Purine and Pyrimidine Nucleotides Inhibit a Noninactivating K+ Current and Depolarize Adrenal Cortical Cells through a G Protein-Coupled Receptor

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Vol. 55, Issue 2, 364-376, February 1999

Purine and Pyrimidine Nucleotides Inhibit a Noninactivating K+ Current and Depolarize Adrenal Cortical Cells through a G Protein-Coupled Receptor

Lin Xu and John J. Enyeart

Department of Pharmacology (L.X., J.J.E.) and Neuroscience Program (J.J.E.), The Ohio State University College of Medicine, Columbus, Ohio

	Summary

Top Summary Introduction Materials and methods Results Discussion References

Bovine adrenal zona fasciculata (AZF) cells express a noninactivating K⁺ current (I_AC) that sets the resting membrane potential and maymediate depolarization-dependent cortisol secretion. ExternalATP stimulates cortisol secretion through activation of a nucleotidereceptor. In whole-cell patch clamp recordings from bovine AZFcells, we found that ATP selectively inhibited I_AC K⁺ current by a maximum of 75.7 ± 3% (n = 13) with a 50% inhibitoryconcentration of 1.3 µM. A rapidly inactivating A-type K⁺ current was not inhibited by ATP. Other nucleotides, includingADP and the pyrimidines UTP and UDP, also inhibited I_AC, whereas2-methylthio-ATP (2-MeSATP) and CTP were completely ineffective.The rank order of potency for six nucleotides was UTP = ADP >ATP > UDP $>>$ 2-MeSATP = CTP. At maximally effective concentrations,UTP, ADP, and UDP inhibited I_AC current by 81.4 ± 5.2% (n = 7),70.7 ± 7.2% (n = 4), and 65.2 ± 7.9% (n = 5), respectively. Inhibitionof I_AC by external ATP was reduced from 71.3 ± 3.2% to 22.8 ±4.5% (n = 18) by substituting guanosine 5'-O-2-(thio) diphosphatefor GTP in the patch pipette. Inhibition of I_AC by external ATP(10 µM) was markedly suppressed (to 17.3 ± 5.5%, n = 9) by thenonspecific protein kinase antagonist staurosporine (1 µM) andeliminated by substituting the nonhydrolyzable ATP analog 5-adenylyl-imidodiphosphateor UTP for ATP in the pipette. ATP-mediated inhibition of I_ACwas not altered by the kinase C antagonist calphostin C, the calmodulininhibitory peptide, or by buffering the intracellular (pipette)Ca⁺⁺ with 20 mM 1,2-bis-(2-aminophenoxy)ethane-N, N,N',N'-tetraaceticacid. In current clamp recordings, ATP and UTP (but not CTP) depolarizedAZF cells at concentrations that inhibited I_AC K⁺ current. These results demonstrate that bovine AZF cells expressa nucleotide receptor with a P2Y₃ agonist profile that is coupledto the inhibition of I_AC K⁺ channels through a GTP-binding protein. The inhibition of I_ACK⁺ current and associated membrane depolarization are the firstcellular responses demonstrated to be mediated through this receptor.Nucleotide inhibition of I_AC proceeds through a pathway that isindependent of phospholipase C, but that requires ATP hydrolysis.The identification of a new signaling pathway in AZF cells, wherebyactivation of a nucleotide receptor is coupled to membrane depolarizationthrough inhibition of a specific K⁺ channel, suggests a mechanism for ATP-stimulated corticosteroidsecretion that depends on depolarization-dependent Ca⁺⁺ entry. This may be a means of synchronizing the stress-inducedsecretion of corticosteroids and catecholamines from the adrenalgland.

	Introduction

Top Summary Introduction Materials and methods Results Discussion References

Extracellular ATP acts as a neurotransmitter or local hormone to elicit responses in a variety of cells. By activation ofspecific receptors, ATP mediates or modulates a range of physiologicalprocesses that include neurotransmission, contraction of smoothand cardiac muscle cells, inflammatory and immune responses, andsecretion of hormones including insulin, glucagon, catecholamines,and corticosteroid hormones (Dalziel and Westfall, 1994; Fredholmet al., 1994; Hoey et al., 1994; Williams and Burnstock, 1997).

Membrane receptors for ATP and other nucleotides can be grouped into two major classes. The P2X receptors form ligand-gated,nonselective cation channels, whereas P2Y receptors are G protein-coupled,membrane proteins (Dubyak and El-Moatassim, 1993; Dalziel andWestfall, 1994; Williams and Burnstock, 1997). Within each ofthese two major groups, multiple subtypes exist that can be distinguishedbased on their sensitivity to ATP and other nucleotides. In particular,G protein-coupled P2Y₁ receptors include those that are preferentiallyactivated by purines such as ATP and ADP, and the pyrimidinesUTP and UDP (Dubyak and El-Moatassim, 1993; Dalziel and Westfall,1994; Williams and Burnstock, 1997). The discovery that P2Y receptorsincluded a subtype that was preferentially activated by both purinesand pyrimidines led to the subclassification of this family intoP2Y₁ and P2Y₂ receptors (Lustig et al., 1993; Parr et al., 1994;Williams and Burnstock, 1997). The cloning of additional P2Y receptorswith distinct structures and pharmacological profiles has resultedin the addition of at least six new subtypes to this family (P2Y₃-P2Y₈)(reviewed in Filtz et al., 1997 and Williams and Burnstock, 1997).

In bovine adrenal zona fasciculata (AZF) cells, ATP, UTP, and ADP stimulate cortisol secretion at concentrations between 10⁶ and 10⁴ M through a Ca⁺⁺-dependent process (Niitsu, 1992; Hoey et al., 1994). The cellularmechanisms by which ATP and other nucleotides stimulate cortisolsecretion are unknown. AZF cells express a novel K⁺ channel (I_AC) that appears to set the resting membrane potential(Mlinar et al., 1993a; Enyeart et al., 1996). Corticotropin [adrencorticotropichormone (ACTH)] and AII, two peptide hormones that physiologicallyregulate cortisol secretion, inhibit I_AC and depolarize AZF cellsat concentrations identical with those that stimulate steroidogenesis(Mlinar et al., 1993a). I_AC channels couple peptide receptor activationto membrane depolarization, Ca⁺⁺ entry, and cortisol secretion (Enyeart et al., 1993; Mlinar etal., 1993a). To determine whether nucleotide receptors on AZFcells might also be linked to I_AC inhibition, we have studiedthe effect of ATP and other nucleotides on I_AC current in whole-cellpatch clamp recordings from bovine AZFcells.

	Materials and Methods

Top Summary Introduction Materials and methods Results Discussion References

Tissue culture media, antibiotics, fibronectin, and fetal bovine sera were obtained from Gibco (Grand Island, NY). Coverslipswere purchased from Bellco Glass, Inc. (Vineland, NJ). Enzymes,ACTH(1-24), MgATP, NaATP, NaUTP, NaUDP, KADP, 5-adenylyl-imidodiphosphate(AMP-PNP, lithium salt), NaCTP, NaGTP, guanosine 5'-O-2-(thio)-diphosphate(GDP- $beta$ -S), 2-MeSATP, 1,2-bis-(2-aminophenoxy)ethane-N, N,N',N'-tetraaceticacid (BAPTA), and staurosporine were obtained from Sigma ChemicalCompany (St. Louis, MO). Calmodulin inhibitory peptide (residues290-309 of CaM kinase II) was obtained from Biomol (Plymouth Meeting,PA).

Isolation and Culture of Adrenocortical Cells. Bovine adrenal glands were obtained from steers (age range, 1-3 years) within 60 min of slaughter at a local slaughterhouse.Fatty tissue was removed immediately and the glands were transportedto the laboratory in ice-cold phosphate-buffered saline (PBS)containing 0.2% dextrose. Isolated AZF cells were prepared asdescribed previously (Gospodarowicz et al., 1977) with some modifications.In a sterile tissue culture hood, the adrenals were cut in halflengthwise and the lighter medulla tissue was trimmed away fromthe cortex and discarded. The capsule with attached glomerulosa,and thicker fasciculata layer were then dissected into piecesapproximately 1.0 × 1.0 × 0.5 cm. A Stadie-Riggs tissue slicer(Thomas Scientific) was used to separate fasciculata tissue fromthe glomerulosa layers by slicing 0.3- to 0.5-mm slices from thelarger pieces. The first medulla/fasciculata slices were discarded.One to two subsequent fasciculata slices were saved in cold, sterilePBS/0.2% dextrose. The fasciculata/glomerulosa margin (about 0.5mm) and capsule with attached glomerulosa were discarded. Fasciculatatissue slices were then diced into 0.5-mm³ pieces and dissociated with 2 mg/ml (about 200-300 U/ml) of TypeI collagenase (neutral protease activity not exceeding 100 units/mgof solid), 0.2 mg/ml deoxyribonuclease in Dulbecco's modifiedEagle's medium (DMEM)/F12 for approximately 1 h at 37°C, trituratingafter 30 and 45 min with a sterile, plastic transfer pipette.The tissue/cell suspension was filtered through two layers ofsterile cheesecloth and then centrifuged to pellet cells at 100gfor 5 min. Undigested tissue remaining in the cheesecloth wascollagenase-treated for an additional hour. Pelleted cells werewashed with DMEM/0.2% BSA, centrifuging as before. After resuspensionin DMEM, cells were filtered through 200-µm stainless steel meshto remove clumps. Dispersed cells were again centrifuged and eitherresuspended in DMEM/F12 (1:1) with 10% fetal bovine serum (FBS),100 U/ml penicillin, and 0.1 mg/ml streptomycin and plated forimmediate use, or resuspended in FBS/5% DMSO, divided into 1-mlaliquots, each containing about 4 × 10⁶ cells, and stored in liquid nitrogen for future use. Cells wereplated in 35-mm dishes containing 9-mm² glass coverslips that had been treated with fibronectin (10 µg/ml)at 37°C for 30 min and then rinsed with warm, sterile PBS immediatelybefore adding cells. Dishes were maintained at 37°C in a humidifiedatmosphere of 95% air and 5% CO₂.

Patch Clamp Experiments. Patch clamp recordings of K⁺ channel currents were made in the whole-cell configuration. The standard pipette solution was120 mM KCl, 2 mM MgCl₂, 1 mM CaCl₂, 10 mM HEPES, 11 mM BAPTA,and 200 µM GTP, and 5 mM MgATP with pH buffered to 7.2 using KOH.Deviations from the standard solution are described in the text.Pipette [Ca⁺⁺] was determined using the "Bound and Determined" program (Brooksand Storey, 1992). The external solution consisted of 140 mM NaCl,5 mM KCl, 2 mM CaCl, 2 mM MgCl₂, 10 mM HEPES, and 5 mM glucose,pH 7.4, using NaOH. All solutions were filtered through 0.22-µmcellulose acetate filters. The Na⁺ salts of ATP, UTP, and CTP were applied externally by bath perfusioncontrolled manually by a six-way rotaryvalve.

AZF cells were used for patch clamp experiments 2 to 12 h after plating. Typically, cells with diameters of <15 µm and capacitancesof 8 to 15 pF were selected. Coverslips were transferred from35-mm culture dishes to the recording chamber (volume, 1.5 ml),which was perfused continuously by gravity at a rate of 3 to 5ml/min. Patch electrodes with resistances of 1.0 to 2.0 M $Omega$ werefabricated from Corning 0010 glass (Garner Glass Co., Claremont,CA). These routinely yielded access resistances of 1.5 to 2 M $Omega$ and voltage clamp time constants of less than 100 µs. K⁺ currents were recorded at room temperature (22-25°C) followingthe procedure of Hamill et al. (1981)

using an Axopatch 1D patchclamp amplifier (Axon Instruments, Burlingame,CA).

Pulse generation and data acquisition were done using a personal computer and PCLAMP software with a TL-1 interface (AxonInstruments). Currents were digitized at 1 to 20 kHz after filteringwith an eight-pole Bessel filter (Frequency Devices, Haverhill,MA). Linear leak and capacity currents were subtracted from currentrecords using scaled hyperpolarizing steps of one-third to one-fourthamplitude. Data were analyzed and plotted using PCLAMP 5.5 and6.02 (CLAMPAN and CLAMPFIT) and SigmaPlot (version 4.0). Series-resistancecompensation was not used in most experiments. The mean amplitudeof I_AC current in AZF cells was less than 750 pA. A current ofthis size in combination with a 4 M $Omega$ access resistance producesa voltage error of only 3 mV, which was notcorrected.

	Results

Top Summary Introduction Materials and methods Results Discussion References

Bovine AZF cells express two types of K⁺ current, a rapidly inactivating, voltage-gated A-type K⁺ current, and a noninactivating weakly voltage-dependent current(I_AC). I_AC is present initially, but grows dramatically over aperiod of minutes in whole-cell recordings, provided that ATPor other nucleotides are present at millimolar concentrationsin the recording pipette (Mlinar and Enyeart, 1993; Mlinar etal., 1993a; Enyeart et al., 1996; Enyeart et al., 1997). The absenceof time and voltage-dependent inactivation of the I_AC K⁺ current allowed it to be easily isolated for measurement in whole-cellrecordings using either of two voltage clamp protocols. When voltagesteps of 300-ms duration are applied from a holding potentialof $-$ 80 mV to a test potential of +20 mV, I_AC could be measuredselectively near the end of a voltage step where the rapidly inactivatingA-type current had completely inactivated (Fig. 1A, left traces).Alternatively, I_AC was selectively activated with an identicalvoltage step, after a 10-s prepulse to $-$ 20 mV had fully inactivatedthe A-type K⁺ current (Fig. 1A, right traces). Results reported in this studywere obtained in recordings from more than 200 AZF cells.

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Fig. 1. Time- and concentration-dependent inhibition of I_AC by external ATP. Whole-cell K⁺ currents were recorded from bovine AZF cells at 30-s intervals in response to voltage steps to +20 mV applied from a holding potential of $-$ 80 mV with or without 10-s prepulses to $-$ 20 mV, which inactivated A-type K⁺ current. After I_AC reached a stable amplitude, cells were superfused with NaATP at various concentrations. A, K⁺ current records made with patch pipettes containing standard pipette solution containing 5 mM MgATP and 200 µM GTP, with (right) or without (left) 10-s prepulses to $-$ 20 mV. Numbers correspond to currents immediately after initiating whole-cell recording (1), after I_AC had reached a maximum amplitude (2), and after inhibition by ATP (10 µM) (3). B, I_AC amplitudes recorded with (open circles) or without (solid circles) depolarizing prepulses are plotted against time. NaATP (10 µM) was perfused as indicated. C, inhibition curve. Fraction of unblocked I_AC is plotted against ATP concentration. Data were fit with an equation of the form: I/I_max = 1/[1+(B/K_d)^x], where B is NaATP concentration, K_d is the equilibrium dissociation constant, and x is the Hill coefficient.

Selective Inhibition of I_AC by External Nucleotides. ATP applied to AZF cells externally by bath perfusionproduced a selective, concentration-dependent inhibition of I_AC (Fig.1). In these experiments, I_AC was recorded at 30-s intervals.When this current reached a stable maximum amplitude, ATP wassuperfused at concentrations ranging from 0.1 to 100 µM. Inhibitionof I_AC by ATP began after a delay of 1.5 to 3 min and requiredseveral additional minutes to reach a steady-state value (Fig.1B). ATP inhibited I_AC half-maximally with an estimated 50% inhibitoryconcentration (IC₅₀) of 1.28 µM. Even at maximally effective concentrations,ATP did not completely inhibit I_AC, reducing this current by 71.3± 3.2% (n = 26) and 73.9 ± 3.5% (n = 13) at concentrations of10 and 100 µM, respectively (Fig. 1C). Inhibition of I_AC by ATPwas, in general, poorly reversible even with prolonged washing(Fig. 1B). In contrast to I_AC current, the rapidly inactivatingvoltage-gated A-type current was not reduced by ATP (Fig. 1A).

Inhibition of I_AC by ATP showed evidence of desensitization. When ATP (10 µM) was superfused without previous exposure tothis nucleotide, I_AC was inhibited by a maximum of 83.1 ± 3.3%(n = 11). By comparison, when cells were first exposed to 1 µMATP before superfusing 10 µM ATP, I_AC was inhibited by a maximumof 62.7 ± 3.8% (n = 15) relative to the current amplitude in controlsaline.

The selective inhibition of I_AC by ATP was independent of test voltage. In the experiment illustrated in Fig. 2, I_AC was allowedto grow to a stable value before recording K⁺ currents at test potentials ranging from $-$ 60 to +60 mV in controlsaline and after inhibition by 10 µM ATP. I_AC was inhibited by84 to 90% at all test potentials where I_AC current was large enoughfor accurate measurement ( $-$ 10 to 100 mV) (Fig. 2B). In contrast,the inactivating A-type K⁺ current was insensitive to ATP at each test voltage (Fig. 2A,right traces).

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Fig. 2. Voltage-independent inhibition of I_AC by ATP. K⁺ currents were activated at 30-s intervals by voltage steps of varying size from a holding potential of $-$ 80 mV before and after superfusing the cell with 10 µM NaATP. A, current records at test potentials between $-$ 60 and +60 mV (in 10-mV increments) before and after superfusing ATP, as indicated. B, current-voltage relationships. I_AC current amplitudes from experiment shown in A are plotted against test voltage.

In addition to ATP, several other nucleotides, including ADP, UTP, and UDP, were found to inhibit I_AC with IC₅₀ values of0.24, 0.34, and 3.94 µM, respectively (Fig. 3,A and C). As observedfor ATP, inhibition by these nucleotides was incomplete, evenat maximally effective concentrations. At a concentration of 10µM, ATP inhibited I_AC by 71.3 ± 3.2% (n = 26) whereas ADP, UTP,and UDP reduced I_AC by 69.1 ± 7.2% (n = 4), 81.4 ± 5.2% (n = 7),and 65.1 ± 7.9% (n = 4), respectively (Fig. 3B). Both 2-MeSATPand CTP at concentrations as high as 100 µM failed to significantlyinhibit I_AC (Fig. 3, B and C). The overall order of effectivenessfor I_AC inhibition was UTP $>=$ ATP $>=$ ADP $>=$ UDP [tmt] 2-MeSATP =CTP. Nucleotide receptors were present on each AZF cell, becauseATP, UTP, ADP, and UDP significantly inhibited I_AC in each ofmore than 100 cells tested.

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Fig. 3. Inhibition of I_AC K⁺ current by purines and pyrimidines. A, AZF cells were clamped in whole-cell configuration and voltage steps were applied at 30-s intervals from a holding potential of $-$ 80 mV with (middle) or without (top) 10-s prepulses to $-$ 20 mV. After I_AC reached a maximum amplitude, cells were superfused with UTP, ADP, UDP, 2-MeSATP, or CTP each at a concentration of 10 µM or 200 pM ACTH, as indicated. Current traces and corresponding plots of I_AC amplitude against time before and after superfusion of nucleotides for four representative cells. B, summary of results from experiments such as in A. Bars indicate fraction of I_AC remaining after steady-state block by each nucleotide as indicated. Values are mean ± S.E.M. for the indicated number of cells. C, inhibition curves for 2-MeSATP, ADP, and UTP. Fraction of I_AC remaining is plotted against nucleotide concentration. Data were fit with an equation of the same form as in Fig. 1. N values range from 3 to 7 for each concentration.

Inhibition of I_AC by ATP Involves a G Protein-Coupled Receptor. When AZF cells were voltage clamped at the standardholding potential of $-$ 80 mV, superfusion of ATP never elicited an inwardcurrent, as would have occurred if an ATP-gated nonselective cationchannel were activated. This finding, coupled with the observedorder of effectiveness of nucleotides as inhibitors of I_AC current,suggested that these activated a G protein-coupled nucleotidereceptor of the P2Y family (Filtz et al., 1997; Williams and Burnstock,1997). To determine whether ATP-mediated inhibition of I_AC requiredactivation of a G protein, GTP in the pipette solution was replacedwith the inactive guanine nucleotide GDP- $beta$ -S. With 1 mM GDP- $beta$ -Sin the patch pipette, ATP (10 µM) inhibited I_AC by only 22.8 ±4.5% (n = 18), compared with 71.3 ± 3.2% (n = 26) under controlconditions (Fig. 4).

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Fig. 4. Effect of guanine nucleotides on ATP-mediated I_AC inhibition. I_AC was measured at 30-s intervals as described in the legend of Fig. 1 with standard pipette solution (200 µM GTP) or the same solution containing 1 mM GDP- $beta$ -S in place of GTP. After I_AC reached a stable value, cells were superfused with 10 µM NaATP. A, K⁺ currents were recorded in the presence of GDP- $beta$ -S with (right) and without (left) 10-s prepulses to $-$ 20 mV immediately after initiating whole-cell recording (1), after I_AC had reached a maximum value (2), and after steady-state inhibition by 10 µM ATP (3). B, I_AC amplitudes recorded using pipette solution containing GDP- $beta$ -S either with (open circles) or without (solid circles) depolarizing pulses are plotted against time. C, summary of results from experiments as in A or B. Bars indicate fraction of I_AC remaining after steady-state block by 10 µM ATP with 200 µM GTP or 1 mM GDP- $beta$ -S in pipette as indicated. Results are mean ± S.E.M. of indicated number of cells.

I_AC Inhibition by ATP Is Independent of Phospholipase C (PLC)-Generated Second Messengers. Experiments with GDP- $beta$ -S indicated that ATP-inhibited I_AC through a G protein-coupled receptor. In many cells, the bindingof ATP to G protein-dependent nucleotide receptors is coupledto activation of PLC (Dubyak and El-Moatassim, 1993). PLC-catalyzedcleavage of phosphatidyl inositol 4,5-bisphosphate generates secondmessengers, including diacylglycerol and IP₃, which, respectively,activate protein kinase C and release intracellular Ca⁺⁺. We have explored the possibility that ATP-mediated inhibitionof I_AC occurs through a PLC-activatedpathway.

Calphostin C is a potent, specific antagonist of protein kinase C (IC₅₀ $approx$ 50 nM) (Tamaoki, 1991

). When applied directly tothe cytoplasm of the AZF cell by addition to the pipette solutionat a concentration of 500 nM, calphostin C failed to significantlyalter inhibition of I_AC by 10 µM ATP (Fig. 5,A and C). In thepresence of this antagonist, external ATP inhibited I_AC by 66.4± 6.8% (n = 11), compared with the control value of 71.3 ± 3.2%(n = 26) (Fig. 5C).

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Fig. 5. I_AC inhibition by ATP is independent of kinase C and Ca⁺⁺/calmodulin. K⁺ currents were recorded from AZF cells using the two protocols described in the legend of Fig. 1. Pipettes contained standard internal solution each supplemented with 500 nM calphostin C (A) or 2.5 µM CaM Kinase inhibitory peptide and 20 mM BAPTA (B). After I_AC reached a stable maximum value, cells were superfused with 10 µM NaATP. A and B, calphostin C and calmodulin inhibitory peptide. Current traces recorded with (middle) and without (left) 10-s prepulses to $-$ 20 mV immediately after initiating whole-cell recording (1), after I_AC had reached a maximum value (2), and after block by 10 µM ATP. I_AC amplitudes recorded either with (open circles) or without (solid circles) 10-s prepulses to $-$ 20 mV are plotted against time at right. C, summary of results from experiments as in A and B. Bars indicate fraction of I_AC remaining after block by 10 µM ATP with pipette solutions containing calphostin or calmodulin inhibitory peptide and 20 mM BAPTA as indicated. Results are mean ± S.E.M. of indicated number of experiments.

ATP-stimulated activation of PLC leads to IP₃-induced release of intracellular Ca⁺⁺. Ca⁺⁺ can modulate the function of ion channels through several differentmechanisms. These include direct interaction with the channel,modulation by a Ca⁺⁺-calmodulin complex, or through a Ca⁺⁺-calmodulin-activated enzyme such as Ca⁺⁺-calmodulin kinase II (CaM Kinase II) (Levitan, 1994

; Liu et al.,1994

; Selyanko and Brown, 1996

; Cui et al., 1997

). To determinewhether ATP-mediated inhibition of I_AC occurred through a Ca⁺⁺ or calmodulin-dependent process, we measured the inhibition ofI_AC by ATP using a high-capacity Ca⁺⁺-buffering pipette solution in which Ca⁺⁺ was buffered with 20 rather than 11 mM BAPTA. This pipette solutionwas supplemented further with a calmodulin inhibitory peptide(residues 290-309 of CaM Kinase II) that potently inhibits CaMKinase II and other calmodulin-dependent processes with an IC₅₀of approximately 50 nM (Payne et al., 1988

The high-BAPTA pipette solution supplemented with 2.5 µM calmodulin inhibitory peptide failed to suppress ATP-mediated inhibitionof I_AC. As illustrated in Fig. 5B, the modified pipette solutionhad no effect on the I_AC growth or its selective inhibition by10 µM ATP. Overall, in five similar experiments, ATP (10 µM) inhibitedI_AC by 75.3 ± 8.0%, compared with the control value of 71.3 ±3.2% (n = 26) (Fig. 5C). These results indicate that ATP-mediatedinhibition of I_AC can occur independently of increases in intracellularCa⁺⁺ or activation ofcalmodulin.

Overall, the results of studies with kinase C and the Ca⁺⁺/calmodulin antagonists indicate that I_AC inhibition by ATP is independentof PLC-generated second messengers. U73122 is a PLC antagonistthat inhibits agonist-induced activation of PLC, with an IC₅₀of 1 to 2 µM (Smith et al., 1990

). When U73122 (10 µM) was includedin the pipette solution, it suppressed almost completely the time-dependentincrease in I_AC that is typically observed with pipette solutionscontaining ATP at millimolar concentrations (n = 26). This resultis inconsistent with a mechanism in which PLC activation leadsto inhibition of I_AC K⁺current.

Effect of Staurosporine and AMP-PNP on I_AC Inhibition by ATP. Staurosporine is a potent nonselective protein kinase antagonist. This microbial alkaloid inhibits most serine/threonine proteinkinases, including A kinase, C kinase, and Ca⁺⁺/CaM kinase II with IC₅₀ values of <20 nM (Tamaoki, 1991). Asillustrated in Fig. 6A, staurosporine (1 µM) applied intracellularlythrough the pipette solution markedly reduced the inhibition ofI_AC K⁺ current by 10 µM ATP. In this experiment, ATP inhibited I_AC byless than 5%. In contrast ACTH (100 pM), which functions througha staurosporine-insensitive mechanism (Enyeart et al., 1996),inhibits I_AC almost completely. In a total of nine similar experiments,ATP (10 µM) inhibited I_AC by only 17.3 ± 5.5% when the pipettesolution contained 1 µM staurosporine (Fig. 6C), compared withthe control value of 71.3 ± 3.2% (n = 26).

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Fig. 6. Inhibition of I_AC by ATP is suppressed by staurosporine and AMP-PNP. K⁺ currents were recorded in AZF cells using the two protocols described in the legend of Fig. 1. Patch pipettes contained standard solution supplemented with 1 µM staurosporine (A) or the same solution in which AMP-PNP (1 mM) was substituted for MgATP (B). After I_AC reached a stable amplitude, cells were superfused with 10 µM NaATP. A and B, current traces recorded with (middle) and without (left) 10-s prepulses to $-$ 20 mV immediately after initiating whole-cell recording (1), after I_AC had reached a maximum value (2), after block by 10 µM ATP (3), and after block by 100 pM ACTH (4). I_AC amplitudes recorded either with (open circles) or without (solid circles) 10-s prepulses to $-$ 20 mV are plotted against time at right. C, summary of results from experiments as in A and B. Bars indicate fraction of I_AC remaining after block by 10 µM external ATP with standard pipette solution or the same solution supplemented with staurosporine or one in which AMP-PNP was substituted for MgATP.

Experiments with staurosporine indicated that ATP-mediated inhibition of I_AC required the activity of an unidentified proteinkinase. Accordingly, when the nonhydrolyzable ATP analog AMP-PNP(1 mM) replaced MgATP in the recording pipette, external NaATPwas totally ineffective at inhibiting I_AC (Fig. 6B). Overall,in a total of seven cells, ATP inhibited I_AC by only 2.1 ± 1.6%when AMP-PNP replaced ATP in the pipette solution (Fig. 6C).

Effect of Intracellular UTP on I_AC Inhibition by External ATP. In addition to intracellular ATP, other nucleotides including UTP can, when added to the pipette at millimolar concentrations,activate I_AC K⁺ channels (Enyeart et al., 1997). Although UTP can bind to anintracellular site to activate I_AC K⁺ channels, it does not replace ATP as a substrate for most kinasesor ATPases (Glynn and Hoffman, 1971; Lemaire et al., 1974). When5 mM UTP was substituted for ATP in the pipette solution, externallyapplied ATP (10 µM) failed to inhibit I_AC channels. In five experimentsin which the pipette solution contained only 5 mM UTP and no ATP,external ATP (10 µM) inhibited I_AC by only 2.0 ± 1.7% (Fig. 7).As previously reported, ACTH (100 pM) also failed to inhibit I_ACunder these conditions (Enyeart et al., 1997).

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Fig. 7. Inhibition of I_AC by external ATP requires intracellular ATP. K⁺ currents were recorded with the two voltage protocols described in the legend of Fig. 1. Patch pipettes contained standard solution supplemented with 5 mM NaUTP, either alone or in combination with MgATP at concentrations of 50 µM, 200 µM, 2 mM, or 5 mM, as indicated. After I_AC reached a maximum value, cells were superfused sequentially with ATP (10 µM) and ACTH (100 pM). A, traces show currents recorded with (bottom) and without (top) 10-s depolarizing prepulses to $-$ 20 mV immediately after initiating recording (1), after I_AC had reached a maximum value (2), after superfusing 10 µM NaATP (3), and after superfusing 100 pM ACTH (4). Pipette ATP and UTP concentrations are as indicated. I_AC amplitudes recorded either with (open circles) or without (solid circles) depolarizing prepulses are plotted beneath corresponding traces. B, summary of results of experiments as in A. Bars indicate fraction of I_AC remaining after inhibition by 10 µM external NaATP with pipette solutions containing ATP and UTP at the indicated concentrations. Results are mean ± S.E.M. of the indicated number of determinations.

When the pipette solution was supplemented with 50 µM or 200 µM MgATP, external ATP remained ineffective, inhibiting I_AC byonly 3.43 ± 2.22% (n = 7) and 5.28 ± 3.61 (n = 5), respectively.In contrast, the addition of only 50 µM MgATP to the pipette solutioncompletely restored the near-complete inhibition of I_AC by ACTH(100 pM) (Fig. 7). Raising pipette ATP to 2 or 5 mM in the continuedpresence of 5 mM UTP only partially restored I_AC inhibition byexternal ATP. Specifically, with pipette solutions containing5 mM ATP and UTP, external ATP (10 µM) inhibited I_AC by 49.2 ±2.7% (n = 5) compared with 71.3 ± 3.2% (n = 26) with pipettescontaining only 5 mM ATP (Fig. 7B). These results indicate thatATP and ACTH inhibit I_AC by different mechanisms and further suggestcompetition between UTP and ATP at an intracellular site involvedin ATP-mediated inhibition of thiscurrent.

Effect of Nucleotides on Membrane Potential. In previous studies, we have shown that I_AC K⁺ channels display little voltage dependence and remain open at negative membranepotentials (Mlinar et al., 1993a; Enyeart et al., 1996), characteristicsindicative of a channel that sets the resting potential. Theseresults suggest that ATP and other nucleotides that inhibit I_AC,when applied externally, also should depolarize AZFcells.

In the experiment illustrated in Fig. 8, I_AC was recorded at 30-s intervals until it reached a stable maximum (Fig. 8, trace2, top and bottom). The membrane potential then was recorded afterswitching to current clamp (Fig. 8, bottom), and the cell wassuperfused with either ATP (10 µM) or UTP (10 µM), as indicated.After a delay of 1 to 2 min, both nucleotides produced a steadymembrane depolarization from the resting potential of $-$ 65 to $-$ 70mV. The depolarization reached a stable value at potentials between $-$ 15 and $-$ 5 mV. Upon switching back to voltage clamp, I_AC had beeninhibited by >90% in both cells. In cells where these nucleotidesproduced smaller inhibition of I_AC, membrane depolarization wasproportionately less. Overall, ATP (10 µM) and UTP (10 µM) depolarizedAZF cells by 44.0 ± 6.5 mV (n = 6) and 47.3 ± 6.6 mV (n = 6),respectively. In contrast, CTP (10 µM), which did not inhibitI_AC, depolarized AZF cells by only 1.33 ± 1.3 mV (n = 3).

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Fig. 8. Effect of ATP and UTP on I_AC K⁺ current and membrane potential. K⁺ currents were recorded in the whole-cell mode using the two voltage clamp protocols described in the legend of Fig. 1. When I_AC reached a stable maximum value, membrane potential was recorded upon switching to current clamp and cells were superfused with either 10 µM NaATP (A) or NaUTP (B). K⁺ currents in A and B were recorded with (bottom traces) and without (top traces) 10-s depolarizing prepulses to $-$ 20 mV immediately after initiating whole-cell recording (1), after I_AC had reached a maximum value (2), and after inhibition with ATP (left) or UTP (right) (3). Bottom panels show membrane potential recordings before, during, and after superfusing ATP or UTP as indicated.

	Discussion

Top Summary Introduction Materials and methods Results Discussion References

Bovine AZF cells express a nucleotide receptor that, when activated by ATP, ADP, UTP, and UDP, inhibits I_AC K⁺ current. The order of nucleotide potency and effectiveness ininhibiting I_AC indicates that this receptor is distinct from purine-specificP2Y₁ and P2Y₂ receptors but similar to P2Y₃ receptors (Lustiget al., 1993; Parr et al., 1994; Webb et al., 1996; Filtz et al.,1997; Williams and Burnstock, 1997). Members of the P2Y familyof receptors are coupled through a G protein-to-PLC activation.However, I_AC inhibition by ATP appears to occur through a distinctmechanism involving a staurosporine-sensitive kinase and, possibly,an ATPase. The inhibition of I_AC K⁺ current by nucleotides was tightly correlated with their effectivenessin depolarizing AZF cells. ATP and UTP inhibit I_AC current anddepolarized AZF cells at nearly identical concentrations. 2-MeSATPand CTP were ineffective in bothrespects.

Overall, purine and pyrimidine nucleotides inhibit I_AC and depolarize AZF cells at concentrations identical with those thatstimulate cortisol secretion (Hoey et al., 1994). The common signalingmechanism that emerges from these studies suggests a model forcortisol secretion similar to that previously proposed for ACTHand AII, wherein I_AC inhibition leads to membrane depolarization,Ca⁺⁺ entry through T-type channels, and cortisol secretion (Enyeartet al., 1993).

Nucleotide Receptor Subtype. Patch clamp experiments showed that the nucleotide receptor whose activation was linked to the inhibition of I_AC K⁺ current and membrane depolarization in AZF cells was a G protein-coupledreceptor of the P2Y family. The results clearly demonstrate thatATP and other nucleotides do not function by activation of nonselectivecation channels. In many cells, ATP-induced membrane depolarizationis mediated through activation of these P2X receptors (Dalzieland Westfall, 1994; Williams and Burnstock, 1997). However, inthe course of our studies, ATP and other adenine nucleotides wereapplied to more than 200 AZF cells at a holding potential of $-$ 80mV. An inward current was never activated in any of these cellsupon superfusing thenucleotides.

The rank order of potency and effectiveness of nucleotides as inhibitors of I_AC demonstrate that a P2Y₁ receptor does notmediate this response. P2Y₁ receptors are potently activated by2-MeSATP but are insensitive to UTP (Filtz et al., 1997

; Williamsand Burnstock, 1997

), a profile quite different from that observedfor I_AC inhibition by nucleotides. By comparison, the potent inhibitionof I_AC by ATP and UTP combined with the ineffectiveness of $alpha$ -methyl-thio-ATPare characteristics typical of P2Y₂ receptors (Marrion et al.,1991

; Parr et al., 1994

; Filtz et al., 1997

; Williams and Burnstock,1997

). However, P2Y₂ receptors are insensitive to ADP and UDP,although these nucleotides potently inhibited I_AC (Lustig et al.,1993

; Filtz et al., 1997

). Thus, in spite of the similarities,the nucleotide sensitivity of this receptor, as measured by I_ACblock, is different from that of P2Y₂ receptors. In this regard,a novel G protein-coupled nucleotide receptor has been clonedfrom a chick brain cDNA library with an agonist profile similarto that observed for I_AC inhibition (Webb et al., 1996

). ThisP2Y₃ receptor is activated by ADP and UDP, in addition to ATPand UTP. The chick brain P2Y₃ receptor is coupled to unknowneffectors.

The results of our study are consistent with the hypothesis that purine and pyrimidine nucleotides inhibit I_AC through activationof a P2Y₃ receptor. However, they do not exclude the possibilitythat multiple receptors contributed to I_AC inhibition in AZFcells.

Modulation of Other K⁺ Channels by Nucleotides. Several reports have appeared demonstrating the modulation of specific K⁺ channels by activation of G protein-coupled purinergic receptors.In cardiac myocytes, several different varieties of K⁺ channels are modulated by purinergic receptor activation (Matsuuraand Ehara, 1996; Matsuura et al., 1996). Ca⁺⁺-activated K⁺ channels are activated by purinergic agonists in smooth musclecells and in rat hepatocytes (Yamashita et al., 1996; Vogalisand Goyal, 1997). In none of these cells was the K⁺ channel modulated by pyrimidine nucleotides. Thus, I_AC K⁺ channels are distinctive in their inhibition through P2Y₃ orclosely relatedreceptors.

PLC-Independent Signaling Pathway. Phospholipase C activation is the major signaling pathway that links various P2Y receptors to cellular responses (Dubyak andEl-Moatassim, 1993; Filtz et al., 1997). Accordingly, extracellularATP and UTP stimulate membrane phosphoinositol turnover and releaseof intracellular Ca⁺⁺ in AZF cells (Niitsu, 1992; Hoey et al., 1994). However, ATP-mediatedinhibition of I_AC appears to occur through an alternative signalingpathway. PLC-mediated responses usually are mediated through PKCor Ca⁺⁺, acting either directly or through a calmodulin-dependent process(Berridge, 1993). The complete inability of the potent kinaseC antagonist calphostin C to suppress ATP-mediated inhibitionof I_AC when applied directly to the cytoplasm through the patchelectrode at 10 times the reported IC₅₀ is convincing evidencethat activation of this enzyme is not necessary for this response.However, we cannot state with certainty that PKC was inhibitedcompletely in theseexperiments.

In whole-cell patch clamp experiments, ion channel modulation mediated directly by Ca⁺⁺ or indirectly through calmodulin is usually suppressed or eliminatedby strongly buffering Ca⁺⁺ in the pipette solution with 20 mM BAPTA or by adding a calmodulinantagonist to this solution (Marrion et al., 1991

; Liu et al.,1994

; Yu et al., 1994

). Because both of these measures in combinationfailed to blunt ATP-mediated inhibition of I_AC, it is unlikelythat Ca⁺⁺ released in response to PLC-mediated synthesis of IP₃ was involvedin I_ACinhibition.

Finally, if ATP-mediated inhibition of I_AC occurred through activation of PLC, a PLC antagonist such as U73122 would be expectedto enhance, rather than inhibit, I_AC expression. However, it ispossible that U73122 inhibited I_AC by a mechanism independentof PLC. Overall, our results strongly indicate that ATP-mediatedinhibition of I_AC occurs through a PLC-independentpathway.

The specific pathway by which ATP and other nucleotides inhibit I_AC remains to be identified. The ability of 1 µM staurosporineto prevent I_AC inhibition by ATP indicates that a protein kinaseis involved. However, at a concentration of 1 µM, staurosporinecompletely inhibits each of the serine/threonine kinases thathave been described, as well as a number of tyrosine kinases (Tamaoki,1991

). The protein kinase whose activity is required for inhibitionof I_AC by external ATP remains to beidentified.

I_AC Inhibition and ATP Hydrolysis. Inhibition of I_AC by external ATP also was prevented by substitution of the nonhydrolyzable ATP analog AMP-PNP or the pyrimidineUTP for ATP in the pipette. This result is not surprising, inview of the fact that neither of these nucleotides acts as a substratefor protein kinases (Azhar and Menon, 1975; Krebs and Beavo, 1979).However, the ineffectiveness of external ATP when the pipettecontained 200 µM MgATP in addition to 5 mM UTP was unexpected.Protein kinases are fully activated by ATP at concentrations lessthan 50 µM (Glynn and Hoffman, 1971; Lemaire et al., 1974), whereascellular ATPases have K_m values for ATP of several millimolar(Hilgemann, 1997). Thus, inhibition of I_AC by nucleotide receptoractivation may require both active kinases as well as ATPases,as appears to be the case for the cystic fibrosis transmembraneconductance regulator Cl channel, where channel gating is fueled by the energy of ATPhydrolysis but depends also on channel phosphorylation by a proteinkinase (Baukrowitz et al., 1994). Alternatively, UTP might actas a competitive antagonist of ATP at its binding site on theprotein kinase responsible for I_AC inhibition. However, to ourknowledge, UTP has not been shown to inhibit proteinkinases.

I_AC Inhibition: Comparison of ATP, ACTH, and AII Signaling Pathways. ATP-mediated inhibition of I_AC occurs through a mechanism that is clearly different from that of ACTH. In contrast to ATP,inhibition of I_AC by ACTH is unaffected by staurosporine. Furthermore,when I_AC is activated by pipette solutions containing 5 mM UTP,50 µM MgATP in the pipette is sufficient to restore complete inhibitionof I_AC by ACTH (100 pM). Under the same conditions, externallyapplied ATP (10 µM) produced no inhibition of I_AC.

Inhibition of I_AC by externally applied ATP does resemble AII-mediated inhibition in several respects. AII inhibits I_AC througha losartan-sensitive receptor that is known to be coupled to activationof PLC (Mlinar et al., 1995

). However, AII-mediated inhibitionof I_AC, similar to ATP-mediated inhibition, occurs through a PLC-independentpathway. Inhibition of I_AC by AII is also suppressed by staurosporine(Mlinar et al., 1995

). These results suggest that external ATPand AII are coupled to I_AC inhibition by a novel, common pathwaythat is different from that used byACTH.

Nucleotide-Mediated Inhibition of I_AC and Membrane Depolarization. Bovine AZF cells express three types of ion channels, including rapidly inactivating Ca⁺⁺ and K⁺ channels and noninactivating K⁺ channels (Mlinar et al., 1993a,b; Mlinar and Enyeart, 1993).Of these, only I_AC channels are open at negative membrane potentialsand exhibit little voltage-dependent gating. It is likely thatthese channels are largely responsible for determining the restingpotential of these cells (Mlinar et al., 1993a; Enyeart et al.,1996; Enyeart et al., 1997). Accordingly, ACTH, AII, ATP, andUTP all depolarize AZF cells at concentrations that maximallyinhibit I_AC. Thus, nucleotides and peptide hormones that inhibitI_AC through activation of three different receptors share theability to depolarize AZF cells and stimulate large (>50-fold)increases in cortisol secretion (Enyeart et al., 1993; Mlinaret al., 1993a; Mlinar et al., 1995).

ACTH-stimulated cortisol secretion is inhibited by T-type Ca⁺⁺ channel antagonists at concentrations identical with those thatinhibit T-type Ca⁺⁺ currents in these cells (Enyeart et al., 1993

). These findingsemphasize the importance of depolarization-dependent Ca⁺⁺ entry through voltage-gated Ca⁺⁺ channels in ACTH-stimulated cortisol secretion. Whether ATP-stimulatedcortisol secretion also requires Ca⁺⁺ entry through T-type Ca⁺⁺ channels is not known, but a requirement for external Ca⁺⁺ in nucleotide-stimulated cortisol secretion has been established(Niitsu, 1992

Physiological Relevance. The physiological significance of external ATP or other nucleotides in the regulation of cortisol secretion is not well established.ATP and other purines are stored and released, along with catecholamines,from secretory granules of adrenal medullary chromaffin cells(Glynn and Hoffman, 1971). In addition to nucleotide receptors,adrenal zona fasciculata cells also express $beta$ -adrenergic receptorsthat, when activated, stimulate cortisol secretion (Kawamura etal., 1984; Walker et al., 1988). Rays of adrenal medullary tissuehave been reported to traverse the adrenal cortex, and clustersof chromaffin cells have been reported to exist in all three regionsof the adrenal cortex (Nussdorfer, 1996). Overall, these resultssuggest that ATP and other nucleotides released from adrenal chromaffincells, along with catecholamines, may act in a paracrine fashionto modulate I_AC current and cortisol secretion in bovine AZFcells.

In this regard, it is important to point out that virtually all of the more than 200 normal AZF cells that we tested expressedthe P2Y₃-type nucleotide receptor as measured by the inhibitionof I_AC current. These receptors were present in the freshly isolatedAZF cells, because these cells were never cultured for more thanseveral hours before use in patch clampexperiments.

A final possibility is that ATP released from AZF cells could act in an autocrine fashion to regulate I_AC and cortisol secretion.A mechanism similar to this appears to function in airway epithelialcells, where the cystic fibrosis transmembrane conductance regulatortriggers the transport of ATP out of the cell, where it acts toactivate chloride channels through activation of a P2U receptor(Schwiebert et al., 1995

). It is interesting that the cystic fibrosistransmembrane conductance regulator-associated chloride channel,as well as the I_AC K⁺ channel, may both be activated by the nonhydrolytic binding ofintracellular ATP (Quinton and Reddy, 1992

), but inhibited byextracellular ATP through activation of a G protein-coupled nucleotidereceptor.

In summary, we have discovered a new signaling pathway in which a nucleotide receptor with a P2Y₃ agonist is profile-coupledthrough a G protein to inhibition of I_AC K⁺ channels and depolarization of AZF cells. This suggests a specificmechanism for ATP-stimulated cortisol secretion that depends ondepolarization-dependent Ca⁺⁺ entry. This may be an important physiological mechanism linkingstress-induced chromaffin cell secretion to corticosteroidproduction.

	Footnotes

Received September 14, 1998; Accepted November 13, 1998

J.J.E. was supported by National Institute of Diabetes and Digestive and Kidney Grant DK-47875 and by National American HeartAssociation Grant-in-Aid94011740.

Send reprint requests to: Dr. John J. Enyeart, Department of Pharmacology, The Ohio State University College of Medicine, 5190 Graves Hall, 333 W. 10th Avenue, Columbus, OH 43210-1239. E-mail: enyeart.1{at}osu.edu

	Abbreviations

I_AC, noninactivating potassium current in bovine adrenal fasciculata cells; 2-MeSATP, 2-methylthio-ATP; AZF, bovine adrenal fasciculata; BAPTA, 1,2-bis-(2-aminophenoxy)ethane-N, N,N',N'-tetraacetic acid; IC₅₀, 50% inhibitory concentration; AMP-PNP, 5'-adenylyl-imidodiphosphate; GDP- $beta$ -S, guanosine 5'-O-2-(thio) diphosphate; DMEM, Dulbecco's modified Eagle's medium; PLC, phospholipase C; ACTH, adrencorticotropic hormone; PBS, phosphate-buffered saline.

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