ATP-Sensitive K+ Channel Modulator Binding to Sulfonylurea Receptors SUR2A and SUR2B: Opposite Effects of MgADP

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Vol. 55, Issue 5, 832-840, May 1999

ATP-Sensitive K⁺ Channel Modulator Binding to Sulfonylurea Receptors SUR2A and SUR2B: Opposite Effects of MgADP

Annette Hambrock, Cornelia Löffler-Walz, Doris Kloor, Ursula Delabar, Yoshiyuki Horio, Yoshihisa Kurachi, and Ulrich Quast

Department of Pharmacology, University of Tübingen, Tübingen, Germany (A.H., C.L-W., D.K., U.D., U.Q.); and Department of Pharmacology II, Faculty of Medicine, Osaka University, Osaka, Japan (Y.H., Y.K.)

	Summary

Top Summary Introduction Experimental Procedures Results Discussion References

K_ATP channels are heteromeric complexes of inwardly rectifying K⁺ channel subunits and sulfonylurea receptors (SURs). SUR2A andSUR2B, which differ within the carboxyl terminal exon 38, arecharacteristic for the cardiac and smooth muscle type channels,respectively. Here we compare binding of the tritiated K_ATP channelopener, [³H]P1075, to membranes from human embryonic kidney (HEK) cellstransfected with murine SUR2A and 2B at 37°C. Binding to bothSURs required addition of Mg²⁺ and ATP in the low micromolar range. In the presence of MgATP,micromolar concentrations of MgADP, formed by the ATPase activityof the membrane preparation, increased binding to SUR2A but inhibitedbinding to SUR2B. Decreasing temperatures strongly reduced [³H]P1075 binding to SUR2A, whereas binding to SUR2B was increasedin a bell-shaped manner. Kinetic experiments revealed a fasterdissociation of the [³H]P1075-SUR2A complex, whereas the association rate constantsfor [³H]P1075 binding to SUR2A and 2B were similar. Openers inhibited[³H]P1075 binding to SUR2A with potencies $approx$ 4 times lower than toSUR2B; in contrast, glibenclamide inhibited [³H]P1075 binding to SUR2A $approx$ 8 times more potently than to SUR2B.The data suggest that SUR2A and 2B represent the opener receptorsof cardiac and vascular smooth muscle K_ATP channels, respectively,and show that MgADP is an important modulator of opener bindingto SUR. The different carboxyl termini of SUR2A and 2B lead todifferences in the MgADP dependence and the thermodynamics of[³H]P1075 binding, as well as in the affinities for openers andglibenclamide, underlining the importance of this part of themolecule for K_ATP channel modulatorbinding.

	Introduction

Top Summary Introduction Experimental Procedures Results Discussion References

ATP-sensitive K⁺ channels (K_ATP channels), first discovered in the heart (Noma, 1983; Trube and Hescheler, 1984), link themembrane potential to the metabolic state of the cell as reflectedby the levels of nucleoside triphosphates and diphosphates (Ashcroftand Ashcroft, 1990; Quast, 1996; Yokoshiki et al., 1998). K_ATPchannels have been shown to be a heteromeric complex of pore-formingsubunits, which belong to the class of inwardly rectifying K⁺ channels (Kir6.x), and of sulfonylurea binding subunits (SURs)(Inagaki et al., 1995; Sakura et al., 1995; reviews: Ashcroftand Gribble, 1998; Babenko et al., 1998). SURs are members ofthe ATP binding cassette proteins (ABC proteins) and contain bindingsites for sulfonylureas and nucleotides (Aguilar-Bryan et al.,1995; Inagaki et al., 1996; Isomoto et al., 1996). Based on multisequencealignments and hydropathy analyses, the classical topology ofABC proteins (i.e., 12 transmembrane helices with two intracellularnucleotide binding folds) has been proposed for the SURs withan extension of five transmembrane helices at the N terminus (Tusnádyet al., 1997). Electrophysiological studies on recombinant K_ATPchannels have shown that the SURs confer on the channel complexthe sensitivity to the sulfonylureas, the openers, and the activatingnucleotides and that they account for the major pharmacologicaldifferences between the K_ATP channels in various tissues (review:Babenko et al., 1998). The channel of the pancreatic $beta$ -cell containsSUR1 (Inagaki et al., 1995; Sakura et al., 1995); current evidencesuggests that the SUR in heart and skeletal muscle is SUR2A (Inagakiet al., 1996) and that in smooth muscle it is SUR2B (Isomoto etal., 1996; Yamada et al., 1997). In the SURs cloned to date (human,rat, and murine) there are species differences in the amino acidsequence (Isomoto et al., 1996; Aguilar-Bryan et al., 1998). However,SUR2A and 2B of the same species are splice variants differingonly within the last carboxyl terminal exon (Aguilar-Bryan etal., 1998); in the case of the murine SUR2 isoforms, this involvesthe last 42 amino acids (Isomoto et al., 1996).

Recent studies examining the binding of the tritiated K_ATP channel opener [³H]P1075 ([³H]-N-cyano-N'-(1,1-dimethylpropyl)-N"-3-pyridylguanidine; Brayand Quast, 1992) to recombinant SUR2A (rat SUR2A, Schwanstecheret al., 1998) and SUR2B (murine SUR2B, Hambrock et al., 1998;human SUR2B, Schwanstecher et al., 1998) have provided strongsupport for the contention that these SURs are indeed the receptorsfor openers and sulfonylureas of the native K_ATP channels in cardiacand vascular smooth muscle. Binding studies with [³H]P1075 to rat cardiocytes in culture (Lemoine et al., 1996) andto cardiac membranes from rat (Löffler-Walz and Quast, 1998)and dog (Atwal et al., 1998), as well as to rat aortic rings (Brayand Quast, 1992; Quast et al., 1993), have provided detailed informationon the ligand binding properties of native cardiac and vascularK_ATPchannels.

In this study we investigated [³H]P1075 binding to membranes from human embryonic kidney (HEK)293 cells transfected with murineSUR2A and 2B. In agreement with other studies (Hambrock et al.,1998; Schwanstecher et al., 1998) we found that opener bindingto SUR requires the presence of MgATP; the EC₅₀ values were 5µM (SUR2A) and 3 µM (SUR2B). HPLC analysis, however, showed, thatmost of the nucleotide (3 µM ATP) added to the solution had beenhydrolyzed at the end of the incubation period. In addition, weshow for the first time that MgADP, which opens the channel byinteracting with SUR (Nichols et al., 1996; Satoh et al., 1998;reviews: Ashcroft and Gribble, 1998; Babenko et al., 1998), alsoaffects opener binding to SUR2A and 2B, modulating it in oppositedirections. Significant differences between the two SURs werealso observed in the kinetics and thermodynamics of [³H]P1075 binding and the modulator bindingprofile.

	Experimental Procedures

Top Summary Introduction Experimental Procedures Results Discussion References

Cell Culture, Transfection, and Membrane Preparation. HEK 293 cells were cultured in plastic dishes with a diameter of 9.4 cm at 37°C in a humidified atmosphere with 95% air and5% CO₂ in minimum essential medium (MEM) containing glutamineand supplemented with 10% fetal bovine serum and 20 µg ml¹ gentamycin. At 60 to 80% confluence (10-16 million cells perdish), cells were transfected with the pcDNA 3.1 vector (Invitrogen,San Diego, CA) containing the coding sequence of murine SUR2Aor murine SUR2B (GenBank accession numbers D86037 and D86038,respectively; Isomoto et al., 1996). Transfections were performedusing lipofectAMINE and OPTIMEM (Life Technologies, Eggenstein,Germany) according to the manufacturer's instructions with 4 µgDNA and 25 µl lipofectAMINE per culture dish. Cells were allowedto express transfected DNA for 48 h. Control experiments wereperformed by omitting either DNA or lipofectAMINE. Isolation ofstably transfected cells was achieved as described previously(Hambrock et al., 1998).

Membranes from control and from stably transfected cells were prepared at a confluence of 70 to 80% (13-16 million cells perdish). Cells were suspended by rinsing with medium and centrifugedfor 6 min at 500 g at 4°C. The pelleted cells were lysed by additionof ice-cold hypotonic buffer (5 ml per culture dish) containing:10 mM HEPES and 1 mM EGTA at pH 7.4. Cell rupture was assuredby microscopy and the lysate centrifuged at 10⁵ g and 4°C for 60 min. The resulting membrane pellet was resuspendedin a buffer containing: 5 mM HEPES, 5 mM KCl, 139 mM NaCl, and0 or 1 mM MgCl₂ (see below) at pH 7.4 and 4°C at a protein concentrationof $approx$ 3.0 mg ml¹ (SUR2A) or $approx$ 1.5 mg ml¹ (SUR2B) and frozen at $-$ 80°C. Protein concentration was determinedaccording to Lowry et al. (1951)

using BSA as thestandard.

Kinetics of [³H]P1075 Binding. Membranes were thawed and homogenized with a polytron homogenizer for 2 × 5 s at 10⁴ rpm at 4°C. To measure the association kinetics, membranes [finalprotein concentration: 200 µg ml¹ (SUR2A) and 50 µg ml¹(SUR2B)] were added to the incubation buffer containing: 139 mMNaCl, 5 mM KCl, 5 mM HEPES, 3.8 mM MgCl₂, and 3 mM Na₂ATP, sothat the concentration of free Mg²⁺ was 1 mM (see below) and were supplemented with [³H]P1075 (2-5 nM) at 37°C. Aliquots (300 µl) were withdrawn atdifferent times for separation of bound and free ligand by dilutioninto 8 ml of ice-cold quench solution (50 mM Tris and 154 mM NaCl,pH 7.4) and rapid filtration under vacuum over Whatman GF/B filters.Filters were washed twice with 8 ml of ice-cold quench solutionand counted for ³H in the presence of 6 ml of scintillant (Ultima Gold; PackardInstruments, Meriden, CT). Nonspecific binding was determinedin the presence of 10 µM unlabeled P1075 and did not change withtime. Because the label concentration (L) was in large excessover the concentrations of binding sites, the data were fittedto a single exponential as function of time (t),

<UP>B</UP>=<UP>Beq</UP> ∗ [1−<UP>exp</UP>(<UP>−</UP>k<UP>app</UP> ∗ <UP>t</UP>)] <UP>with</UP> (1)

k<UP>app</UP>=k<UP>+</UP> ∗ <UP>L</UP>+k<UP>−</UP>=k<UP>−</UP>(1+<UP>L</UP>/K<UP>D</UP>)

where B_eq denotes the concentration of the receptor-label complex at equilibrium and k_app the apparent rate constant of association.For a simple bimolecular association reaction, k_app depends onthe rate constants of association and dissociation (k₊, k)and on the concentration of L as written in eq. 1 (Tallarida,1995). K_D = k/k₊ is the equilibrium dissociationconstant.

Dissociation was initiated by addition of P1075 (10 µM) to the receptor-label complex at equilibrium after incubation of themembrane preparation with [³H]P1075 (1.5-3 nM) at 37°C for 10 min (SUR2A) or 30 min (SUR2B).Aliquots were then withdrawn to follow the dissociation kinetics,which were fitted to the equation of exponential decay,

<UP>B</UP>=<UP>B<SUB>eq</SUB></UP> ∗ <UP>exp</UP>(<UP>−</UP>k<SUB><UP>−</UP></SUB> ∗ <UP>t</UP>)

(2)

with B_eq and k defined asabove.

Equilibrium Competition Experiments. Membranes (SUR2A: 150 µg protein ml¹; SUR2B: 60 µg protein ml¹) were added to the incubation buffer described above containing[³H]P1075 (1.5-3 nM) and the inhibitor of interest in a total volumeof 1 ml at pH 7.4 and 37°C. After equilibrium had been reached(SUR2A: 13 min; SUR2B: 30 min), incubation was stopped by diluting0.3-ml aliquots in triplicate into 8 ml of ice-cold quench solutionand filtrating as indicated above. Concentration dependencieswere analyzed by fitting the logistic form of the Hill equation,

<UP>y</UP>=<UP>b</UP>+(<UP>a</UP>−<UP>b</UP>)/(1+10<UP>n ∗ </UP>(<UP>px</UP>−<UP>p</UP>K)). (3)

Here, b denotes the starting level of the curve, a the level at saturation, so that a-b represents the extent of the effect(amplitude); n (=n_H) is the Hill coefficient, x the concentrationof the compound under study and K the midpoint of the curve withpx = $-$ logx and pK = $-$ logK. The dependence of the midpoint of aninhibition curve (IC₅₀ value) on the concentration of the radioligand,L, was calculated according to the Cheng-Prusoff equation (Chengand Prusoff, 1973),

<UP>IC</UP>50=K<UP>i</UP> ∗ (1+<UP>L</UP>/K<UP>D</UP>) (4)

where K_i is the inhibition constant and K_D the equilibrium dissociation constant of theradioligand.

To measure the dependence of [³H]P1075 binding to SUR2A/2B on the free Mg²⁺ or the total ATP concentration, the concentrations of MgCl_2,EDTA, and Na₂ATP were adjusted as indicated in Results. Free Mg²⁺ concentrations in the presence of varying concentrations of ATP(added as Na₂ATP) and EDTA (1 mM) were calculated using a programwritten by Drs. T. Suzuki (Australian National University, Canberra,Australia) and U. Russ (University of Tübingen, Germany) usingthe pK values and enthalpies of the MgATP and MgEDTA complexescompiled by Smith and Martell (1989)

Determination of Nucleotides. Adenine nucleotides were analyzed with HPLC using a Grom-Sil 120 ODS-3 CP column (5 µm, 125 × 4 mm i.d.; Sykam, München,Germany) and an UV detector (UVIS 200; Sykam) for absorbance recordingat 254 nm. The column was eluted at 30°C with a flow rate of 1ml min^-1 and a low pressure gradient. Eluent A consisted of 65 mM potassiumphosphate, pH 4.6, and 5 mM tetrabutylammonium sulfate as ion-pairforming agent. Solvent B was solvent A + 40% (v/v) acetonitrile.The mobile phase was kept at 100% solvent A for 3 min after injectionof the sample (50 µl). After 4 min, a linear gradient was startedto increase solvent B to 23% at 10 min and to 60% at 17 min; thereafter,solvent B was kept to 60% for 3 min. To reequilibrate the system,solvent A had to be kept at 100% for 8 min before the next sampleinjection. The chromatogram was completed within 30 min. AMP,ADP, and ATP were identified by their retention times (AMP, 5.8min; ADP, 10.25 min; and ATP, 13.15 min) and quantified by peakarea measurement by means of online computing integrator (AXXIOMchromatographic system 747; Sykam). Samples were prepared as describedfor the equilibrium binding studies. Incubation was stopped byfiltration using FP 030/30 filters (Schleicher & Schuell, Dassel,Germany) and the filtrate stored immediately at $-$ 80°C for HPLCanalysis.

Data Analysis. Fits of the equations to the data were performed according to the method of least-squares using the FigP program (Biosoft,Cambridge, UK). Errors in the parameters derived from the fitto a single curve were estimated using the univariate approximation(Draper and Smith, 1981) and assuming that amplitudes and pK valuesare normally distributed. In the text, pK ± S.E.M. or K valueswith the 95% confidence interval in parentheses are given. Propagationof errors was taken into account according to Bevington (1969).

Materials. [³H]P1075 (specific activity 121 Ci mmol¹) was purchased from Amersham Buchler (Braunschweig, Germany). The reagents and mediaused for cell culture and transfection were purchased from LifeTechnologies. Na₂ATP was purchased from Boehringer Mannheim (Mannheim,Germany); EDTA and UTP were purchased from Fluka (Deisenhofen,Germany); and creatine phosphate, creatine kinase, phosphoenolpyruvate, and pyruvate kinase were purchased from Sigma (Deisenhofen,Germany). Acetonitril and tetrabutylammonium sulfate (HPLC grade)were obtained from Merck (Darmstadt, Germany). The following drugswere kind gifts of the pharmaceutical companies indicated in parentheses:aprikalim (Rhône-Poulenc Rorer, Paris, France), AZ-DF 265 (4-[[N-( $alpha$ -phenyl-2-piperidino-benzyl)carbamoyl]methyl] benzoic acid (Thomae, Biberach, Germany), diazoxide(Essex Pharma, München, Germany), levcromakalim (SmithKline-Beecham,Harlow, UK), nicorandil (Chugai, Tokyo, Japan), P1075 (N-cyano-N'-(1,1-dimethylpropyl)-N"-3-pyridylguanidine;Leo Pharmaceuticals, Ballerup, Denmark). Minoxidil sulfate andthe active enantiomer of pinacidil (( $-$ )pinacidil) were synthesizedby Dr. W. P. Manley (Novartis, Basel, Switzerland). Glibenclamidewas from Sigma. K_ATP channel modulators were dissolved in ethanoland dimethyl sulfoxide (1:1) and further diluted with the samesolvent or with incubation buffer; the final solvent concentrationin the assays was always below 0.3%.

	Results

Top Summary Introduction Experimental Procedures Results Discussion References

Kinetic Experiments. The association and dissociation kinetics of [³H]P1075 binding at 37°C to membranes from HEK cells transfected with SUR2A and2B are illustrated in Fig. 1. With SUR2A, the kinetics at 1.9nM [³H]P1075 were fast and close to the resolution limit of the filtrationassay (fastest sampling rate $approx$ 30 s per point). The rate constantof dissociation, k, was determined to 0.61 ± 0.01 min¹, corresponding to a half-time (T_1/2) of 1.1 min; the apparentrate constant of association, k_app, at 1.9 nM [³H]P1075 was 0.67 ± 0.03 min¹. Assuming a one-step bimolecular binding mechanism, the rateconstant of association, k₊, is calculated according to eq.1 to (3.2 ± 1.6)*10⁷ M¹ min¹, where the large error in this value follows from the laws oferror propagation (Bevington, 1969). From these kinetic values,K_D is calculated to 19 ± 10 nM, a value in excellent agreementwith the K_i value of 17 nM determined in equilibrium competitionexperiments (see Fig. 7 and Table 2. Figure 1A shows that after10 min, [³H]P1075 binding to SUR2A started to decline, and, after 30 min,tended to plateau at $approx$ 80%. Attempts to stabilize binding by couplingof ATP-regenerating systems like creatine kinase (20 U ml¹) and creatine phosphate (10 mM) or pyruvate kinase (20 U ml¹) and phosphoenol pyruvate (10 mM) in the presence of 13 mM Mg²⁺ did not improve stability, whereas in the presence of other nucleotideslike UTP or ATP $gamma$ S (3 mM, instead of ATP), stability decreased(data not shown). For equilibrium experiments, incubation wasstopped after 13 min when binding was still at its maximum; inview of the rapid kinetics (T_1/2 = 1.1 min), equilibrium was reached.

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Fig. 1. Kinetics of [³H]P1075 binding to membranes from HEK cells transfected with SUR2A (A) and SUR2B (B) at 37°C. A, $black-square$ , association of [³H]P1075 (1.9 nM) with SUR2A and

, dissociation of the complex, induced by addition of 10 µM unlabeled P1075 after 10 min. B,

, association of [³H]P1075 (4.8 nM) with SUR2B and $open circle$ , dissociation of the complex, addition of 10 µM unlabeled P1075 after 30 min. Note different time scales in A and B. Fit of monoexponential kinetics to data (n = 3) gave for k_app 0.67 ± 0.03/0.221 ± 0.006 min¹ and for k 0.61 ± 0.01/0.070 ± 0.002 min¹ for SUR2A/2B, respectively. Data are normalized to percentage of specific binding (B_s) at maximum, which was 57 ± 4/230 ± 10 fmol mg protein¹ for SUR2A/2B, respectively.

The kinetics of [³H]P1075 binding to SUR2B were considerably slower and binding was more stable (Fig. 1B). k was determinedto 0.070 ± 0.002 min¹, corresponding to T_1/2 = 10 min and, at 4.8 nM radiolabel, k_appwas 0.221 ± 0.006 min¹. Applying eq. 1, k₊ was calculated to (3.1 ± 0.1)*10⁷ M¹ min, i.e., identical with the estimate for SUR2A. From these values,a K_D value of 2.2 ± 0.2 nM was calculated in good agreement withthat determined from saturation binding and homologous competitionexperiments (3.4 nM at 1 mM [Mg²⁺]_free; Hambrock et al., 1998

). According to the slower kineticsobserved with SUR2B, incubation time for equilibrium experimentswas set to 30min.

ATP Saturation Curves. Figure 2A shows the dependence of [³H]P1075 binding to SUR2A on [ATP] at a total Mg²⁺ concentration of 2.2 mM. ATP supported binding with an EC₅₀ valueof 5 µM and Hill coefficient of 1. This value was 20 times lowerthan that found for the ATP dependence of [³H]P1075 binding in rat cardiac membranes (EC₅₀ = 100 µM; Löffler-Walzand Quast, 1998); however, the latter experiments had to be performedin the presence of an ATP-regenerating system to assure continuedpresence of ATP in spite of a high nucleotidase activity of thepreparation (Löffler-Walz and Quast, 1998; see also Dickinsonet al., 1997). Initially, we used the system also employed withcardiac membranes (Löffler-Walz and Quast, 1998), which consistedof creatine phosphate (20 mM), creatine kinase (50 U ml¹), and Mg²⁺ (25 mM) in the presence of 20 mM HEPES to preserve pH (Stryer,1995). Later experiments showed that with SUR₂ this could be reducedto creatine phosphate (3 mM), creatine kinase (5 U ml¹), Mg²⁺ (10 mM) and 10 mM HEPES, and these concentrations were used routinely.Adding these components to the incubation solution, the ATP-dependenceof [³H]P1075 binding to SUR2A was shifted from 5 to 110 µM, a valuesimilar to that observed in cardiac membranes. Control experimentsshowed that neither high Mg²⁺, nor creatine phosphate, nor the enzyme alone had any effectand that only the three components together produced the rightwardshift of the ATP activation curve (not illustrated).

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Fig. 2. Dependence of [³H]P1075 binding to SUR2A and 2B on total ATP concentration, [ATP]_o, and effect of an ATP-regenerating system. ATP was added as Na₂ATP. A, SUR2A: in absence ( $black-square$ )/presence (

) of an ATP-regenerating system, ATP activated binding to SUR2A with pEC₅₀ values of 5.30 ± 0.01/3.96 ± 0.05 and Hill coefficients = 0.97 ± 0.03/1.03 ± 0.11, respectively. B, SUR2B:

, absence of ATP-regenerating system: ATP activated binding with pEC₅₀ = 5.47 ± 0.08 and n_H = 1.04 ± 0.18; at ATP >1 mM, binding increased further to a final level of 166 ± 4%. $black-triangle$ , Addition of ATP as MgATP. $open circle$ , Presence of ATP-regenerating system. ATP activated binding with pEC₅₀ = 5.37 ± 0.04; amplitude = 183 ± 10%; n_H = 1.18 ± 0.11. Membranes (SUR2A/2B) were incubated with [³H]P1075 (2.5/1.5 nM) for 13/30 min at 37°C in presence of 2.2 mM Mg²⁺(n = 4 for each point). The ATP- regenerating system consisted of creatine phosphate (3 mM), creatine kinase (5 U ml¹), Mg²⁺ (10 mM) in presence of 10 mM HEPES to buffer pH against activity of the ATP-regenerating system that consumes 1 proton/cycle (Stryer, 1995

). Data were normalized with respect to (specific) binding at 1 mM ATP, which was 58 ± 3/150 ± 50 fmol mg protein¹ for SUR2A/SUR2B, respectively.

Figure 2B shows similar experiments performed with SUR2B. At 2.2 mM total Mg²⁺ and in the absence of the ATP-regenerating system, ATP enabled[³H]P1075 binding with an EC₅₀ value of 3 µM and Hill coefficientof 1 reaching a plateau normalized to 100% (binding at 1 mM ATP).Increasing [ATP] (added as Na₂ATP) beyond 1 mM led to a furtherincrease in binding up to 166%. When ATP was added as MgATP, thesecond phase was not observed (Fig. 2B). This indicated that theincrease in binding at [Na₂ATP] >1 mM was due to the increasingdepletion of the free Mg²⁺ concentration ([Mg²⁺]_free) by ATP. In the presence of the ATP-regenerating system,the midpoint of the activation curve remained unchanged; however,the amplitude increased to 180% (n = 4), i.e., to a value similarto that reached before by depletion of [Mg²⁺]_free (Fig. 2B).

MgADP Dependence. It was thought that the effects of the ATP-regenerating system reflected the depletion of ADP. This hypothesis was testedin experiments performed at 30 µM ATP, a concentration at which[³H]P1075 binding to both isoforms of SUR2 is essentially saturatedunder control conditions but where coupling of the ATP-regeneratingsystem should produce a major effect (Fig. 2). Indeed, addingthe ATP-regenerating system depressed binding to SUR2A to 45%but increased binding to SUR2B to 188% of control (Fig. 3). Additionof 1 mM ADP reversed the effects of the ATP-regenerating systemand brought binding back to control values (Fig. 3). Analogousexperiments were performed using the phosphoenolpyruvate (3 mM)/pyruvatekinase (5 U ml¹) system (Mg²⁺= 10 mM). Coupling of this system produced effects similar tothose obtained with the creatine-based system; again these changeswere reversed by addition of ADP (n = 3; not shown). These experimentsclearly show that it is depletion of ADP by the ATP-regeneratingsystems that produced the observed effects.

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Fig. 3. Reversal of effects of ATP-regenerating system by ADP. ATP-regenerating system was: creatine phosphate (3 mM), creatine kinase (5 U ml¹), and Mg²⁺ (10 mM). Binding after addition of 30 µM ATP under control conditions was 48 ± 3 fmol mg protein¹ and 120 ± 15 fmol mg protein¹ at 2.5 and 1.5 nM [³H]P1075 for SUR2A (solid bars) and SUR2B (crosshatched bars), respectively.

Because ADP was recognized as a modulator of [³H]P1075 binding, it was of interest to determine its concentration at the endof the incubation period. HPLC analysis (Table 1) showed thatstock solutions of ATP (3000, 1000, 30, and 3 µM), adjusted topH 7.4 in the absence of membranes and incubated at 37°C for 13or 30 min (i.e., the incubation times of SUR2A and 2B), contained<1% ADP. In the presence of membranes (SUR2A, 150 µg protein ml¹; SUR2B, 60 µg protein ml¹) and at 1000 and 3000 µM ATP, ADP at the end of incubation wasincreased by 5 to 15 times ranging from 58 to 92 µM. From thesedata the ATPase rate of the two membrane preparations was calculatedto approximately 40 µM min¹ (mg protein ml¹)¹; a similar ATPase rate was obtained with membranes from nontransfectedHEK cells. In the presence of 1000 µM ATP, coupling of the ATP-regeneratingsystem reduced ADP by 20 (SUR2A) and 4 times (SUR2B); additionof 1 mM ADP approximately restored the original ADP levels (Table1).

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TABLE 1
Determination of adenine nucleotides in incubation samples
Samples were incubated for 13 min (SUR2A) or 30 min (SUR2B) min at 37°C in absence or presence of SUR2A (150 µg membrane protein ml¹) or SUR2B (60 µg membrane protein ml¹), the ATP-regenerating (reg.) system (creatine phosphate, 3 mM; creatine kinase, 5 U ml¹; Mg²⁺, 10 mM; HEPES, 10 mM) and ADP (1 mM). Each sample was prepared at least three times and analyzed three to five times.

Figure 4 shows the effect of ADP on [³H]P1075 binding to SUR2A and 2B in the presence of 1 mM ATP and high [Mg²⁺]_free ( $approx$ 1 mM). Binding to SUR2B decreased strongly with increasingADP from 200% at the lowest ADP concentration attainable (13 µM;coupling of the ATP-regenerating system, Table 1) to 40% in thepresence of mM ADP (data normalized with respect to binding withoutexogenous ADP). Due to the ATPase activity of the membrane preparationlow ADP concentrations are difficult to control and this partof the concentration curve could not be completed. However, applyingthe Law of Mass Action to the data, one estimates a midpoint of13 µM (95% confidence intervals: 7,24) and a maximum binding inthe absence of MgADP of 340 ± 35% (not shown). In case of SUR2A,MgADP increased binding by 40 ± 3% with an EC₅₀ value of 340 µM(95% confidence intervals: 257,446).

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Fig. 4. Dependence of [³H]P1075 binding to SUR2A ( $black-square$ ) and 2B (

) on [ADP] in presence of 1 mM ATP and [Mg²⁺]_free $approx$ 1 mM (n = 3-5). Data are normalized to 100% at standard conditions (1 mM ATP, 1 mM [Mg²⁺]_free, no ADP added). First two ADP concentrations are from Table 1, other concentrations represent sum of endogenously formed + added ADP. Fits were performed according to eq. 3 with Hill coefficient = 1, giving for SUR2A/2B pK values of 3.47 ± 0.12/4.89 ± 0.10; starting levels (b) were 95 ± 2/340 ± 35%, and amplitudes (b-a) 41 ± 3/299 ± 34%, respectively (see text for details).

The nucleotide composition after addition of 30 µM ATP was analyzed to complement the binding data shown in Fig. 3. In thepresence of SUR2A and 2B, respectively, ATP was converted by 50and 30% into ADP (13 and 10 µM) and AMP (7 and 6 µM). Couplingof the ATP-regenerating system reduced ADP by more than 10 timesbelow 1 µM and addition of ADP (1 mM) restored the ADP concentrationagain approximately to the levels present in the absence of theATP-regenerating system (Table 1). The nucleotide compositionafter addition of 3 µM ATP was also of interest, because thisATP concentration is close to the EC₅₀ values of MgATP for activationof [³H]P1075 binding (Fig. 2). Table 1 shows that at the end of equilibrationtime, little ATP ( $<=$ 0.2 µM) and ADP (0.3 and 0.5 µM) were presentand AMP wasdominant.

Mg²⁺ Dependence. The dependence of [³H]P1075 binding to SUR2A and 2B on [Mg²⁺]_free at saturating [ATP] (3 mM) is illustrated in Fig. 5. Both curveswere biphasic. In either case, the first component of the curveswas activatory with EC₅₀ values of 0.8 µM (SUR2A) and 0.6 µM (SUR2B)and Hill coefficients (n_H) of 1. With SUR2A, the second componentshowed a further activation leading to more than a doubling ofbinding with EC₅₀ $approx$ 70 µM and n_H = 1. For SUR2B, the second componentwas inhibitory and binding decreased by about one-half with IC₅₀ $approx$ 170 µM and n_H = 1. Basal binding in the absence of Mg²⁺ was $approx$ 10%, caused by contaminations of Na₂ATP with Mg²⁺ (Hambrock et al., 1998). In the case of SUR2B, the creatine-basedATP-regenerating system was coupled at saturating [Mg²⁺]_free (>3 mM). Under these conditions binding increased from 100to 165 ± 2% (n = 4, data not illustrated). This showed that atsaturating Mg²⁺ ADP is important and it suggested that the second component ofthe [Mg²⁺]_free dependence reflects changes in MgADP similar to those seenin Fig. 2. Similarly, one may speculate that the first componentreflects changes in MgATP. Indeed, a replot of these data as functionof [MgATP] gave a regular concentration dependence for the firstcomponent with EC₅₀ values of 42 ± 6 and 20 ± 3 µM for SUR2A andSUR2B, respectively; however, the second component of this plotwas extremely steep and compressed into less than 1 order of magnitude(replot not shown).

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Fig. 5. Dependence of [³H]P1075 binding to SUR2A ( $black-square$ ) and 2B (

) on [Mg²⁺]_free, in presence of 3 mM ATP and 1 mM EDTA (n = 4). Data are normalized to 100% at standard conditions (1 mM ATP, 1 mM [Mg²⁺]_free) with absolute values given in Fig. 2. Logistic form of Hill equation with two components was fitted to data, giving for first component pEC₅₀ values for SUR2A/2B of 6.08 ± 0.10/6.21 ± 0.06 and amplitudes (%) of 39 ± 3/224 ± 8; for second component, pEC₅₀ values were 4.14 ± 0.06/3.77 ± 0.08 and amplitudes of 52 ± 3/-135 ± 7%.

The experiments described below were performed at 3 mM ATP and 3.8 mM Mg²⁺ ([Mg²⁺]_free $approx$ 1 mM). Inspection of Figs. 2 and 4 shows that under theseconditions the binding sites on SUR2A/2B for MgATP and MgADP arenearlysaturated.

Temperature Dependence. Initial experiments at 0°C showed very low binding of [³H]P1075 to SUR2A but good binding to SUR2B; at 37°C, however, bindingto SUR2A was increased $approx$ 10-fold and that to SUR2B was decreasedby 30%. These observations prompted us to investigate the temperaturedependence of binding in more detail. First, the association kineticswere measured at 24, 12, and 0°C to determine the appropriateincubation times (see legend to Fig. 6). Figure 5A shows thatbinding of [³H]P1075 to SUR2A at equilibrium decreased continuously in thetemperature range from 37 to 0°C to reach a level of 11 ± 2% at0°C. In contrast, [³H]P1075 binding to SUR2B exhibited a bell-shaped temperature dependenceincreasing by more than a factor of 2 at 24 and 12°C; at 0°C,binding was still 150% of that at 37°C.

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Fig. 6. Temperature dependence of [³H]P1075 binding to SUR2A (solid bars) and SUR2B (cross-hatched bars). Specific binding (B_s) measured in presence of 2.8 nM [³H]P1075 (SUR2A) or 4.5 nM [³H]P1075 (SUR2B). Measurement of association kinetics indicated that following incubation times (minutes) were sufficient to reach equilibrium (SUR2A/2B): 37°C: 13/30; 24°C: 45/90; 12°C: 60/180; 0°C: 240 min for SUR2B. At 0°C, binding to SUR2A was too small to perform kinetic and homologous competition experiments and samples were incubated for 300 min. B_S is normalized with respect to values at 37°C, which were 55/243 fmol mg protein¹ for SUR2A/2B, respectively. Data are from three to four experiments.

Pharmacological Properties. [³H]P1075 binding was inhibited by K_ATP channel openers and blockers with regular inhibition curves (Hill coefficient $approx$ 1) reaching100% with the exception of minoxidil sulfate where maximum inhibitionwas only 70%. Figure 7 illustrates the inhibition curves of theopeners pinacidil, minoxidil sulfate, and diazoxide and of theinhibitor, glibenclamide, in SUR2A-containing membranes; the pK_ivalues of all compounds tested are listed in Table 2. The resultsfor several channel modulators obtained in membranes with SUR2Bhave been published before (Hambrock et al., 1998); they are includedin Table 2 together with additional values for pinacidil andnicorandil determined in this study. Also listed are the pK_i valuesof these compounds obtained against [³H]P1075 in rat cardiac membranes (Löffler-Walz and Quast, 1998)and in rat aortic strips (Quast et al., 1993). The results ofthe correlation analysis are presented in Table 3. Excellentcorrelations were obtained comparing the potencies at SUR2A andSUR2B with those in heart membranes and rat aortic strips, respectively;in addition, slopes were near unity and the correlation lineswere close to the line of identity. The comparison of opener potenciestoward SUR2A with those toward SUR2B gave similar results concerningcorrelation coefficient and slope but showed that openers wereon average 3.5 times more potent at SUR2B.

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Fig. 7. Competition between [³H]P1075 and selected K_ATP channel modulators binding to SUR2A. $black-square$ , P1075, $black-triangle$ , minoxidil sulfate,

, glibenclamide, and $star$ , diazoxide. Data are means ± S.E.M. from four experiments. From fit of logistic equation to pooled data IC₅₀ values of 19 nM (P1075), 166 nM (minoxidil sulfate), 370 nM (glibenclamide), and 46 µM (nicorandil) were calculated; Hill coefficients were close to 1. Note that maximum inhibition by minoxidil sulfate was only 73 ± 2%. mean pK_i values determined from fits to individual inhibition curves and corrected for presence of radiolabel are listed in Table 2. Inhibition of [³H]P1075 binding was studied in presence of [³H]P1075 (3 nM) and inhibitor of interest at 3 mM ATP and a free Mg²⁺ concentration of 1 mM; 100% (specific) binding corresponds to 63 ± 3 fmol mg protein¹ and nonspecific binding amounted to 29 ± 2% of total binding.

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TABLE 2
Inhibition of [³H]P1075 binding by K_ATP channel modulators
Binding experiments with SUR2A were performed as shown in Fig. 7. Logistic equation (see Experimental Procedures) was fitted to individual competition curves (n = 4) yielding pIC₅₀, amplitudes ( $approx$ 100% with exception of minoxidil sulphate, see below) and Hill coefficients n_H ( $approx$ 1). pIC₅₀ values were corrected for presence of the radiolabel according to equation of Cheng-Prusoff which, on logarithmic scale, corresponded to addition of 0.07. Data for SUR2B are from Hambrock et al. (1998)

with exception of values for nicorandil and ( $-$ ) pinacidil, which were determined in this study. pK_i values in rat heart microsomes are from Löffler-Walz and Quast (1998)

with a Cheng-Prusoff correction of 0.06, and, those for rat aortic strips from Quast et al., 1993

. Temperature was 37°C in all cases. In all four preparations, minoxidil sulfate inhibited [³H]P1075 binding only by 68 to 75%.

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TABLE 3
Comparison of K_ATP channel modulators in different preparations
Linear correlation analysis of the pK_i values listed in Table 2 gave correlation coefficients (r), slopes (s), and mean distance (d) from line of identity as listed below. s = 1 means that K_i values on the two axes are proportional to one another and 10^d gives factor by which, in mean, K_i values on ordinate differ from those on abscissa.

	Discussion

Top Summary Introduction Experimental Procedures Results Discussion References

MgATP and [³H]P1075 Binding to SUR2A and SUR2B. This study showed that addition of ATP in the presence of mM Mg²⁺ enabled binding of the opener [³H]P1075 to SUR2A and SUR2B with EC₅₀ values of 5 and 3 µM, respectively(see also Hambrock et al., 1998; Schwanstecher et al., 1998).In addition, Schwanstecher et al. (1998) showed that nonhydrolyzableATP-analogs do not support opener binding to SUR2B. The HPLC measurementsperformed in this study showed, however, that at the end of theincubation period, >90% of the 3 µM ATP originally present hadbeen hydrolyzed and that this was due mostly to the ATPase activityof proteins other than SUR. Hence, the EC₅₀ values for ATP determinedhere and elsewhere cannot be taken at face value. On the otherhand, the ATPase rate of SUR is unknown and the nucleotides boundto SUR need not to be at equilibrium with the changing nucleotidecomposition of the incubation solution, in particular if the hydrolyticactivity of SUR islow.

Effect of MgADP. A major new result of this study is the observation that, in the obligatory presence of MgATP, MgADP is an important modulatorof [³H]P1075 binding. At SUR2A, MgADP (<100 µM) shifted the MgATP dependenceof binding toward the left by 20 times; higher concentrationsincreased binding. At SUR2B, MgADP inhibited opener binding bythree- fourths. Several points deserve comment: First, the oppositedirection of the MgADP effect at the two SUR2 isoforms (whichonly differ in their carboxyl terminus) suggests that the carboxylterminus affects the MgADP binding site. Second, the inhibitoryeffect of MgADP on opener binding to SUR2B is intriguing becauseMgADP opens the vascular K_ATP channel (=nucleoside diphosphate-dependentK⁺ channel, K_NDP; Beech et al., 1993) and the SUR2B/Kir6.1 construct(Satoh et al., 1998). Third, SUR2B, in the presence of 1 mM ATP,senses changes in the ADP concentration from 10 to 100 µM, suggestingthat the nucleotide binding site that mediates the MgADP effectshas a >10-fold selectivity for MgADP over MgATP. In this contextit is of interest that on the multidrug resistance-associatedprotein, another ABC protein, a binding site with high selectivityfor nucleoside diphosphates has been described that is distinctfrom the catalytic (nucleoside triphosphate) site (Chang et al.,1998). Occupation of this site stimulates the ATPase activityof the proteinseveralfold.

That Mg²⁺ is required for ADP to be effective is shown in Fig. 5, which illustrates the dependence of [³H]P1075 binding to SUR2 on [Mg²⁺]_free at saturating [ATP]. The curves were biphasic and the experimentalevidence suggests that the second component, starting at [Mg²⁺]_free $approx$ 10 µM, represents the effect of MgADP. Indeed, at [Mg²⁺]_free >10 µM, one calculates [MgATP] >350 µM, which is saturatingfor [³H]P1075 binding and sufficient to fuel the ATPase activity inthe preparation, leading to appreciable amounts of ADP. The stabilityof the MgADP complex is 5 to 10 times weaker than that of MgATP(Smith and Martell, 1989

), hence, it is essentially [Mg²⁺]_free, which is limiting for formation of MgADP under the experimentalconditions of Fig. 5. This gives rise to the second componentof these curves with an apparent EC₅₀ $approx$ 100 µM. In the cell, [Mg²⁺]_free has been determined to 0.5 to 1 mM; hence, Mg²⁺ is close to saturation under physiological conditions. As forthe ADP levels, these are estimated to $approx$ 100 µM in smooth muscleat rest (Butler and Davies, 1980

; Taggart and Wray, 1998

) andthe MgADP site of SUR2B is saturated under physiological conditions.The free ADP concentration in cardiocytes at rest is $approx$ 15 µM andreaches >100 µM in early hypoxia (Venkatesh et al., 1991

); thisis approximately the range over which MgADP exerts its effectonSUR2A.

Comparison of the binding data with the nucleotide measurements after addition of 30 µM ATP showed that at the end of theincubation period similar concentrations of MgADP and MgATP haddeveloped and that MgADP strongly affected opener binding. Reductionof [MgADP] to $approx$ 2% of [MgATP] by the ATP-regenerating system reversedthe effect, supporting the estimate of a >10-fold selectivityof the MgADP site over MgATP. When the experiments were performedin the additional presence of 1 mM ADP, i.e., ATP (30 µM) + ADP(1 mM) + ATP- regenerating system, the nucleotide compositionat the end of the incubation period was similar to that at 1 mMATP in the presence of the ATP- regenerating system (ADP $approx$ 10 µM,see Table 1). The binding result with SUR2B in Fig. 3 (last column)was, however, that of an MgADP-inhibited state which, at 1 mMATP, requires the presence of 60 to 90 µM ADP. This showed againthat the conformational state of the SUR lags behind the changein nucleotide composition of the solution (seeabove).

The effects of MgADP described here extend the earlier report of an inhibitory effect of [Mg²⁺]_free >10 µM on [³H]P1075 binding to murine SUR2B where, however, additional factorslike the ADP formed by the ATPase activity of SUR2B were not excluded(Hambrock et al., 1998

). They are not necessarily in contradictionwith the lack of effect of MgADP and MgGDP on P1075 binding toSUR2B reported by Schwanstecher et al. (1998)

. In their study,performed at room temperature and with human SUR2B, the MgADPsite on SUR2B may have been saturated before the addition of nucleosidediphosphates.

Temperature Dependence. A surprising result of this study is the opposite temperature dependence of [³H]P1075 binding to SUR2A and 2B; falling temperatures decreasedbinding to SUR2A monotonously but induced a bell-shaped increasein binding to SUR2B. Necessarily, these changes reflect the thermodynamicsof the interaction of the opener and of the nucleotides with SURand the temperature dependence of ADP formation. Lowering temperaturewill lead to a decrease in the amount of ADP formed and this maycontribute to the observed decrease in binding to SUR2A and tothe increase with SUR2B. A detailed interpretation of the datarequires the direct measurement of nucleotide binding to SUR which,in turn, requires very high expression of theproteins.

Pharmacological Properties. Openers representative of the different chemical families of this class of drugs as well as glibenclamide inhibited [³H]P1075 binding to murine SUR2A with Hill coefficient of 1 andto completion; the exception was minoxidil sulfate with only 73%inhibition. Similar observations had been made for minoxidil sulfatein membranes from HEK cells transfected with murine SUR2B (Hambrocket al., 1998), in cardiac membranes (Löffler-Walz and Quast,1998), in A10 cells (a cell line derived from embryonic rat aorta;Russ et al., 1997), and in calf coronary myocytes (Lemoine etal., 1996). For human SUR2B expressed in COS cells, Schwanstecheret al. (1998) reported a biphasic inhibition curve with aboutequal amplitudes for the low- and the high-affinity component.These results have mostly been interpreted as reflecting heterogeneityof the otherwise homogeneous opener sites, although allostericmechanisms were not ruled out (Hambrock et al., 1998; Löffler-Walzand Quast, 1998; Schwanstecher et al., 1998). Alternatively, minoxidilsulfate could transfer its sulfate group to a neighboring aminoacid, thereby inhibiting further binding of the drug to the receptorsite (W. P. Manley, personal communication); protein sulfationby minoxidil sulfate has been reported to occur easily (Meisheriet al., 1993).

The potencies (pK_i values) of the K_ATP channel modulators for binding to SUR2A are similar to those obtained in membranesfrom rat heart (Table 3). This suggests that SUR2A is the functionallyrelevant receptor for the openers in heart; however, the correlationof the binding data with electrophysiological studies in cardiocytesis not so clear (see also Löffler-Walz and Quast, 1998

). Diazoxidehas been accepted as the diagnostic compound to differentiatebetween vascular and cardiac K_ATP channels because it activatesthe native channel in the vasculature (Quast and Cook, 1989

) andthe recombinant channel SUR2B/Kir6.2 (Isomoto et al., 1996

), butnot the channel in the heart nor the recombinant channel SUR2A/Kir6.2(Inagaki et al., 1996

; Okuyama et al., 1998

). In the binding experiments,however, diazoxide exhibits a regular competition pattern at SUR2Band 2A being only four times weaker at SUR2A (Table 1, see alsoSchwanstecher et al., 1998

). Similarly, nicorandil is a ratherselective opener of the vascular channel, with a 100-fold higherpotency at the recombinant vascular channel, SUR2B/Kir6.2 thanat SUR2A/Kir6.2 (Shindo et al., 1998

) but only a 2-fold differencein binding. Taken together, these results raise questions concerningthe relationship between binding of openers and activation ofthe cardiacchannel.

In case of SUR2B, there is little doubt that this SUR is indeed the drug receptor for the openers in vascular smooth muscle.First, the pK_i values for binding to SUR2B are very similar tothose obtained in rat aortic strips (Tables 2 and 3). Second,opener binding in rat aorta correlates very well with opener-inducedvasorelaxation and channel opening (measured by ⁸⁶Rb⁺ efflux; Quast et al., 1993

). Third, mutations in SUR2B affectedopener binding and activation of mutant SUR2B/wild-type Kir6.2channels in a similar way (Schwanstecher et al., 1998

When opener binding to murine SUR2A is compared with that to murine SUR2B, an excellent correlation is obtained again (Table3). In the mean, the openers bind 3.5 times weaker to SUR2A;glibenclamide, however, is about 7.6 times more potent than atSUR2B. Hence, it appears that the pharmacological profile of SUR2Ais slightly shifted in the direction of SUR1, where the openersare very weak and glibenclamide is very potent (see e.g., Schwanstecheret al., 1998

). This is paradoxical because the carboxyl terminusof SUR2B shows much higher homology to SUR1 than that of SUR2A(Isomoto et al., 1996

; Inagaki et al., 1996

; review: Aguilar-Bryanet al., 1998

). These observations suggest that the carboxyl terminusis important for ligand binding to SUR, but that the remainderof the molecule plays a decisivepart.

Conclusion. This study has shown that MgADP stimulates opener binding to SUR2A but inhibits binding to SUR2B. One may speculate that thecarboxyl termini of these SURs fold back to affect the interactionof MgADP with its binding site. Finally, the results suggest thatthe carboxyl terminus may form part of the binding pockets foropeners and glibenclamide; alternatively, it may affect thesebinding pockets allosterically. Further work, including mutationalanalyses of the SURs is required to decide between thesepossibilities.

	Acknowledgments

We thank Dr. U. Russ (Tübingen) for the computer program used to calculate the Mg²⁺ and MgATP concentrations and for helpful discussion, and Dr.W. P. Manley (Novartis, Basel) for a stimulating discussion concerningminoxidil sulfate and synthesis of some K_ATP channelopeners.

	Footnotes

Received December 15, 1998; Accepted February 23, 1999

This study was supported by the Deutsche Forschungsgemeinschaft, Grant Qu 100/2-2.

Send reprint requests to: Dr. Ulrich Quast, Department of Pharmacology, University of Tübingen, Wilhelmstrasse 56, D-72074 Tübingen, Germany. E-mail: ulrich.quast{at}uni-tuebingen.de

	Abbreviations

ABC proteins, ATP binding cassette proteins; HEK cells, human embryonic kidney cells; K_ATP channel, ATP-sensitive K⁺ channel; P1075, [³H]-N-cyano-N'-(1,1-dimethylpropyl)-N"-3-pyridylguanidine); SUR, sulfonylurea receptor.

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Y. Kang, Y.-M. Leung, J. E. Manning-Fox, F. Xia, H. Xie, L. Sheu, R. G. Tsushima, P. E. Light, and H. Y. Gaisano
Syntaxin-1A Inhibits Cardiac KATP Channels by Its Actions on Nucleotide Binding Folds 1 and 2 of Sulfonylurea Receptor 2A
J. Biol. Chem., November 5, 2004; 279(45): 47125 - 47131.
[Abstract] [Full Text] [PDF]

M. Yamada and Y. Kurachi
The Nucleotide-Binding Domains of Sulfonylurea Receptor 2A and 2B Play Different Functional Roles in Nicorandil-Induced Activation of ATP-Sensitive K+ Channels
Mol. Pharmacol., May 1, 2004; 65(5): 1198 - 1207.
[Abstract] [Full Text]

R. Davis-Taber, E. J. Molinari, R. J. Altenbach, K. L. Whiteaker, C.-C. Shieh, G. Rotert, S. A. Buckner, J. Malysz, I. Milicic, J. S. McDermott, et al.
[125I]A-312110, a Novel High-Affinity 1,4-Dihydropyridine ATP-sensitive K+ Channel Opener: Characterization and Pharmacology of Binding
Mol. Pharmacol., July 1, 2003; 64(1): 143 - 153.
[Abstract] [Full Text] [PDF]

E. A. Cartier, S. Shen, and S.-L. Shyng
Modulation of the Trafficking Efficiency and Functional Properties of ATP-sensitive Potassium Channels through a Single Amino Acid in the Sulfonylurea Receptor
J. Biol. Chem., February 21, 2003; 278(9): 7081 - 7090.
[Abstract] [Full Text] [PDF]

C. Loffler-Walz, A. Hambrock, and U. Quast
Interaction of KATP Channel Modulators with Sulfonylurea Receptor SUR2B: Implication for Tetramer Formation and Allosteric Coupling of Subunits
Mol. Pharmacol., February 1, 2002; 61(2): 407 - 414.
[Abstract] [Full Text] [PDF]

U. Russ, U. Lange, C. Loffler-Walz, A. Hambrock, and U. Quast
Interaction of the Sulfonylthiourea HMR 1833 with Sulfonylurea Receptors and Recombinant ATP-Sensitive K+ Channels: Comparison with Glibenclamide
J. Pharmacol. Exp. Ther., December 1, 2001; 299(3): 1049 - 1055.
[Abstract] [Full Text] [PDF]

F. Reimann, F. M. Ashcroft, and F. M. Gribble
Structural Basis for the Interference Between Nicorandil and Sulfonylurea Action
Diabetes, October 1, 2001; 50(10): 2253 - 2259.
[Abstract] [Full Text]

A. Hambrock, C. Loffler-Walz, U. Russ, U. Lange, and U. Quast
Characterization of a Mutant Sulfonylurea Receptor SUR2B with High Affinity for Sulfonylureas and Openers: Differences in the Coupling to Kir6.x Subtypes
Mol. Pharmacol., July 1, 2001; 60(1): 190 - 199.
[Abstract] [Full Text]

F. Reimann, F. M. Gribble, and F. M. Ashcroft
Differential Response of KATP Channels Containing SUR2A or SUR2B Subunits to Nucleotides and Pinacidil
Mol. Pharmacol., April 13, 2001; 58(6): 1318 - 1325.
[Abstract] [Full Text]

M. Okamura, M. Kakei, K. Ichinari, A. Miyamura, N. Oketani, N. Koriyama, and C. Tei
State-dependent modification of ATP-sensitive K+ channels by phosphatidylinositol 4,5-bisphosphate
Am J Physiol Cell Physiol, February 1, 2001; 280(2): C303 - C308.
[Abstract] [Full Text] [PDF]

M. BIENENGRAEBER, A. E. ALEKSEEV, M. R. ABRAHAM, A. J. CARRASCO, C. MOREAU, M. VIVAUDOU, P. P. DZEJA, and A. TERZIC
ATPase activity of the sulfonylurea receptor: a catalytic function for the KATP channel complex
FASEB J, October 1, 2000; 14(13): 1943 - 1952.
[Abstract] [Full Text]

F. M. Gribble, F. Reimann, R. Ashfield, and F. M. Ashcroft
Nucleotide Modulation of Pinacidil Stimulation of the Cloned KATP Channel Kir6.2/SUR2A
Mol. Pharmacol., June 1, 2000; 57(6): 1256 - 1261.
[Abstract] [Full Text]

A. P. Babenko, G. Gonzalez, and J. Bryan
Pharmaco-topology of Sulfonylurea Receptors. SEPARATE DOMAINS OF THE REGULATORY SUBUNITS OF KATP CHANNEL ISOFORMS ARE REQUIRED FOR SELECTIVE INTERACTION WITH K+ CHANNEL OPENERS
J. Biol. Chem., January 14, 2000; 275(2): 717 - 720.
[Abstract] [Full Text] [PDF]

U. Russ, A. Hambrock, F. Artunc, C. Löffler-Walz, Y. Horio, Y. Kurachi, and U. Quast
Coexpression with the Inward Rectifier K+ Channel Kir6.1 Increases the Affinity of the Vascular Sulfonylurea Receptor SUR2B for Glibenclamide
Mol. Pharmacol., November 1, 1999; 56(5): 955 - 961.
[Abstract] [Full Text]

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				Y. Kang, Y.-M. Leung, J. E. Manning-Fox, F. Xia, H. Xie, L. Sheu, R. G. Tsushima, P. E. Light, and H. Y. Gaisano Syntaxin-1A Inhibits Cardiac KATP Channels by Its Actions on Nucleotide Binding Folds 1 and 2 of Sulfonylurea Receptor 2A J. Biol. Chem., November 5, 2004; 279(45): 47125 - 47131. [Abstract] [Full Text] [PDF]

				M. Yamada and Y. Kurachi The Nucleotide-Binding Domains of Sulfonylurea Receptor 2A and 2B Play Different Functional Roles in Nicorandil-Induced Activation of ATP-Sensitive K+ Channels Mol. Pharmacol., May 1, 2004; 65(5): 1198 - 1207. [Abstract] [Full Text]

				R. Davis-Taber, E. J. Molinari, R. J. Altenbach, K. L. Whiteaker, C.-C. Shieh, G. Rotert, S. A. Buckner, J. Malysz, I. Milicic, J. S. McDermott, et al. [125I]A-312110, a Novel High-Affinity 1,4-Dihydropyridine ATP-sensitive K+ Channel Opener: Characterization and Pharmacology of Binding Mol. Pharmacol., July 1, 2003; 64(1): 143 - 153. [Abstract] [Full Text] [PDF]

				E. A. Cartier, S. Shen, and S.-L. Shyng Modulation of the Trafficking Efficiency and Functional Properties of ATP-sensitive Potassium Channels through a Single Amino Acid in the Sulfonylurea Receptor J. Biol. Chem., February 21, 2003; 278(9): 7081 - 7090. [Abstract] [Full Text] [PDF]

				C. Loffler-Walz, A. Hambrock, and U. Quast Interaction of KATP Channel Modulators with Sulfonylurea Receptor SUR2B: Implication for Tetramer Formation and Allosteric Coupling of Subunits Mol. Pharmacol., February 1, 2002; 61(2): 407 - 414. [Abstract] [Full Text] [PDF]

				U. Russ, U. Lange, C. Loffler-Walz, A. Hambrock, and U. Quast Interaction of the Sulfonylthiourea HMR 1833 with Sulfonylurea Receptors and Recombinant ATP-Sensitive K+ Channels: Comparison with Glibenclamide J. Pharmacol. Exp. Ther., December 1, 2001; 299(3): 1049 - 1055. [Abstract] [Full Text] [PDF]

				F. Reimann, F. M. Ashcroft, and F. M. Gribble Structural Basis for the Interference Between Nicorandil and Sulfonylurea Action Diabetes, October 1, 2001; 50(10): 2253 - 2259. [Abstract] [Full Text]

				A. Hambrock, C. Loffler-Walz, U. Russ, U. Lange, and U. Quast Characterization of a Mutant Sulfonylurea Receptor SUR2B with High Affinity for Sulfonylureas and Openers: Differences in the Coupling to Kir6.x Subtypes Mol. Pharmacol., July 1, 2001; 60(1): 190 - 199. [Abstract] [Full Text]

				F. Reimann, F. M. Gribble, and F. M. Ashcroft Differential Response of KATP Channels Containing SUR2A or SUR2B Subunits to Nucleotides and Pinacidil Mol. Pharmacol., April 13, 2001; 58(6): 1318 - 1325. [Abstract] [Full Text]

				M. Okamura, M. Kakei, K. Ichinari, A. Miyamura, N. Oketani, N. Koriyama, and C. Tei State-dependent modification of ATP-sensitive K+ channels by phosphatidylinositol 4,5-bisphosphate Am J Physiol Cell Physiol, February 1, 2001; 280(2): C303 - C308. [Abstract] [Full Text] [PDF]

				M. BIENENGRAEBER, A. E. ALEKSEEV, M. R. ABRAHAM, A. J. CARRASCO, C. MOREAU, M. VIVAUDOU, P. P. DZEJA, and A. TERZIC ATPase activity of the sulfonylurea receptor: a catalytic function for the KATP channel complex FASEB J, October 1, 2000; 14(13): 1943 - 1952. [Abstract] [Full Text]

				F. M. Gribble, F. Reimann, R. Ashfield, and F. M. Ashcroft Nucleotide Modulation of Pinacidil Stimulation of the Cloned KATP Channel Kir6.2/SUR2A Mol. Pharmacol., June 1, 2000; 57(6): 1256 - 1261. [Abstract] [Full Text]

				A. P. Babenko, G. Gonzalez, and J. Bryan Pharmaco-topology of Sulfonylurea Receptors. SEPARATE DOMAINS OF THE REGULATORY SUBUNITS OF KATP CHANNEL ISOFORMS ARE REQUIRED FOR SELECTIVE INTERACTION WITH K+ CHANNEL OPENERS J. Biol. Chem., January 14, 2000; 275(2): 717 - 720. [Abstract] [Full Text] [PDF]

				U. Russ, A. Hambrock, F. Artunc, C. Löffler-Walz, Y. Horio, Y. Kurachi, and U. Quast Coexpression with the Inward Rectifier K+ Channel Kir6.1 Increases the Affinity of the Vascular Sulfonylurea Receptor SUR2B for Glibenclamide Mol. Pharmacol., November 1, 1999; 56(5): 955 - 961. [Abstract] [Full Text]