DREAM(-/-) islets also show elevated glucagon secretion in low glucose compared with controls. These results demonstrate that PDN transcription is regulated by DREAM in a calcium-dependent manner and suggest a role for dynorphin regulation of alpha-cell glucagon secretion. The data provide a molecular basis for opiate stimulation of glucagon secretion first observed over 25 years ago.

Published

2006

31. Stevioside counteracts the alpha-cell hypersecretion caused by long-term palmitate exposure.

Author

Hong J, Chen L, Jeppesen PB, Nordentoft I, and Hermansen K

Subjects

Acetyl-CoA Carboxylase biosynthesis, Acetyl-CoA Carboxylase genetics, Animals, Carnitine O-Palmitoyltransferase biosynthesis, Carnitine O-Palmitoyltransferase genetics, Cell Line, Tumor, Drug Interactions, Gene Expression drug effects, Glucagon antagonists & inhibitors, Glucagon genetics, Glucagon-Secreting Cells metabolism, Mice, Mice, Transgenic, PPAR gamma biosynthesis, PPAR gamma genetics, Reverse Transcriptase Polymerase Chain Reaction, Secretory Rate drug effects, Stearoyl-CoA Desaturase biosynthesis, Stearoyl-CoA Desaturase genetics, Sterol Regulatory Element Binding Protein 1 biosynthesis, Sterol Regulatory Element Binding Protein 1 genetics, Diterpenes, Kaurane pharmacology, Glucagon metabolism, Glucagon-Secreting Cells drug effects, Glucosides pharmacology, Hypoglycemic Agents pharmacology, Palmitates pharmacology

Abstract

Long-term exposure to fatty acids impairs beta-cell function in type 2 diabetes, but little is known about the chronic effects of fatty acids on alpha-cells. We therefore studied the prolonged impact of palmitate on alpha-cell function and on the expression of genes related to fuel metabolism. We also investigated whether the antihyperglycemic agent stevioside was able to counteract these effects of palmitate. Clonal alpha-TC1-6 cells were cultured with palmitate in the presence or absence of stevioside. After 72 h, we evaluated glucagon secretion, glucagon content, triglyceride (TG) content, and changes in gene expression. Glucagon secretion was dose-dependently increased after 72-h culture, with palmitate at concentrations >or=0.25 mM (P< 0.05). Palmitate (0.5 mM) enhanced TG content of alpha-cells by 73% (P< 0.01). Interestingly, stevioside (10(-8) and 10(-6) M) reduced palmitate-stimulated glucagon release by 22 and 45%, respectively (P< 0.01). There was no significant change in glucagon content after 72-h culture with palmitate and/or stevioside. Palmitate increased carnitine palmitoyltransferase I (CPT I) mRNA level, whereas stevioside enhanced CPT I, peroxisome proliferator-activated receptor-gamma, and stearoyl-CoA desaturase gene expressions in the presence of palmitate (P<0.05). In conclusion, long-term exposure to elevated fatty acids leads to a hypersecretion of glucagon and an accumulation of TG content in clonal alpha-TC1-6 cells. Stevioside was able to counteract the alpha-cell hypersecretion caused by palmitate and enhanced the expression of genes involved in fatty acid metabolism. This indicates that stevioside may be a promising antidiabetic agent in treatment of type 2 diabetes.

Published

2006

32. Cell type-specific activation of metabolism reveals that beta-cell secretion suppresses glucagon release from alpha-cells in rat pancreatic islets.

Author

Takahashi R, Ishihara H, Tamura A, Yamaguchi S, Yamada T, Takei D, Katagiri H, Endou H, and Oka Y

Subjects

Animals, Cell Line, Dicarboxylic Acid Transporters genetics, Dicarboxylic Acid Transporters metabolism, Glycerol Kinase genetics, Glycerol Kinase metabolism, Organic Anion Transporters, Sodium-Dependent genetics, Organic Anion Transporters, Sodium-Dependent metabolism, Rats, Recombinant Proteins metabolism, Symporters genetics, Symporters metabolism, Glucagon metabolism, Glucagon-Secreting Cells metabolism, Insulin-Secreting Cells metabolism, Paracrine Communication physiology

Abstract

Abnormal glucagon secretion is often associated with diabetes mellitus. However, the mechanisms by which nutrients modulate glucagon secretion remain poorly understood. Paracrine modulation by beta- or delta-cells is among the postulated mechanisms. Herein we present further evidence of the paracrine mechanism. First, to activate cellular metabolism and thus hormone secretion in response to specific secretagogues, we engineered insulinoma INS-1E cells using an adenovirus-mediated expression system. Expression of the Na+-dependent dicarboxylate transporter (NaDC)-1 resulted in 2.5- to 4.6-fold (P < 0.01) increases in insulin secretion in response to various tricarboxylic acid cycle intermediates. Similarly, expression of glycerol kinase (GlyK) increased insulin secretion 3.8- or 4.2-fold (P < 0.01) in response to glycerol or dihydroxyacetone, respectively. This cell engineering method was then modified, using the Cre-loxP switching system, to activate beta-cells and non-beta-cells separately in rat islets. NaDC-1 expression only in non-beta-cells, among which alpha-cells are predominant, caused an increase (by 1.8-fold, P < 0.05) in glucagon secretion in response to malate or succinate. However, the increase in glucagon release was prevented when NaDC-1 was expressed in whole islets, i.e., both beta-cells and non-beta-cells. Similarly, an increase in glucagon release with glycerol was observed when GlyK was expressed only in non-beta-cells but not when it was expressed in whole islets. Furthermore, dicarboxylates suppressed basal glucagon secretion by 30% (P < 0.05) when NaDC-1 was expressed only in beta-cells. These data demonstrate that glucagon secretion from rat alpha-cells depends on beta-cell activation and provide insights into the coordinated mechanisms underlying hormone secretion from pancreatic islets.

Published

2006