boa revisÃo sulfonilurÉias
TRANSCRIPT
Sulfonylurea action re-revisited
Sulfonylureas (SU), commonly usedin the treatment of type 2 diabetesmellitus (T2DM), stimulate insulinsecretion by inhibiting adenosinetriphosphate (ATP)-sensitive K+ (KATP)channels in pancreatic b-cells. SU arenow known to also activate cyclicadenosine monophosphate (cAMP)sensor Epac2 (cAMP-GEFII) to Rap1signaling, which promotes insulinsecretion. The different effects ofvarious SU on Epac2 ⁄ Rap1 signaling,as well as KATP channels in differenttissues, underlie the diverse pancre-atic and extra-pancreatic actions ofSU. (J Diabetes Invest, doi: 10.1111 ⁄j.2040-1124.2010.00014.x, 2010)
Although earlier studies have suggestedvarious mechanisms of sulfonylurea (SU)action, the discovery of KATP channels byelectrophysiology brought a breakthroughin the understanding of the mechanismof the action of SU as well as the mecha-nism of glucose-stimulated insulin secre-tion. KATP channels were first reported incardiac cell membranes and were laterdescribed in many other tissues includingpancreatic islet cells1. In 1985, Sturgesset al. found that tolbutamide inhibitsKATP channels in pancreatic b-cells, sug-gesting that the channels are the target ofSU2. In 1995, Aguilar-Bryan et al. clonedthe SU receptor (now called SUR1) fromthe pancreatic b-cell cDNA libraries3.SUR1 belongs to members of the adeno-sine triphosphate (ATP)-binding cassette(ABC) protein superfamily. At almost thesame time, we cloned Kir6.24, a memberof the inwardly rectifying K+ channel
family, and showed for the first time thatthe b-cell KATP channel is composed ofKir6.2 and SUR1.4 The KATP channel is ahetero-octameric complex comprisingtwo subunits: a pore-forming subunitKir6.x (Kir6.1 or Kir6.2) and a regula-tory subunit SURx (SUR1, SUR2A orSUR2B)5. Different combinations ofKir6.1 or Kir6.2 and SUR1 or a SUR2variant (mix and match) form KATP
channels with differing nucleotides andSU sensitivities that play distinct physio-logical and pathophysiological roles indifferent tissues5,6. While Kir6.2 plusSUR1 constitutes pancreatic b-cell KATP
channels, Kir6.2 plus SUR2A constitutescardiac and skeletal muscle KATP chan-nels. Kir6.2 plus SUR2B constitutessmooth muscle KATP channels and Kir6.1plus SUR2B constitutes vascular smoothmuscle KATP channels, both of which aresomewhat ATP-insensitive, nucleotidediphosphate-activated and glibenclamide-sensitive K+ channels. SU actions wererevisited after the cloning of the variousKATP channels7.
Mice lacking KATP channels (Kir6.2null mice and SUR1 null mice) were gen-erated6. Neither glucose nor tolbutamidestimulation elicited any change in [Ca2+]i
in Kir6.2 null b-cells. Importantly, neitherglucose nor tolbutamide stimulationcaused a significant insulin secretion inKir6.2 null mice. Examination of SUR1null mice also confirmed that both glu-cose-stimulated and sulfonylurea-stimu-lated insulin secretion depend criticallyon the activity of b-cell KATP channels.Based on these findings, it is generallyaccepted that the primary target of SU isSUR1 and that action of SU is mediatedby closure of the KATP channels throughbinding to SUR1.
Cyclic adenosine monophosphate(cAMP) is a universal intracellular secondmessenger involved in the regulation ofvarious cellular functions in many celltypes. cAMP has long been considered to
exert its action through protein phosphor-ylation by protein kinase A (PKA). How-ever, a novel cAMP-binding proteinfamily, termed Epac (exchange proteinactivated by cAMP) or cAMP-GEF(cAMP-regulated guanine nucleotideexchange factor) has been identified8.There are two members of the Epac fam-ily, Epac1 and Epac2, both of which pos-sess guanine nucleotide exchange factor(GEF) activity towards Rap1, the smallmolecular weight GTP-binding protein, ina cAMP-dependent manner. We showedthat Epac2 is involved in the potentiationof cAMP-dependent, PKA-independentinsulin secretion9. By studying Epac2 nullmice, we recently found that Epac2 ⁄ Rap1signaling is especially important in earlyphase (first phase) potentiation by cAMPof glucose-stimulated insulin granule exo-cytosis10. We have proposed a model inwhich Epac2 ⁄ Rap1 signaling regulatescAMP-induced insulin granule exocytosisby controlling the size of a readily releas-able pool (RPP), most likely through theregulation of granule density near theplasma membrane10.
In the course of the studies of Epac2-mediated mechanisms of insulin secre-tion, we developed a fluorescenceresonance energy transfer (FRET)-basedEpac2 sensor (termed C-Epac2-Y) inwhich the full-length Epac2 is fusedamino-terminally to enhanced cyan fluo-rescent protein (ECFP) and carboxyl-ter-minally to enhanced yellow fluorescentprotein (EYFP)11. Epac2 is a closed formin the inactive state8, so that ECFP andEYFP are located very closely to eachother (within 10 nm), which causesFRET. On cAMP binding to Epac2,Epac2 changes its conformation to anopen form. As a result, ECFP and EYFPseparate away, so that FRET does notoccur (active state)8. Utilizing this princi-ple, we are able to monitor the activationstatus of Epac2. In the search for agentsthat activate Epac2 using this FRET
*Corresponding author. Susumu SeinoTel.: +81-78-382-5860 Fax: +81-78-382-6762E-mail address: [email protected] 19 January 2010; accepted 22 January 2010
C O M M E N T A R Y
ª 2010 Asian Association for the Study of Diabetes and Blackwell Publishing Asia Pty Ltd Journal of Diabetes Investigation Volume 1 Issue 1/2 February/April 2010 37
sensor, we found that tolbutamide, gli-benclamide, chlorpropamide, acetohexa-mide and glipizide significantly decreasedthe FRET response in COS-1 cells trans-fected with the Epac2 FRET sensor in dif-ferent degrees and varying kinetics,suggesting strongly that these SU activateEpac2. However, gliclazide, another SU,did not decrease the FRET response.Direct binding of SU to Epac2 was con-firmed by specific binding of radiolabeledglibenclamide to Epac2 expressed inCOS-1 cells. We also found that tolbuta-mide and glibenclamide activate Rap1 inclonal pancreatic b-cells (MIN6 cells),but gliclazide does not. In addition, tol-butamide-stimulated insulin secretionand glibenclamide-stimulated insulinsecretion from isolated pancreatic isletsof Epac2 null mice were significantlyreduced, compared with those of wild-type mice. However, there was no sig-nificant difference in insulin secretion inresponse to gliclazide. Furthermore, theinsulin response to the oral administra-tion of tolbutamide alone or concomi-tant administration of glucose andtolbutamide in Epac2 null mice was sig-nificantly reduced, compared with thatin wild-type mice, and the glucose low-ering effect of tolbutamide in Epac2 null
mice was significantly less than that inwild-type mice.
As described above, it is well estab-lished that SU stimulate insulin secretionby eliciting a series of ionic events includ-ing closure of KATP channels, openingof voltage-dependent Ca2+ channels(VDCC), and Ca2+ influx into the b-cells.Although closure of the KATP channels isa prerequisite for SU to stimulate insulinsecretion, the activation of Epac2 ⁄ Rap1signaling is required for SU to exert theirfull effects in insulin secretion (except inthe case of gliclazide). Considering therole of Epac2 ⁄ Rap1 signaling in insulingranule exocytosis10, SU might increasethe size of a readily releasable pool ofinsulin granules near the plasma mem-brane (Figure 1).
A two-site (A-site and B-site) modelfor the interaction of SU and glinideswith SUR has been proposed6. The A-siteis located on the eighth (between trans-membrane segment (TM) 15 and 16)cytosolic loop, which is specific for SUR1,and the B-site involves the third (betweenTM 5 and 6) cytosolic loop, which is verysimilar in all SUR. Based on this model,SU and glinides can be divided into threegroups. The first group (which includestolbutamide, gliclazide and nateglinide)
binds specifically to the A-site of SUR1;the second group (which includes gliben-clamide and glimepiride) binds to theB-sites of both SUR1 and SUR2A as wellas the A-site of SUR1; and the thirdgroup (which includes meglinitide andrepaglinide) binds to the B-site of SUR1and SUR2A. In addition, SU, with theexception of gliclazide, activate Epac2 ⁄Rap1 signaling, whereas glinides do not.Thus, different SU and glinides have dif-ferent mechanisms of action in insulinsecretion in terms of specificities forSUR1 and Epac2.
Mutations of Kir6.2 have recentlybeen shown to cause neonatal diabetesmellitus (ND) with varying degrees ofseverity12. In most ND patients, insulininjection can be replaced by high-doseSU orally. Studies by Zhang et al. sug-gest that the effectiveness of SU in thetreatment of ND patients might vary,depending on the properties of theSU11.
Incretin-related drugs such as analogsof glucagon-like peptide 1 (GLP-1) anddipeptidyl peptidase IV (DPP-IV) inhibi-tors, which potentiate insulin secretionthrough cAMP signaling in pancreaticb-cells, are currently being used as newhypoglycemic agents to treat T2DM.Because Epac2 is also required for poten-tiation of insulin secretion by cAMP, it isa target of both SU and incretin-relateddrugs. There are many basic and clinicalquestions yet to be answered. Where isthe SU binding site in Epac2? Is thereany additive or synergistic effect of cAMPand SU on activation of Epac2 ⁄ Rap1 sig-naling? Is there any accessory protein thatmight facilitate direct interaction of SUand Epac2? Is Epac2 ⁄ Rap1 signalinginvolved in the extrapancreatic effectsof SU and incretin-related drugs andwhich SU has the least adverse effect? IsEpac2 ⁄ Rap1 signaling involved in the sec-ondary failure of SU and incretin-relateddrugs, and which SU shows least second-ary failure? What is the best combinationof SU and incretin-related drugs for themost beneficial effect for treatment ofT2DM in terms of insulin secretion,glycemic control and adverse effects?Answers to these questions are required
Figure 1 | Model of sulfonylurea (SU) action in insulin secretion. Closure of KATP channels is essen-tial for SU to stimulate insulin secretion. Activation of Epac2 ⁄ Rap1 signaling is required for SU toexert their full effect on insulin secretion. cAMP, cyclic adenosine monophosphate; GIP, glucose-dependent insulinotropic polypeptide; GLP-1, glucagon-like peptide 1; PKA, protein kinase A; RRP,readily releasable pool; SUR, SU receptor; VDDC, voltage-dependent Ca2+ channels.
38 Journal of Diabetes Investigation Volume 1 Issue 1/2 February/April 2010 ª 2010 Asian Association for the Study of Diabetes and Blackwell Publishing Asia Pty Ltd
Seino et al.
to provide a basis of beneficial treatmentof T2DM. Thus, the actions of the SUmust be re-revisited.
Susumu Seino1,2,3*, Chang-LiangZhang1,4, Tadao Shibasaki1
1Division of Cellular and MolecularMedicine, Department of Physiology and
Cell Biology and 2Division of Diabetes,Metabolism and Endocrinology,
Department of Internal Medicine, KobeUniversity Graduate School of Medicine,
Kobe, 3Core Research for EvolutionalScience and Technology (CREST), Japan
Science and Technology Agency, Saitamaand 4Department of Neurology, Kyoto
University Graduate School of Medicine,Kyoto, Japan
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ª 2010 Asian Association for the Study of Diabetes and Blackwell Publishing Asia Pty Ltd Journal of Diabetes Investigation Volume 1 Issue 1/2 February/April 2010 39
Sulfonylurea action