52 results on '"Nenquin, Myriam"'
Search Results
2. Activators of PKA and epac distinctly influence insulin secretion and cytosolic Ca2+in female mouse islets stimulated by glucose and tolbutamide
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UCL - SSS/IREC/EDIN - Pôle d'endocrinologie, diabète et nutrition, Henquin, Jean-Claude, Nenquin, Myriam, UCL - SSS/IREC/EDIN - Pôle d'endocrinologie, diabète et nutrition, Henquin, Jean-Claude, and Nenquin, Myriam
- Abstract
Amplification of insulin secretion by cAMP is mediated by protein kinase A (PKA) and exchange protein directly activated by cAMP (Epac). Using selective activators, we determined how each effector influences the cytosolic free Ca2+ concentration ([Ca2+]c) and insulin secretion in mouse islets. Alone PKA activator amplified glucose- and tolbutamide-induced insulin secretion, with a greater impact on second than first phase. Epac activator strongly amplified both phases in response to either secretagogue. Amplification was even greater when activators were combined. Although both activators similarly amplified glucose-induced insulin secretion, Epac activator was particularly efficient on tolbutamide-induced insulin secretion. That greater efficacy is attributed to higher [Ca2+]c rather than interaction of tolbutamide with Epac, because it was also observed during KCl stimulation. Moreover, in contrast to Epac activator, tolbutamide was inactive when insulin secretion was increased by gliclazide, and its effect on glucose-induced insulin secretion was unaffected by an inhibitor of Epac2. PKA activator increased [Ca2+]c during acute or steady-state glucose stimulation, whereas Epac activator had no effect alone or in combination. Neither activator affected [Ca2+]c response to tolbutamide or KCl. Metabolic (glucose-mediated) amplification of insulin secretion was unaffected by PKA activator. It was attenuated when insulin secretion was augmented by Epac activator but insensitive to Epac2 inhibitor, which suggests distinct although somewhat overlapping mechanisms. In conclusion, activators of PKA and Epac amplify insulin secretion by augmenting the action of Ca2+ on exocytosis and, for PKA only, slightly increasing glucose-induced [Ca2+]c rise. The influence of Epac seems more important than that of PKA during first phase.
- Published
- 2014
3. Pharmacological stimulation and inhibition of insulin secretion in mouse islets lacking ATP-sensitive K(+) channels.
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UCL - SSS/IREC - Institut de recherche expérimentale et clinique, UCL - SSS/IREC/EDIN - Pôle d'endocrinologie, diabète et nutrition, Szollosi, Andras, Nenquin, Myriam, Henquin, Jean-Claude, UCL - SSS/IREC - Institut de recherche expérimentale et clinique, UCL - SSS/IREC/EDIN - Pôle d'endocrinologie, diabète et nutrition, Szollosi, Andras, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
Background and purpose: ATP-sensitive potassium channels (K(ATP) channels) in beta cells are a major target for insulinotropic drugs. Here, we studied the effects of selected stimulatory and inhibitory pharmacological agents in islets lacking K(ATP) channels. Experimental approach: We compared insulin secretion (IS) and cytosolic calcium ([Ca(2+)](c)) changes in islets isolated from control mice and mice lacking sulphonylurea receptor1 (SUR1), and thus K(ATP) channels in their beta cells (Sur1KO). Key results: While similarly increasing [Ca(2+)](c) and IS in controls, agents binding to site A (tolbutamide) or site B (meglitinide) of SUR1 were ineffective in Sur1KO islets. Of two non-selective blockers of potassium channels, quinine was inactive, whereas tetraethylammonium was more active in Sur1KO compared with control islets. Phentolamine, efaroxan and alinidine, three imidazolines binding to K(IR)6.2 (pore of K(ATP) channels), stimulated control islets, but only phentolamine retained weaker stimulatory effects on [Ca(2+)](c) and IS in Sur1KO islets. Neither K(ATP) channel opener (diazoxide, pinacidil) inhibited Sur1KO islets. Calcium channel blockers (nimodipine, verapamil) or diphenylhydantoin decreased [Ca(2+)](c) and IS in both types of islets, verapamil and diphenylhydantoin being more efficient in Sur1KO islets. Activation of alpha(2)-adrenoceptors or dopamine receptors strongly inhibited IS while partially (clonidine > dopamine) lowering [Ca(2+)](c) (control > Sur1KO islets). Conclusions and implications: Those drugs retaining effects on IS in islets lacking K(ATP) channels, also affected [Ca(2+)](c), indicating actions on other ionic channels. The greater effects of some inhibitors in Sur1KO than in control islets might be relevant to medical treatment of congenital hyperinsulinism caused by inactivating mutations of K(ATP) channels.
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- 2010
4. Metabolic amplifying pathway increases both phases of insulin secretion independently of beta-cell actin microfilaments
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UCL - SSS/IREC - Institut de recherche expérimentale et clinique, UCL - SSS/IREC/EDIN - Pôle d'endocrinologie, diabète et nutrition, Mourad, Nizar, Nenquin, Myriam, Henquin, Jean-Claude, UCL - SSS/IREC - Institut de recherche expérimentale et clinique, UCL - SSS/IREC/EDIN - Pôle d'endocrinologie, diabète et nutrition, Mourad, Nizar, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
Mourad NI, Nenquin M, Henquin J.-C. Metabolic amplifying pathway increases both phases of insulin secretion independently of beta-cell actin microfilaments. Am J Physiol Cell Physiol 299: C389-C398, 2010. First published May 19, 2010; doi: 10.1152/ajpcell.00138.2010.-Two pathways control glucose-induced insulin secretion (IS) by beta-cells. The triggering pathway involves ATP-sensitive potassium (K-ATP) channel-dependent depolarization, Ca2+ influx, and a rise in the cytosolic Ca2+ concentration ([Ca2+](c)), which triggers exocytosis of insulin granules. The metabolic amplifying pathway augments IS without further increasing [Ca2+](c). The underlying mechanisms are unknown. Here, we tested the hypothesis that amplification implicates actin microfilaments. Mouse islets were treated with latrunculin B and cytochalasin B to depolymerize actin or jasplakinolide to polymerize actin. They were then perifused to measure [Ca2+](c) and IS. Metabolic amplification was studied during imposed steady elevation of [Ca2+](c) by tolbutamide or KCl or by comparing the magnitude of [Ca2+](c) and IS changes produced by glucose and tolbutamide. Both actin polymerization and depolymerization augmented IS triggered by all stimuli without increasing (sometimes decreasing) [Ca2+](c), which indicates a predominantly inhibitory function of microfilaments in exocytosis at a step distal to [Ca2+](c) increase. When [Ca2+](c) was elevated and controlled by KCl or tolbutamide, the amplifying action of glucose was facilitated by actin depolymerization and unaffected by polymerization. Both phases of IS were larger in response to high-glucose than to tolbutamide in low-glucose, although triggering [Ca2+](c) was lower. This difference in IS, due to amplification, persisted when the IS rate was doubled by actin depolymerization or polymerization. In conclusion, metabolic amplification is rapid and influences the first as well as the second phase of IS. It is a late step of stimulus-secretion coupling
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- 2010
5. Glucose controls cytosolic Ca2+ and insulin secretion in mouse islets lacking ATP-sensitive K+ channels owing to a knockout of the pore-forming subunit Kir6.2
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UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Ravier, Magalie A., Nenquin, Myriam, Miki, Takashi, Seino, Susumu, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Ravier, Magalie A., Nenquin, Myriam, Miki, Takashi, Seino, Susumu, and Henquin, Jean-Claude
- Abstract
Glucose-induced insulin secretion is classically attributed to the cooperation of a KATP channel-dependent Ca(2+) influx with subsequent rise of the cytosolic free Ca(2+) concentration ([Ca(2+)]c) (triggering pathway) and a KATP channel-independent augmentation of secretion without further increase of [Ca(2+)]c (amplifying pathway). Here we characterized the effects of glucose in beta-cells lacking KATP channels because of a knockout of the pore-forming subunit Kir6.2. Islets from 1-year and 2-week-old Kir6.2KO mice were used freshly after isolation and after 18h culture to measure glucose effects on [Ca(2+)]c and insulin secretion. Kir6.2KO islets were insensitive to diazoxide and tolbutamide. In fresh adult Kir6.2KO islets, basal [Ca(2+)]c and insulin secretion were marginally elevated, and high glucose increased [Ca(2+)]c only transiently, so that the secretory response was minimal (10% of controls) despite a functioning amplifying pathway (evidenced in 30mM KCl). Culture in 10mM glucose increased basal secretion and considerably improved glucose-induced insulin secretion (200% of controls), unexpectedly because of a rise in [Ca(2+)]c with modulation of [Ca(2+)]c oscillations. Similar results were obtained in 2-week-old Kir6.2KO islets. Under selected conditions, high glucose evoked biphasic increases in [Ca(2+)]c and insulin secretion, by inducing KATP channel-independent depolarization and Ca(2+) influx via voltage-dependent Ca(2+) channels. In conclusion, Kir6.2KO beta-cells down-regulate insulin secretion by maintaining low [Ca(2+)]c but culture reveals a glucose-responsive phenotype mainly by increasing [Ca(2+)]c. The results support models implicating a KATP channel-independent amplifying pathway in glucose-induced insulin secretion, and show that KATP channels are not the only possible transducers of metabolic effects on the triggering Ca(2+) signal.
- Published
- 2009
6. Insulin secretion in islets from mice with a double knockout for the dense core vesicle proteins islet antigen-2 (IA-2) and IA-2beta.
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UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Nenquin, Myriam, Szollosi, Andras, Kubosaki, Atsutaka, Louis Notkins, Abner, UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Nenquin, Myriam, Szollosi, Andras, Kubosaki, Atsutaka, and Louis Notkins, Abner
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Islet antigen-2 (IA-2 or ICA 512) and IA-2beta (or phogrin) are major autoantigens in type 1 diabetes. They are located in dense core secretory vesicles including insulin granules, but their role in beta-cell function is unclear. Targeted disruption of either IA-2 or IA-2beta, or both, impaired glucose tolerance, an effect attributed to diminution of insulin secretion. In this study, we therefore characterized the dynamic changes in cytosolic Ca2+([Ca2+](c)) and insulin secretion in islets from IA-2/IA-2beta double knockout (KO) mice. High glucose (15 mM) induced biphasic insulin secretion in IA-2/IA-2beta KO islets, with a similar first phase and smaller second phase compared with controls. Since the insulin content of IA-2/IA-2beta KO islets was approximately 45% less than that of controls, fractional insulin secretion (relative to content) was thus increased during first phase and unaffected during second phase. This peculiar response occurred in spite of a slightly smaller rise in [Ca2+](c), could not be attributed to an alteration of glucose metabolism (NADPH fluorescence) and also was observed with tolbutamide. The dual control of insulin secretion via the K(ATP) channel-dependent triggering pathway and K(ATP) channel-independent amplifying pathway was unaltered in IA-2/IA-2beta KO islets, and so were the potentiations by acetylcholine or cAMP (forskolin). Intriguingly, amino acids, in particular the cationic arginine and lysine, induced larger fractional insulin secretion in IA-2/IA-2beta KO than control islets. In conclusion, IA-2 and IA-2beta are dispensable for exocytosis of insulin granules, but are probably more important for cargo loading and/or stability of dense core vesicles.
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- 2008
7. Glucose-induced cytosolic pH changes in beta-cells and insulin secretion are not causally related: studies in islets lacking the Na+/H+ exchangeR NHE1.
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UCL - MD/FSIO - Département de physiologie et pharmacologie, Stiernet, Patrick, Nenquin, Myriam, Moulin, Pierre, Jonas, Jean-Christophe, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Stiernet, Patrick, Nenquin, Myriam, Moulin, Pierre, Jonas, Jean-Christophe, and Henquin, Jean-Claude
- Abstract
The contribution of Na(+)/H(+) exchange (achieved by NHE proteins) to the regulation of beta-cell cytosolic pH(c), and the role of pH(c) changes in glucose-induced insulin secretion are disputed and were examined here. Using real-time PCR, we identified plasmalemmal NHE1 and intracellular NHE7 as the two most abundant NHE isoforms in mouse islets. We, therefore, compared insulin secretion, cytosolic free Ca(2+) ([Ca(2+)](c)) and pH(c) in islets from normal mice and mice bearing an inactivating mutation of NHE1 (Slc9A1-swe/swe). The experiments were performed in HCO(-)(3)/CO(2) or HEPES/NaOH buffers. PCR and functional approaches showed that NHE1 mutant islets do not express compensatory pH-regulating mechanisms. NHE1 played a greater role than HCO(-)(3)-dependent mechanisms in the correction of an acidification imposed by a pulse of NH(4)Cl. In contrast, basal pH(c) (in low glucose) and the alkalinization produced by high glucose were independent of NHE1. Dimethylamiloride, a classic blocker of Na(+)/H(+) exchange, did not affect pH(c) but increased insulin secretion in NHE1 mutant islets, indicating unspecific effects. In control islets, glucose similarly increased [Ca(2+)](c) and insulin secretion in HCO(-)(3) and HEPES buffer, although pH(c) changed in opposite directions. The amplification of insulin secretion that glucose produces when [Ca(2+)](c) is clamped at an elevated level by KCl was also unrelated to pH(c) and pH(c) changes. All effects of glucose on [Ca(2+)](c) and insulin secretion proved independent of NHE1. In conclusion, NHE1 protects beta-cells against strong acidification, but has no role in stimulus-secretion coupling. The changes in pH(c) produced by glucose involve HCO(-)(3)-dependent mechanisms. Variations in beta-cell pH(c) are not causally related to changes in insulin secretion.
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- 2007
8. Overnight culture unmasks glucose-induced insulin secretion in mouse islets lacking ATP-sensitive K+ channels by improving the triggering Ca2+ signal.
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UCL - MD/FSIO - Département de physiologie et pharmacologie, Szollosi, Andras, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Szollosi, Andras, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
A current model ascribes glucose-induced insulin secretion to the interaction of a triggering pathway (K(ATP) channel-dependent Ca(2+) influx and rise in cytosolic [Ca(2+)](c)) and an amplifying pathway (K(ATP) channel-independent augmentation of secretion without further increase of [Ca(2+)](c)). However, several studies of sulfonylurea receptor 1 null mice (Sur1KO) failed to measure significant effects of glucose in their islets lacking K(ATP) channels. We addressed this issue that challenges the model. Compared with controls, fresh Sur1KO islets showed slightly elevated basal [Ca(2+)](c) and insulin secretion. In 15 mm glucose, the absolute rate of secretion was approximately 3-fold lower in Sur1KO than control islets, with only poor increase above base line. Overnight culture of Sur1KO islets in 10 mm glucose (not in 5 mm) augmented basal insulin secretion and considerably improved the response to 15 mm glucose, which reached higher values than in control islets, in which culture had little impact. Glucose stimulation during KCl depolarization showed that the amplifying pathway is functional in fresh and cultured Sur1KO islets. The differences in insulin secretion between fresh and cultured Sur1KO islets and between Sur1KO and control islets were not attributable to differences in insulin content, glucose oxidation rate, or synchronization of [Ca(2+)](c) oscillations. The unmasking of glucose-induced insulin secretion in beta-cells lacking K(ATP) channels is paradoxically due to improvement in the production of a triggering signal (elevated [Ca(2+)](c)). The results show that K(ATP) channels are not the only transducer of glucose effects on [Ca(2+)](c) in beta-cells. They explain controversies in the literature and refute arguments raised against the model implicating an amplifying pathway in glucose-induced insulin secretion.
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- 2007
9. Nutrient control of insulin secretion in perifused adult pig islets.
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UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/CHIR - Département de chirurgie, UCL - (SLuc) Centre de thérapie tissulaire et cellulaire, Dufrane, Denis, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/CHIR - Département de chirurgie, UCL - (SLuc) Centre de thérapie tissulaire et cellulaire, Dufrane, Denis, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
OBJECTIVES: Xenotransplantation of pig islets is a potential solution to the shortage of human islets, but our knowledge of how these islets secrete insulin in response to nutrients is still fragmentary. This was the question addressed in the present study. METHODS: After 24 h culture adult pig islets were perifused to characterize the dynamics of insulin secretion. Some responses were compared to those in human islets. RESULTS: Increasing glucose from 1 to 15 mM weakly (approximately 2x) stimulated insulin secretion, which was potentiated (approximately 12x) by the cAMP-producing agent, forskolin. The effect of glucose was concentration-dependent (threshold at 3-5 mM and maximum at approximately 10 mM). The pattern of secretion was biphasic with a small first phase and an ascending second phase, and a paradoxical increase when the glucose concentration was abruptly lowered. Diazoxide abolished glucose-induced insulin secretion and tolbutamide reversed the inhibition. Glucose also increased secretion when islets were depolarized with tolbutamide or KCl. Insulin secretion was increased by leucine+glutamine, arginine, alanine or a mixture of amino acids, but their effect was significant only in the presence of forskolin. Upon stimulation by glucose alone, human islets secreted approximately 10x more insulin than pig islets, and the kinetics was characterized by a large first phase, a flat second phase, and rapid reversibility. CONCLUSIONS: Compared with human islets, in vitro insulin secretion by adult pig islets is characterized by a different kinetics and a major quantitative deficiency that can be corrected by cAMP.
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- 2007
10. Glucose stimulates Ca2+ influx and insulin secretion in 2-week-old beta-cells lacking ATP-sensitive K+ channels.
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UCL - MD/FSIO - Département de physiologie et pharmacologie, Szollosi, Andras, Nenquin, Myriam, Aguilar-Bryan, Lydia, Bryan, Joseph, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Szollosi, Andras, Nenquin, Myriam, Aguilar-Bryan, Lydia, Bryan, Joseph, and Henquin, Jean-Claude
- Abstract
In adult beta-cells glucose-induced insulin secretion involves two mechanisms (a) a K(ATP) channel-dependent Ca(2+) influx and rise of cytosolic [Ca(2+)](c) and (b) a K(ATP) channel-independent amplification of secretion without further increase of [Ca(2+)](c). Mice lacking the high affinity sulfonylurea receptor (Sur1KO), and thus K(ATP) channels, have been developed as a model of congenital hyperinsulinism. Here, we compared [Ca(2+)](c) and insulin secretion in overnight cultured islets from 2-week-old normal and Sur1KO mice. Control islets proved functionally mature: the magnitude and biphasic kinetics of [Ca(2+)](c) and insulin secretion changes induced by glucose, and operation of the amplifying pathway, were similar to adult islets. Sur1KO islets perifused with 1 mm glucose showed elevation of both basal [Ca(2+)](c) and insulin secretion. Stimulation with 15 mm glucose produced a transient drop of [Ca(2+)](c) followed by an overshoot and a sustained elevation, accompanied by a monophasic, 6-fold increase in insulin secretion. Glucose also increased insulin secretion when [Ca(2+)](c) was clamped by KCl. When Sur1KO islets were cultured in 5 instead of 10 mm glucose, [Ca(2+)](c) and insulin secretion were unexpectedly low in 1 mm glucose and increased following a biphasic time course upon stimulation by 15 mm glucose. This K(ATP) channel-independent first phase [Ca(2+)](c) rise was attributed to a Na(+)-, Cl(-)-, and Na(+)-pump-independent depolarization of beta-cells, leading to Ca(2+) influx through voltage-dependent calcium channels. Glucose indeed depolarized Sur1KO islets under these conditions. It is suggested that unidentified potassium channels are sensitive to glucose and subserve the acute and long-term metabolic control of [Ca(2+)](c) in beta-cells without functional K(ATP) channels.
- Published
- 2007
11. Both triggering and amplifying pathways contribute to fuel-induced insulin secretion in the absence of sulfonylurea receptor-1 in pancreatic beta-cells.
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UCL - MD/FSIO - Département de physiologie et pharmacologie, Nenquin, Myriam, Szollosi, Andras, Aguilar-Bryan, Lydia, Bryan, Joseph, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Nenquin, Myriam, Szollosi, Andras, Aguilar-Bryan, Lydia, Bryan, Joseph, and Henquin, Jean-Claude
- Abstract
In normal beta-cells glucose induces insulin secretion by activating both a triggering pathway (closure of K(ATP) channels, depolarization, and rise in cytosolic [Ca(2+)](i)) and an amplifying pathway (augmentation of Ca(2+) efficacy on exocytosis). It is unclear if and how nutrients can regulate insulin secretion by beta-cells lacking K(ATP) channels (Sur1 knockout mice). We compared glucose- and amino acid-induced insulin secretion and [Ca(2+)](i) changes in control and Sur1KO islets. In 1 mm glucose (non-stimulatory for controls), the triggering signal [Ca(2+)](i) was high (loss of regulation) and insulin secretion was stimulated in Sur1KO islets. This "basal" secretion was decreased or increased by imposed changes in [Ca(2+)](i) and was dependent on ATP production, indicating that both triggering and amplifying signals are involved. High glucose stimulated insulin secretion in Sur1KO islets, by an unsuspected, transient increase in [Ca(2+)](i) and a sustained activation of the amplifying pathway. Unlike controls, Sur1KO islets were insensitive to diazoxide and tolbutamide, which rules out effects of either drug at sites other than K(ATP) channels. Amino acids potently increased insulin secretion by Sur1KO islets through both a further electrogenic rise in [Ca(2+)](i) and a metabolism-dependent activation of the amplifying pathway. After sulfonylurea blockade of their K(ATP) channels, control islets qualitatively behaved like Sur1KO islets, but their insulin secretion rate was consistently lower for a similar or even higher [Ca(2+)](i). In conclusion, fuel secretagogues can control insulin secretion in beta-cells without K(ATP) channels, partly by an unsuspected influence on the triggering [Ca(2+)](i) signal and mainly by the modulation of a very effective amplifying pathway.
- Published
- 2004
12. Hierarchy of the beta-cell signals controlling insulin secretion
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UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Henquin, Jean-Claude, Ravier, M A, Nenquin, Myriam, Jonas, Jean-Christophe, Gilon, Patrick, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Henquin, Jean-Claude, Ravier, M A, Nenquin, Myriam, Jonas, Jean-Christophe, and Gilon, Patrick
- Published
- 2003
13. SERCA3 ablation does not impair insulin secretion but suggests distinct roles of different sarcoendoplasmic reticulum Ca(2+) pumps for Ca(2+) homeostasis in pancreatic beta-cells
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UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/MNOP - Département de morphologie normale et pathologique, Arredouani, Abdelilah, Guiot, Yves, Jonas, Jean-Christophe, Liu, Lynne H, Nenquin, Myriam, Pertusa, José A, Rahier, Jacques, Rolland, Jean-François, Shull, Gary E, STEVENS, Martine, Wuytack, Frank, Henquin, Jean-Claude, Gilon, Patrick, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/MNOP - Département de morphologie normale et pathologique, Arredouani, Abdelilah, Guiot, Yves, Jonas, Jean-Christophe, Liu, Lynne H, Nenquin, Myriam, Pertusa, José A, Rahier, Jacques, Rolland, Jean-François, Shull, Gary E, STEVENS, Martine, Wuytack, Frank, Henquin, Jean-Claude, and Gilon, Patrick
- Abstract
Two sarcoendoplasmic reticulum Ca(2+)-ATPases, SERCA3 and SERCA2b, are expressed in pancreatic islets. Immunocytochemistry showed that SERCA3 is restricted to beta-cells in the mouse pancreas. Control and SERCA3-deficient mice were used to evaluate the role of SERCA3 in beta-cell cytosolic-free Ca(2+) concentration ([Ca(2+)](c)) regulation, insulin secretion, and glucose homeostasis. Basal [Ca(2+)](c) was not increased by SERCA3 ablation. Stimulation with glucose induced a transient drop in basal [Ca(2+)](c) that was suppressed by inhibition of all SERCAs with thapsigargin (TG) but unaffected by selective SERCA3 ablation. Ca(2+) mobilization by acetylcholine was normal in SERCA3-deficient beta-cells. In contrast, [Ca(2+)](c) oscillations resulting from intermittent glucose-stimulated Ca(2+) influx and [Ca(2+)](c) transients induced by pulses of high K(+) were similarly affected by SERCA3 ablation or TG pretreatment of control islets; their amplitude was increased and their slow descending phase suppressed. This suggests that, during the decay of each oscillation, the endoplasmic reticulum releases Ca(2+) that was pumped by SERCA3 during the upstroke phase. SERCA3 ablation increased the insulin response of islets to 15 mmol/l glucose. However, basal and postprandial plasma glucose and insulin concentrations in SERCA3-deficient mice were normal. In conclusion, SERCA2b, but not SERCA3, is involved in basal [Ca(2+)](c) regulation in beta-cells. SERCA3 becomes operative when [Ca(2+)](c) rises and is required for normal [Ca(2+)](c) oscillations in response to glucose. However, a lack of SERCA3 is insufficient in itself to alter glucose homeostasis or impair insulin secretion in mice.
- Published
- 2002
14. Signals and pools underlying biphasic insulin secretion.
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UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Henquin, Jean-Claude, Ishiyama, Nobuyoshi, Nenquin, Myriam, Ravier, Magalie A., Jonas, Jean-Christophe, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Henquin, Jean-Claude, Ishiyama, Nobuyoshi, Nenquin, Myriam, Ravier, Magalie A., and Jonas, Jean-Christophe
- Abstract
Rapid and sustained stimulation of beta-cells with glucose induces biphasic insulin secretion. The two phases appear to reflect a characteristic of stimulus-secretion coupling in each beta-cell rather than heterogeneity in the time-course of the response between beta-cells or islets. There is no evidence indicating that biphasic secretion can be attributed to an intrinsically biphasic metabolic signal. In contrast, the biphasic rise in cytoplasmic Ca(2+) concentration ([Ca(2+)](i)) induced by glucose is important to shape the two phases of secretion. The first phase requires a rapid and marked elevation of [Ca(2+)](i) and corresponds to the release of insulin granules from a limited pool. The magnitude of the second phase is determined by the elevation of [Ca(2+)](i), but its development requires production of another signal. This signal corresponds to the amplifying action of glucose and may serve to replenish the pool of granules that are releasable at the prevailing [Ca(2+)](i). The species characteristics of biphasic insulin secretion and its perturbations in pathological situations are discussed.
- Published
- 2002
15. The elevation of glutamate content and the amplification of insulin secretion in glucose-stimulated pancreatic islets are not causally related.
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UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Bertrand, Gyslaine, Ishiyama, Nobuyoshi, Nenquin, Myriam, Ravier, Magalie A., Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Bertrand, Gyslaine, Ishiyama, Nobuyoshi, Nenquin, Myriam, Ravier, Magalie A., and Henquin, Jean-Claude
- Abstract
Glucose increases insulin secretion by raising cytoplasmic Ca(2+) ([Ca(2+)](i)) in beta-cells (triggering pathway) and augmenting the efficacy of Ca(2+) on exocytosis (amplifying pathway). It has been suggested that glutamate formed from alpha-ketoglutarate is a messenger of the amplifying pathway (Maechler, P., and Wollheim, C. B. (1999) Nature 402, 685-689). This hypothesis was tested with mouse islets depolarized with 30 mm KCl (+ diazoxide) or with a saturating concentration of sulfonylurea. Because [Ca(2+)](i) was elevated under these conditions, insulin secretion was stimulated already in 0 mm glucose. The amplification of secretion produced by glucose was accompanied by an increase in islet glutamate. However, glutamine (0.5-2 mm) markedly augmented islet glutamate without affecting insulin secretion, whereas glucose augmented secretion without influencing glutamate levels when these were elevated by glutamine. Allosteric activation of glutamate dehydrogenase by BCH (2-amino 2-norbornane carboxylic acid) lowered islet glutamate but increased insulin secretion. Similar insulin secretion thus occurred at very different cellular glutamate levels. Glutamine did not affect islet [Ca(2+)](i) and pH(i), whereas glucose and BCH slightly raised pH(i) and either slightly decreased (30 mm KCl) or increased (tolbutamide) [Ca(2+)](i). The general dissociation between changes in islet glutamate and insulin secretion refutes a role of beta-cell glutamate in the amplification of insulin secretion by glucose.
- Published
- 2002
16. Inhibition of protein synthesis sequentially impairs distinct steps of stimulus-secretion coupling in pancreatic beta cells
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UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Garcia-Barrado, Maria José, Ravier, Magalie A, Rolland, Jean-François, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - (SLuc) Service d'endocrinologie et de nutrition, Garcia-Barrado, Maria José, Ravier, Magalie A, Rolland, Jean-François, Gilon, Patrick, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
Proteins with a short half-life are potential sites of pancreatic ss cell dysfunction under pathophysiological conditions. In this study, mouse islets were used to establish which step in the regulation of insulin secretion is most sensitive to inhibition of protein synthesis by 10 microM cycloheximide (CHX). Although islet protein synthesis was inhibited approximately 95% after 1 h, the inhibition of insulin secretion was delayed and progressive. After long (18-20 h) CHX-treatment, the strong (80%) inhibition of glucose-, tolbutamide-, and K(+)-induced insulin secretion was not due to lower insulin stores, to any marked impairment of glucose metabolism or to altered function of K(+)-ATP channels (total K(+)-ATP currents were however decreased). It was partly caused by a decreased Ca(2+) influx (whole-cell Ca(2+) current) resulting in a smaller rise in cytosolic Ca(2+) ([Ca(2+)](i)). The situation was very different after short (2-5 h) CHX-treatment. Insulin secretion was 50-60% inhibited although islet glucose metabolism was unaffected and stimulus-induced [Ca(2+)](i) rise was not (2 h) or only marginally (5 h) decreased. The efficiency of Ca(2+) on secretion was thus impaired. The inhibition of insulin secretion by 15 h of CHX treatment was more slowly reversible (>4 h) than that of protein synthesis. This reversibility of secretion was largely attributable to recovery of a normal Ca(2+) efficiency. In conclusion, inhibition of protein synthesis in islets inhibits insulin secretion in two stages: a rapid decrease in the efficiency of Ca(2+) on exocytosis, followed by a decrease in the Ca(2+) signal mediated by a slower loss of functional Ca(2+) channels. Glucose metabolism and the regulation of K(+)-ATP channels are more resistant. Proteins with a short half-life appear to be important to ensure optimal Ca(2+) effects on exocytosis, and are the potential Achille's heel of stimulus-secretion coupling.
- Published
- 2001
17. The oscillatory behavior of pancreatic islets from mice with mitochondrial glycerol-3-phosphate dehydrogenase knockout.
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Ravier, M A, Eto, K, Jonkers, F C, Nenquin, Myriam, Kadowaki, T, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Ravier, M A, Eto, K, Jonkers, F C, Nenquin, Myriam, Kadowaki, T, and Henquin, Jean-Claude
- Abstract
Glucose stimulation of pancreatic beta cells induces oscillations of the membrane potential, cytosolic Ca(2+) ([Ca(2+)](i)), and insulin secretion. Each of these events depends on glucose metabolism. Both intrinsic oscillations of metabolism and repetitive activation of mitochondrial dehydrogenases by Ca(2+) have been suggested to be decisive for this oscillatory behavior. Among these dehydrogenases, mitochondrial glycerol-3-phosphate dehydrogenase (mGPDH), the key enzyme of the glycerol phosphate NADH shuttle, is activated by cytosolic [Ca(2+)](i). In the present study, we compared different types of oscillations in beta cells from wild-type and mGPDH(-/-) mice. In clusters of 5-30 islet cells and in intact islets, 15 mM glucose induced an initial drop of [Ca(2+)](i), followed by an increase in three phases: a marked initial rise, a partial decrease with rapid oscillations and eventually large and slow oscillations. These changes, in particular the frequency of the oscillations and the magnitude of the [Ca(2+)] rise, were similar in wild-type and mGPDH(-/-) mice. Glucose-induced electrical activity (oscillations of the membrane potential with bursts of action potentials) was not altered in mGPDH(-/-) beta cells. In single islets from either type of mouse, insulin secretion strictly followed the changes in [Ca(2+)](i) during imposed oscillations induced by pulses of high K(+) or glucose and during the biphasic elevation induced by sustained stimulation with glucose. An imposed and controlled rise of [Ca(2+)](i) in beta cells similarly increased NAD(P)H fluorescence in control and mGDPH(-/-) islets. Inhibition of the malate-aspartate NADH shuttle with aminooxyacetate only had minor effects in control islets but abolished the electrical, [Ca(2+)](i) and secretory responses in mGPDH(-/-) islets. The results show that the two distinct NADH shuttles play an important but at least partially redundant role in glucose-induced insulin secretion. The oscillatory behavior of b
- Published
- 2000
18. Unbound rather than total concentration and saturation rather than unsaturation determine the potency of fatty acids on insulin secretion.
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Warnotte, C., Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Warnotte, C., Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
Isolated mouse islets were used to compare the effects of three saturated (myristate, palmitate and stearate) and three unsaturated (oleate, linoleate and linolenate) long-chain fatty acids on insulin secretion. By varying the concentrations of fatty acid (250-1250 micromol/l) and albumin simultaneously or independently, we also investigated whether the insulinotropic effect is determined by the unbound or total concentration of the fatty acids. Only palmitate and stearate slightly increased basal insulin secretion (3 mmol/l glucose). All tested fatty acids potentiated glucose-induced insulin secretion (10-15 mmol/l), and the following rank order of potency was obtained when they were compared at the same total concentrations: palmitate approximately = stearate > myristate > or = oleate > or = linoleate approximately = linolenate. The effect of a given fatty acid varied with the fatty acid to albumin molar ratio, in a way which indicated that the unbound fraction is the important one for the stimulation of beta cells. When the potentiation of insulin secretion was expressed as a function of the unbound concentrations, the following rank order emerged: palmitate > myristate > stearate approximately = oleate > linoleate approximately = linolenate. In conclusion, the acute and direct effects of long-chain fatty acids on insulin secretion are due to their unbound fraction. They are observed only at fatty acid/albumin ratios higher than those normally occurring in plasma. Saturated fatty acids are stronger insulin secretagogues than unsaturated fatty acids. Unbound palmitate is by far the most potent of the six common long-chain fatty acids.
- Published
- 1999
19. Relative contribution of Ca2+-dependent and Ca2+-independent mechanisms to the regulation of insulin secretion by glucose.
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Sato, Y, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Sato, Y, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
Although insulin secretion is usually regarded as a Ca2+-dependent mechanism, recent studies have suggested the existence of a Ca2+-independent pathway of regulation by glucose. Here, mouse islets were used to compare the contribution of Ca2+-dependent and -independent pathways. Glucose increased insulin release in a concentration-dependent manner both in a control medium, when it depolarizes beta cells and raises [Ca2+]i (triggering signal), and in the presence of 30 mM K+ and diazoxide, when it does not further raise [Ca2+]i but increases its efficacy on exocytosis. Both Ca2+-dependent responses were amplified by glucagon-like peptide-1+acetylcholine, and were strongly potentiated by forskolin+PMA. Under conditions of mild or stringent Ca2+ deprivation, glucose had no effect either alone or with GLP-1 and acetylcholine, and was poorly effective even during pharmacological activation of protein kinases A and C. Similar results were obtained with rat islets. It is concluded that physiological regulation of insulin release by glucose is essentially achieved through the two Ca2+-dependent pathways without significant contribution of a Ca2+-independent mechanism.
- Published
- 1998
20. Physiological relevance of a Ca2+-independent pathway of regulation of insulin secretion by glucose
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Sato, Y, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Sato, Y, Nenquin, Myriam, and Henquin, Jean-Claude
- Published
- 1998
21. Do sulfonylureas and diazoxide influence insulin secretion by modulating the action of Ca2+ in pancreatic beta cells?
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Gilon, Patrick, Mariot, P., Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Gilon, Patrick, Mariot, P., Nenquin, Myriam, and Henquin, Jean-Claude
- Published
- 1998
22. No evidence for a role of reverse Na(+)-Ca2+ exchange in insulin release from mouse pancreatic islets
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Garcia-Barrado, Maria José, Gilon, Patrick, Sato, Yoshihiko, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Garcia-Barrado, Maria José, Gilon, Patrick, Sato, Yoshihiko, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
We studied whether reverse Na(+)-Ca2+ exchange can increase cytoplasmic Ca2+ ([Ca2+]i) in mouse islets and contribute to insulin release. The exchange was stimulated by replacing Na+ with choline, sucrose, or lithium in a medium containing 15 mM glucose. Na+ omission increased electrical activity in B cells, [Ca2+]i, and insulin release. When voltage-dependent Ca2+ channels were blocked by nimodipine or closed by holding the membrane polarized with diazoxide, Na+ omission caused a slight hyperpolarization, a small rise in [Ca2+]i, and a marginal increase in insulin release (the latter only with choline). This small rise in [Ca2+]i was dependent on extracellular Ca2+ but was hardly augmented when intracellular Na+ was raised with alanine. When B cells were depolarized by 30 mM K+, Na+ omission did not affect the membrane potential but increased [Ca2+]i and insulin release. If Ca2+ channels were blocked by nimodipine, only marginal increases in Ca2+ and insulin release persisted, which were not different from those observed when the cells were not depolarized. This indicates that Ca2+ influx through voltage-dependent Ca2+ channels rather than via reverse Na(+)-Ca2+ exchange underlies the rise in [Ca2+]i and in insulin release produced by Na+ removal. No decisive support for Ca2+ influx by reverse Na(+)-Ca2+ exchange could be found.
- Published
- 1996
23. Multiple effects and stimulation of insulin secretion by the tyrosine kinase inhibitor genistein in normal mouse islets
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/NOPS - Département de neurologie et de psychiatrie, UCL - (SLuc) Service de psychiatrie adulte, Jonas, Jean-Christophe, Plant, T D, Gilon, Patrick, de Timary, Philippe, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/NOPS - Département de neurologie et de psychiatrie, UCL - (SLuc) Service de psychiatrie adulte, Jonas, Jean-Christophe, Plant, T D, Gilon, Patrick, de Timary, Philippe, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
1. Islets from normal mice were used to test the acute effects of genistein, a potent tyrosine kinase inhibitor, on stimulus-secretion coupling in pancreatic beta-cells. 2. Genistein produced a concentration-dependent (10-100 microM), reversible, increase of insulin release. This effect was marginal on basal release or in the presence of non-metabolized secretagogues, and much larger in the presence of glucose or other nutrients. The increase in insulin release caused by 100 microM genistein was abolished by adrenaline or omission of extracellular Ca2+. It was not accompanied by any rise of cyclic AMP, inositol phosphate or adenine nucleotide levels. 3. Although genistein slightly inhibited ATP-sensitive K+ channels, as shown by 86Rb efflux and patch-clamp experiments, this effect could not explain the action of the drug on insulin release because the latter persisted when ATP-sensitive K+ channels were all blocked by maximally effective concentrations of glucose and tolbutamide. Genistein was also effective when ATP-sensitive K+ channels were opened by diazoxide and the beta-cell membrane depolarized by 30 mM K, but ineffective in the presence of diazoxide and normal extracellular K. 4. Genistein paradoxically decreased Ca2+ influx in beta-cells, as shown by the inhibition of glucose-induced electrical activity, by the inhibition of Ca2+ currents (perforated patches) and by the lowering of cytosolic [Ca2+]i (fura-2 technique). Genistein thus increases insulin release in spite of a lowering of [Ca2+]i in beta-cells. 5. Daidzein, an analogue of genistein reported not to affect tyrosine kinases, was slightly less potent than genistein on K+ and Ca2+ channels, but increased insulin secretion in a similar way.(ABSTRACT TRUNCATED AT 250 WORDS)
- Published
- 1995
24. Muscarinic stimulation exerts both stimulatory and inhibitory effects on the concentration of cytoplasmic Ca2+ in the electrically excitable pancreatic B-cell
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Gilon, Patrick, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
Mouse pancreatic islets were used to investigate how muscarinic stimulation influences the cytoplasmic Ca2+ concentration ([Ca2+]i) in insulin-secreting B-cells. In the absence of extracellular Ca2+, acetylcholine (ACh) triggered a transient, concentration-dependent and thapsigargin-inhibited increase in [Ca2+]i. In the presence of extracellular Ca2+ and 15 mM glucose, ACh induced a biphasic rise in [Ca2+]i. The initial, transient phase increased with the concentration of ACh, whereas the second, sustained, phase was higher at low (0.1-1 microM) than at high (> or = 10 microM) concentrations of ACh. Thapsigargin attenuated (did not suppress) the first phase of the [Ca2+]i rise and did not affect the sustained response. This sustained rise was inhibited by omission of extracellular Na+ (which prevents the depolarizing action of ACh) and by D600 or diazoxide (which prevent activation of voltage-dependent Ca2+ channels). During steady-state stimulation, the Ca2+ action potentials in B-cells were stimulated by 1 microM ACh but inhibited by 100 microM ACh. When B-cells were depolarized by 45 mM K+, ACh induced a concentration-dependent, biphasic change in [Ca2+]i, consisting of a first peak rapidly followed by a decrease. Thapsigargin suppressed the peak without affecting the drop in [Ca2+]i. Measurements of 45Ca2+ efflux under similar conditions indicated that ACh decreases Ca2+ influx and slightly increases the efflux. All effects of ACh were blocked by atropine. In conclusion, three mechanisms at least are involved in the biphasic change in [Ca2+]i that muscarinic stimulation exerts in excitable pancreatic B-cells. A mobilization of Ca2+ from the endoplasmic reticulum contributes significantly to the first peak, but little to the steady-state rise in [Ca2+]i. This second phase results from an influx of Ca2+ through voltage-dependent Ca2+ channels activated by a Na(+)-dependent depolarization. However, when high concentrations of ACh are used, Ca2+ influx is attenuated
- Published
- 1995
25. Two sites of glucose control of insulin release with distinct dependence on the energy state in pancreatic B-cells
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/NOPS - Département de neurologie et de psychiatrie, UCL - (SLuc) Service de psychiatrie adulte, UCL - (SLuc) Service d'endocrinologie et de nutrition, de Timary, Philippe, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/NOPS - Département de neurologie et de psychiatrie, UCL - (SLuc) Service de psychiatrie adulte, UCL - (SLuc) Service d'endocrinologie et de nutrition, de Timary, Philippe, Gilon, Patrick, Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
The energy state of pancreatic B-cells may influence insulin release at several steps of stimulus-secretion coupling. By closing ATP-sensitive K+ channels (K(+)-ATP channels), a rise in the ATP/ADP ratio may regulate the membrane potential, and hence Ca2+ influx. It may also modulate the effectiveness of Ca2+ on its intracellular targets. To assess the existence of these two roles and determine their relative importance for insulin release, we tested the effects of azide, a mitochondrial poison, on mouse B-cell function under various conditions. During stimulation by glucose alone, when K(+)-ATP channels are controlled by cellular metabolism, azide caused parallel, concentration-dependent (0.5-5 mM), membrane repolarization, decrease in cytosolic Ca2+ concentration [Ca2+]i and inhibition of insulin release. When K(+)-ATP channels were closed pharmacologically (by tolbutamide in high glucose), azide did not repolarize the membrane or decrease [Ca2+]i, and was much less effective in inhibiting insulin release. A similar resistance to azide was observed when K(+)-ATP channels were opened by diazoxide, and high K+ was used to depolarize the membrane and raise [Ca2+]i. In contrast, azide similarly decreased ATP levels and increased ADP levels, thereby lowering the ATP/ADP ratio under all conditions. In conclusion, lowering the ATP/ADP ratio in B-cells can inhibit insulin release even when [Ca2+]i remains high. However, this distal step is much more resistant to a decrease in the energy state of B-cells than is the control of membrane potential by K(+)-ATP channels. Generation of the signal triggering insulin release, high [Ca2+]i, through metabolic control of membrane potential requires a higher global ATP/ADP ratio than does activation of the secretory process itself.
- Published
- 1994
26. Role of the Energy-state of B-cells in the Control of Insulin Release
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/NOPS - Département de neurologie et de psychiatrie, UCL - (SLuc) Service de psychiatrie adulte, de Timary, Philippe, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, Belgian Society of Fundamental and Clinical Physiology and Pharmacology (Autumn Meeting), UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/NOPS - Département de neurologie et de psychiatrie, UCL - (SLuc) Service de psychiatrie adulte, de Timary, Philippe, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, and Belgian Society of Fundamental and Clinical Physiology and Pharmacology (Autumn Meeting)
- Abstract
of the Belgian Society of Fundamental and Clinical Physiology and Pharmacology (Autumn Meeting), 20 November 1993, Brussels, Belgium
- Published
- 1994
27. Mechanisms of Stimulation of Insulin Release By Fatty-acids
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Warnotte, Catherine, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, 29th General Assembly of the European Association for the study of diabetes, UCL - MD/FSIO - Département de physiologie et pharmacologie, Warnotte, Catherine, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, and 29th General Assembly of the European Association for the study of diabetes
- Published
- 1993
28. A Dual Role of Atp in the Control of Insulin Release
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/NOPS - Département de neurologie et de psychiatrie, UCL - (SLuc) Service de psychiatrie adulte, de Timary, Philippe, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, 29th General Assembly of the European Association for the study of diabetes, UCL - MD/FSIO - Département de physiologie et pharmacologie, UCL - MD/NOPS - Département de neurologie et de psychiatrie, UCL - (SLuc) Service de psychiatrie adulte, de Timary, Philippe, Gilon, Patrick, Nenquin, Myriam, Henquin, Jean-Claude, and 29th General Assembly of the European Association for the study of diabetes
- Published
- 1993
29. Vanadate stimulation of insulin release in normal mouse islets
- Author
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UCL - MD/FSIO - Département de physiologie et pharmacologie, Zhang, Anqi, Gao, ZHI-YONG, Gilon, Patrick, Nenquin, Myriam, Drews, Gisela, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Zhang, Anqi, Gao, ZHI-YONG, Gilon, Patrick, Nenquin, Myriam, Drews, Gisela, and Henquin, Jean-Claude
- Abstract
The effects of vanadate (Na3VO4) on pancreatic B-cell function were studied in normal mouse islets. Vanadate did not affect basal insulin release but potentiated the effect of 7-30 mM glucose at concentrations of 0.1-1 mM. This effect was progressive and slowly reversible. It was abolished by omission of extracellular Ca2+ but unaffected by blockers of adrenergic or muscarinic receptors. Comparison of the changes in membrane potential, 86Rb efflux and 45Ca efflux that vanadate and ouabain produced in B-cells made it possible to exclude the hypothesis that vanadate increases insulin release by blocking the sodium pump. Vanadate was also without effect on cAMP levels. On the other hand, it markedly changed the characteristics of the Ca(2+)-dependent electrical activity and of the oscillations of cytoplasmic Ca2+ recorded in B-cells stimulated by 15 mM glucose. In the steady state, Ca2+ influx was increased by vanadate, and this resulted in a rise in cytoplasmic Ca2+. The exact mechanisms underlying these changes could not be established but a blockade of K channels was excluded. In the presence of LiCl, vanadate markedly increased inositol phosphate levels in islet cells. This effect was attenuated but not suppressed by omission of Ca2+. A small increase in inositol bisphosphate was still produced by vanadate in the absence of LiCl. These results suggest that vanadate both stimulates phosphoinositide breakdown and inhibits inositol phosphate degradation. In conclusion, vanadate does not induce insulin release, but markedly potentiates the stimulation by glucose. This property is not due to an inhibition of the sodium pump or to a rise in cAMP concentration. It results from a complex interplay between changes in B-cell membrane potential, phosphoinositide metabolism and Ca2+ handling.
- Published
- 1991
30. Galanin and Epinephrine Act On Distinct Receptors To Inhibit Insulin Release By the Same Mechanisms Including An Increase in K+ Permeability of the B-cell Membrane
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Drews, G., Debuyser, A., Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Drews, G., Debuyser, A., Nenquin, Myriam, and Henquin, Jean-Claude
- Published
- 1990
31. Comparison of the inhibition of insulin release by activation of adenosine and alpha 2-adrenergic receptors in rat beta-cells.
- Author
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UCL - MD/FSIO - Département de physiologie et pharmacologie, Bertrand, G., Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Bertrand, G., Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
Rat islets were used to compare the mechanisms whereby adenosine and adrenaline inhibit insulin release. Adenosine (1 microM-2.5 mM) and its analogue N6(-)-phenylisopropyladenosine (L-PIA) (1 nM-10 microM) caused a concentration-dependent but incomplete (45-60%) inhibition of glucose-stimulated release. L-PIA was more potent than D-PIA [the N6(+) analogue], but much less than adrenaline, which caused nearly complete inhibition (85% at 0.1 microM). 8-Phenyltheophylline prevented the inhibitory effect of L-PIA and 50 microM-adenosine, but not that of 500 microM-adenosine or of adrenaline. In contrast, yohimbine selectively prevented the inhibition by adrenaline. Adenosine and L-PIA thus appear to exert their effects by activating membrane A1 receptors, whereas adrenaline acts on alpha 2-adrenergic receptors. Adenosine, L-PIA and adrenaline slightly inhibited 45Ca2+ efflux, 86Rb+ efflux and 45Ca2+ influx in glucose-stimulated islets. The inhibition of insulin release by adenosine or L-PIA was totally prevented by dibutyryl cyclic AMP, but was only attenuated when adenylate cyclase was activated by forskolin or when protein kinase C was stimulated by a phorbol ester. Adrenaline, on the other hand, inhibited release under these conditions. It is concluded that inhibition of adenylate cyclase, rather than direct changes in membrane K+ and Ca2+ permeabilities, underlies the inhibition of insulin release induced by activation of A1-receptors. The more complete inhibition mediated by alpha 2-adrenergic receptors appears to result from a second mechanism not triggered by adenosine.
- Published
- 1989
32. The muscarinic receptor subtype in mouse pancreatic B-cells.
- Author
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UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Nenquin, Myriam, UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, and Nenquin, Myriam
- Abstract
Isolated mouse islets were used to identify the muscarinic receptor subtype present in pancreatic B-cells. We thus compared the inhibitory potencies of atropine (non-specific), of pirenzepine (specific for M1 receptors) and of compound AF-DX 116 (specific for cardiac M2 receptors) on acetylcholine-induced insulin release, 86Rb+ efflux and 45Ca2+ efflux. The three antagonists inhibited all effects of acetylcholine, but EC50 values were markedly different: atropine = 1.5-5 nM, pirenzepine = 0.6-1.7 microM and AF-DX 116 = 1.7-11 microM. The results did not suggest that the various effects of ACh could result from the activation of different subtypes of receptors. It is concluded that muscarinic receptors of pancreatic B-cells belong to an M2 subtype distinct from the cardiac M2 receptors.
- Published
- 1988
33. Stimulation of insulin release by benzoic acid derivatives related to the non-sulphonylurea moiety of glibenclamide: structural requirements and cellular mechanisms.
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Garrino, M G, Nenquin, Myriam, UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Garrino, M G, and Nenquin, Myriam
- Abstract
A decrease in membrane permeability to K+ is the first critical event occurring in pancreatic B-cells upon stimulation by hypoglycemic sulphonylureas. Compound HB 699 (4-[2-(5-chloro-2-methoxybenzamido)ethyl]benzoic acid), the non-sulphonylurea moiety of glibenclamide stimulates B-cells by the same mechanisms as glibenclamide itself. Selected derivatives of HB 699 were used to test, with isolated mouse islets, whether this property is due to the benzoic acid end of the molecule (not present in glibenclamide) or to another active site (also present in glimenclamide). Of the two halves of HB 699, p-ethylbenzoic acid, but not 5-Cl-2-methoxybenzamide, was weakly effective. Replacement of the carboxyl group of HB 699 by various non-acidic groups decreased but did not abolish the ionic and secretory effects on B-cells. Modifications of the other end of the molecule altered the efficacy in both directions. Removal of the substituents on the benzamide ring decreased the efficacy, whereas replacement of the 5-Cl-2-methoxybenzyl group by a 1,1-diphenylethyl group or a 9-fluorenylmethyl group led to substantially more active compounds. Their cellular mode of action was however not modified. It is concluded that compound HB 699 contains two active sites, both of which can trigger insulin release by decreasing K+ permeability of the B-cell membrane. K channels appear to possess, not a sulphonylurea receptor, but a target site for various chemical groups. The chemical environment of the latter may also determine their efficacy by modulating their access to the channel.
- Published
- 1987
34. Effects of acute sodium omission on insulin release, ionic flux and membrane potential in mouse pancreatic B-cells.
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, de Miguel, R, Tamagawa, T., Schmeer, W., Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, de Miguel, R, Tamagawa, T., Schmeer, W., Nenquin, Myriam, and Henquin, Jean-Claude
- Abstract
The effects of acute omission of extracellular Na+ on pancreatic B-cell function were studied in mouse islets, using choline and lithium salts as impermeant and permeant substitutes, respectively. In the absence of glucose, choline substitution for Na+ hyperpolarized the B-cell membrane, inhibited 86Rb+ and 45Ca2+ efflux, but did not affect insulin release. In contrast, Li+ substitution for Na+ depolarized the B-cell membrane and caused a Ca2+-independent, transient acceleration of 45Ca2+ efflux and insulin release. Na+ replacement by choline in the presence of 10 mM glucose and 2.5 mM Ca2+ again rapidly hyperpolarized the B-cell membrane. This hyperpolarization was then followed by a phase of depolarization with continuous spike activity, before long slow waves of the membrane potential resumed. Under these conditions, 86Rb+ efflux first decreased before accelerating, concomitantly with marked and parallel increases in 45Ca2+ efflux and insulin release. In the absence of Ca2+, 45Ca2+ and 86Rb+ efflux were inhibited and insulin release was unaffected by choline substitution for Na+. Na+ replacement by Li+ in the presence of 10 mM glucose rapidly depolarized the B-cell membrane, caused an intense continuous spike activity, and accelerated 45Ca2+ efflux, 86Rb+ efflux and insulin release. In the absence of extracellular Ca2+, Li+ still caused a rapid but transient increase in 45Ca2+ and 86Rb+ efflux and in insulin release. Although not indispensable for insulin release, Na+ plays an important regulatory role in stimulus-secretion coupling by modulating, among others, membrane potential and ionic fluxes in B-cells.
- Published
- 1988
35. Distinct Mechanisms for 2 Amplification Systems of Insulin Release
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Bozem, M., Schmeer, W., Nenquin, Myriam, UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Bozem, M., Schmeer, W., and Nenquin, Myriam
- Published
- 1987
36. The Ionic, Electrical, and Secretory Effects of Protein-kinase-c Activation in Mouse Pancreatic B-cells - Studies With a Phorbol Ester
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Bozem, M., Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Bozem, M., Nenquin, Myriam, and Henquin, Jean-Claude
- Published
- 1987
37. Magnesium Uptake By Pancreatic-islet Cells Is Modulated By Stimulators and Inhibitors of the B-cell Function
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Nenquin, Myriam, Awouters, P., Cogneau, M., UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Nenquin, Myriam, Awouters, P., and Cogneau, M.
- Published
- 1986
38. Mechanism of the Stimulation of Insulin Release Invitro By Hb-699, a Benzoic-acid Derivative Similar To the Non-sulfonylurea Moiety of Glibenclamide
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Garrino, MG., Schmeer, W., Nenquin, Myriam, Meissner, HP., Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Garrino, MG., Schmeer, W., Nenquin, Myriam, Meissner, HP., and Henquin, Jean-Claude
- Published
- 1985
39. Sparteine Increases Insulin Release By Decreasing the K+ Permeability of the B-cell Membrane
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Paolisso, G., Nenquin, Myriam, Schmeer, W., Mathot, F., Meissner, HP., Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Paolisso, G., Nenquin, Myriam, Schmeer, W., Mathot, F., Meissner, HP., and Henquin, Jean-Claude
- Published
- 1985
40. Nutrient Insulin Secretagogues Decrease Ca-45(2+) Efflux From Islet Cells By a Mechanism Other Than the Inhibition of the Na+-ca2+ Countertransport
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Demiguel, R., Garrino, MG., Hermans, Michel, Nenquin, Myriam, UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Demiguel, R., Garrino, MG., Hermans, Michel, and Nenquin, Myriam
- Published
- 1985
41. Effects of a Calcium-channel Agonist On the Electrical, Ionic and Secretory Events in Mouse Pancreatic B-cells
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Schmeer, W., Nenquin, Myriam, Meissner, HP., UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Schmeer, W., Nenquin, Myriam, and Meissner, HP.
- Published
- 1985
42. The Effects of Cesium-chloride On Insulin Release, Ionic Fluxes and Membrane-potential in Pancreatic B-cells
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Paolisso, G., Nenquin, Myriam, Meissner, HP., Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Paolisso, G., Nenquin, Myriam, Meissner, HP., and Henquin, Jean-Claude
- Published
- 1985
43. Distinct Effects of Acetylcholine and Glucose On Ca-45 and Rb-86 Efflux From Mouse Pancreatic-islets
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Nenquin, Myriam, Awouters, P., Mathot, F., Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Nenquin, Myriam, Awouters, P., Mathot, F., and Henquin, Jean-Claude
- Published
- 1984
44. Forskolin Suppresses the Slow Cyclic Variations of Glucose-induced Electrical-activity in Pancreatic B-cells
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Schmeer, W., Nenquin, Myriam, Meissner, HP., UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Schmeer, W., Nenquin, Myriam, and Meissner, HP.
- Published
- 1984
45. Diazoxide and D600 Inhibition of Insulin Release - Distinct Mechanisms Explain the Specificity for Different Stimuli
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Charles, S., Nenquin, Myriam, Mathot, F., Tamagawa, T., UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Charles, S., Nenquin, Myriam, Mathot, F., and Tamagawa, T.
- Published
- 1982
46. Glucose Modulates Mg-2+ Fluxes in Pancreatic-islet Cells
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Tamagawa, T., Nenquin, Myriam, Cogneau, M., UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Tamagawa, T., Nenquin, Myriam, and Cogneau, M.
- Published
- 1983
47. Does Protein Kinase-c Link Glucose-metabolism To B-cell Membrane Depolarization
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Schmeer, W., Nenquin, Myriam, Plant, TD., UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Schmeer, W., Nenquin, Myriam, and Plant, TD.
- Published
- 1989
48. Comparison of the Effects of Adenosine and Adrenaline in Rat B-cells
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Bertrand, G., Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Bertrand, G., Nenquin, Myriam, and Henquin, Jean-Claude
- Published
- 1988
49. How Does Activation of Protein-kinase-c Amplify the B-cell Response To Glucose
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Bozem, M., Nenquin, Myriam, Henquin, Jean-Claude, UCL - MD/FSIO - Département de physiologie et pharmacologie, Bozem, M., Nenquin, Myriam, and Henquin, Jean-Claude
- Published
- 1986
50. Mechanisms of Magnesium Efflux From Islet Cells - Analogies With and Differences From Calcium Efflux
- Author
-
UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Nenquin, Myriam, Cogneau, M., Tamagawa, T., UCL - MD/FSIO - Département de physiologie et pharmacologie, Henquin, Jean-Claude, Nenquin, Myriam, Cogneau, M., and Tamagawa, T.
- Published
- 1984
Catalog
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