The Steroid Promegestone Is a Noncompetitive Antagonist of the Torpedo Nicotinic Acetylcholine Receptor that Interacts with the Lipid-Protein Interface

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Vol. 55, Issue 2, 269-278, February 1999

The Steroid Promegestone Is a Noncompetitive Antagonist of the Torpedo Nicotinic Acetylcholine Receptor that Interacts with the Lipid-Protein Interface

Michael P. Blanton,¹ Yu Xie,² Lawrence J. Dangott,³ and Jonathan. B. Cohen

Department of Neurobiology, Harvard Medical School, Boston, Massachusetts

	Summary

Top Summary Introduction Materials and methods Results Discussion References

17,21-Dimethyl-19-nor-pregn-4,9-diene-3,20-dione (promegestone) was used to characterize the mechanism of inhibition of nicotinicacetylcholine (ACh) receptors (AChR) by progestin steroids. Promegestonereversibly inhibited ACh-induced currents of Torpedo AChRs expressedin Xenopus oocytes. Between 1-30 µM promegestone produced a concentration-dependentenhancement of the equilibrium binding affinity of [³H]ACh to Torpedo AChR-rich membranes. For AChRs in the presenceof agonist (desensitized state) promegestone was a more potentinhibitor of the binding of the noncompetitive antagonist [³H]phencyclidine (IC₅₀ = 9 µM) than of [³H]histrionicotoxin (IC₅₀ ~ 100 µM). To identify AChR domains incontact with the steroid, AChR-rich membranes equilibrated with[³H]promegestone were irradiated at 312 nm, and ³H-labeled amino acids were identified by amino-terminal sequencingof fragments isolated from subunit proteolytic digests. WithinAChR $alpha$ -subunit, 70% of ³H was covalently incorporated in a 10-kDa fragment beginning atAsn-339 and containing the M4 membrane spanning segment, and 30%was in a 20-kDa fragment beginning at Ser-173 and containing theM1-M3 segments. Fragments containing the M2 channel domains aswell as the M4 segments were isolated from proteolytic digestsof AChR subunits and subjected to amino-terminal sequence analysis.No evidence of [³H]promegestone incorporation was detected in any of the M2 segments.The amino acids in the M4 segments labeled by [³H]promegestone were among those previously shown to be in contactwith the lipid bilayer (Blanton and Cohen, 1994). These resultsindicate that the steroid promegestone is an AChR noncompetitiveantagonist that may alter AChR function by interactions at thelipid-proteininterface.

	Introduction

Top Summary Introduction Materials and methods Results Discussion References

Steroid hormones, including endogenously occurring metabolites of progesterone, testosterone, and deoxycorticosterone, aswell as synthetic derivatives, act as allosteric modulators ofthe nicotinic acetylcholine (ACh) receptor (AChR) family of ligand-gatedion channels (reviewed in Franks and Lieb, 1994; MacDonald andOlsen, 1994; Lambert et al., 1995). Progesterone is a weak allostericpotentiator of type A $gamma$ -aminobutyric acid (GABA_A) receptors (Wuet al., 1990), whereas endogenous and synthetic 3 $alpha$ -hydroxy derivativesact at submicromolar concentrations (Harrison et al., 1987; Geeet al., 1995). In contrast, at micromolar concentrations progesteroneand its derivatives inhibit ACh-activated responses of both neuronaland muscle-type AChRs (Gillo and Lass, 1984; Valera et al., 1992;Ke and Lukas, 1996; Bullock et al., 1997) as well as glycine receptor-activatedcurrents in spinal cord neurons (Wu et al., 1990). For GABA_A receptorselectrophysiological studies show that potentiation by steroidsis not associated with changes in channel conductance but withan increase in open channel probability at low agonist concentrationsand an alteration of the kinetics of desensitization at high agonistconcentrations (Twyman and MacDonald, 1992; Lambert et al., 1996;Zhu and Vicini, 1997). For muscle AChR, single-channel analysesof the acute effects of hydrocortisone and corticosterone indicatea dose-dependent decrease in the mean channel open time (Bouzatand Barrantes, 1996; Nurowska and Ruzzier, 1996). Although a mutationwithin the M2 ion channel domain that increases channel lifetimealso increases hydrocortisone potency, there was no evidence forhydrocortisone competition with QX-222, an open channel blocker(Bouzat and Barrantes, 1996). Because substitutions of amino acidswithin AChR M4 hydrophobic segments at the lipid-protein interfacecan result in alteration of the duration of the open channel state(Bouzat et al., 1994; Lee et al., 1994; Lasalde et al., 1996),it is possible that steroid interactions with the AChR at thelipid interface result in functionalantagonism.

To identify binding sites for progestin steroids in AChRs, we have characterized interactions of 17,21-dimethyl-19-nor-pregn-4,9-diene-3,20-dione(promegestone) with AChR-rich membranes isolated from the electricorgan of the marine elasmobranch Torpedo californica. UV irradiationof promegestone results in the formation of a triplet-state biradicalat the 3' ketone allowing a covalent bond to be formed betweenthe steroid and an adjacent polypeptide (Benisek, 1977). Photoincorporationof [³H]promegestone has been used to identify several different progesteronereceptors (Sadler and Maller, 1982; Stromstedt et al., 1990).The Torpedo electric organ is an extremely rich source of muscle-typeAChR containing upwards of 100 mg of receptor protein/kg electroplacquetissue, thus facilitating the use of protein chemistry techniquesto identify sites of photoincorporation of competitive and noncompetitiveantagonists (reviewed in Hucho et al., 1996).

We report here that promegestone reversibly inhibits ACh-evoked currents of Torpedo AChR expressed in Xenopus oocytes andthat it interacts with both the resting and desensitized statesof the AChR, inhibiting the specific binding of radiolabeled noncompetitiveantagonists to Torpedo AChR-rich membranes in the absence andin the presence of carbamylcholine, respectively. [³H]Promegestone photoincorporates into each of the AChR subunitswith the extent of incorporation insensitive to AChR conformationalstate. No evidence of [³H]promegestone incorporation was detected in any of the channellining M2 segments, but labeled residues were identified in theM4 hydrophobic segments at positions shown previously to be atthe AChR-lipid interface. These results support the hypothesisthat inhibition of AChRs by progestin steroids results from directinteractions at the AChR-lipidinterface.

	Materials and Methods

Top Summary Introduction Materials and methods Results Discussion References

Materials. [³H]Promegestone (86.7 Ci/mmol; Fig. 1), nonradioactive promegestone, and [³H]phencyclidine ([³H]PCP; 52 Ci/mmol) were obtained from New England Nuclear (Boston,MA). [³H]Tetracaine (36 Ci/mmol) and [³H]histrionicotoxin ([³H]HTX, 60 Ci/mmol) were prepared at New England Nuclear by thetritium gas catalytic reduction of 3,5 dibromotetracaine and dl-decahydro(pentyl)histrionicotoxin,respectively. [³H]HTX was diluted with dl-perhydrohistrionicotoxin (HTX) to aradiochemical specific activity of 3 Ci/mmol for binding assays.1-Azidopyrene (1-AP) was purchased from Molecular Probes (Eugene,OR). L-1-tosylamido-2-phenylethyl chloromethyl ketone-treatedtrypsin was purchased from Worthington Biochemical Corp. (Freehold,NJ), endoproteinase Lys-C (EKC) from Boehringer Mannheim (Indianapolis,IN) and Genapol C-100 (10%) from Calbiochem (La Jolla, CA). Prestainedlow molecular weight gel standards were purchased from Life Technologies,Inc. (Gaithersburg, MD)

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Fig. 1. Structure of [³H]promegestone [17 $alpha$ -methyl-³H]

AChR-Rich Membranes. AChR-rich membranes were isolated from the electric organ of T. californica (Marinus, Inc., Westchester, CA) as describedpreviously (Pedersen et al., 1986). The final membrane suspensionsin 36% sucrose/0.02% NaN₃ were stored at $-$ 80°C under argon andcontained 1-1.5 nmol of ACh binding sites/mg of protein as measuredby a direct [³H]AChR binding assay (Pedersen et al., 1986).

Electrophysiological Recordings. Plasmid cDNAs (pMXT) encoding wild-type $alpha$ -, $gamma$ -, and $delta$ -subunits of Torpedo AChR were gifts from Dr. Michael White (AlleghenyHealth Sciences University, Philadelphia, PA), and the $beta$ -subunitcDNA (pSP64 vector) was from Dr. Henry Lester (California Instituteof Technology, Pasadena, CA). cDNAs were linearized with eitherXbaI (for $alpha$ -, $gamma$ -, and $delta$ -subunits) or FspI (for $beta$ -subunit). LinearDNAs were transcribed in vitro with SP6 RNA polymerase (Promega,Madison, WI). Isolated follicle-free oocytes were microinjectedwith 10 ng of subunit-specific RNAs in a molar ratio of $alpha$ ₂ $beta$ $gamma$ $delta$ .Oocytes were maintained in low-Ca⁺⁺ ND96 solution containing 96 mM NaCl, 2 mM KCl, 0.3 mM CaCl₂,1 mM MgCl₂, 5 mM HEPES ,and 50 µg/ml gentamicin (pH 7.6) for atleast 48 h before use. Currents elicited by ACh were measuredwith a standard two-electrode voltage-clamp (OC-725B, Warner InstrumentCorp., Hamden, CT) at a holding potential of $-$ 70 mV. Electrodeswere filled with 3 M KCl and had resistance of 0.5-3.0 M $Omega$ . Therecording chamber (~150 µl in volume) was continually perfusedby gravity with low-Ca⁺⁺ ND96 (+1 µM atropine, pH 7.6). Stock solutions of steroid wereprepared in ethanol and then diluted in low-Ca⁺⁺ ND96 so that the oocytes were exposed to ethanol concentrations<1% (v/v). Various concentrations of steroid were applied simultaneouslywith 3 µM ACh for 5 s through solenoid valves to the oocyte inthe recording chamber. In some experiments, progesterone was perfusedcontinuously through the chamber for up to 5 min, with responsesto ACh testedperiodically.

Binding of Cholinergic Ligands to AChR-Rich Membranes. Centrifugation assays were used to determine the equilibrium binding of [³H]ACh, [³H]HTX, [³H]PCP, and [³H]tetracaine to Torpedo AChR-rich membranes in Torpedo physiologicalsaline (TPS; 250 mM NaCl, 5 mM KCl, 3 mM CaCl₂, 2 mM MgCl₂, 5mM sodium phosphate, pH 7.0.). The final concentration of ethanolwas <0.3% (v/v) for [³H]ACh or equal to 1% (v/v) for the ³H noncompetitive antagonists. For [³H]ACh, membrane suspensions (50 µg/ml of protein, 50 nM ACh bindingsites) were pretreated with 0.3 mM diisopropylphosphofluoridateto inhibit acetylcholinesterase. Membranes were equilibrated at4°C with [³H]ACh (50 nM) and varying concentrations of noncompetitive antagonistfor 30 min, and 0.5 ml aliquots were centrifuged for 45 min at10,000 rpm in a Sorvall SA-600 rotor. After complete removal ofthe supernatant, membrane pellets were resuspended in 0.1 ml of10% SDS and pellet ³H was determined by liquid scintillation counting. For the ³H noncompetitive antagonists, membrane suspensions (0.5 mg ofprotein/ml, 0.6 µM ACh binding sites) were equilibrated with radioligandand appropriate concentrations of modulatory drug for 2-3 h atroom temperature ([³H]HTX, 10 nM) or at 4°C ([³H]PCP, 6 nM; [³H]tetracaine, 2 nM) before centrifugation. Nonspecific bindingof [³H]ACh was measured in the presence of 0.1 mM carbamylcholine,that of [³H]HTX and [³H]PCP in the presence of 0.2 mM meproadifen, and that of [³H]tetracaine in the presence of 0.2 mMtetracaine.

Photolabeling AChR-Rich Membranes with [³H]Promegestone. Membranes in TPS (2 mg of protein/ml) were incubated with [³H]promegestone at a final concentration 80-110 nM in the absenceor presence of 0.2 mM carbamylcholine. After a 1-h incubation,suspensions were irradiated for 7 min at a distance of <1 cm witha 312-nm lamp (EB-Spectroline, Spectronics, Westbury, NY). Eachsample was then pelleted (15,000g), and for analytical labelingsthe pellets were then solubilized in sample loading buffer (Laemmli,1970) and submitted to SDS-polyacrylamide gel electrophoresis(PAGE). For preparative scale labelings (12-15 mg of AChR-richmembranes), the pellets were then resuspended in TPS at 2 mg/mlof protein and 1-AP was added to a final concentration of 350µM. After a 30-min incubation, membranes were once again irradiated(365 nm for 5 min, at <1 cm; EN-Spectroline,) and each samplewas pelleted. Samples were then solubilized in electrophoresissample loading buffer and submitted to preparative scale SDS-PAGE.Labeling with the fluorescent hydrophobic probe 1-AP was usedto assist in the initial identification and isolation of AChRsubunits and in the subsequent isolation of hydrophobic segmentsof these subunits (Blanton and Cohen, 1994).

SDS-PAGE. SDS-PAGE was performed as described (Laemmli, 1970) with either 1.0-mm (analytical) or 1.5-mm thick (preparative scale) 8%T (total acrylamide concentration), 4% bis-acrylamide cross-linkerconcentration relative to total acrylamide concentration (C).For analytical gels, polypeptides were visualized by stainingwith Coomassie blue R-250 (0.25% w/v in 45% methanol and 10% aceticacid) and destaining in 25% methanol and 10% acetic acid. Thegels were then impregnated with fluor (Amplify; Amersham, ArlingtonHeights, IL) for 20 min with rapid shaking, dried, and exposedat $-$ 80°C to X-OMAT LS film (Eastman Kodak Co., Rochester, NY)for various times (4-16 weeks). For preparative scale gels, polypeptidesincorporating 1-AP were visualized from their associated fluorescencewhen the gels were illuminated at 365 nm on a UV-light box. Bandscorresponding to AChR subunits were excised either for polypeptideisolation or in the case of the AChR $alpha$ -subunit for proteolyticdigestion once the gel piece was transferred to the well of a15% mapping gel (Cleveland et al., 1977; Pedersen et al., 1986).Mapping gels were composed of a 4.5% T, 2.6% C stacking gel anda 15% T, 2.6% C separating gel. The $alpha$ -subunit gel piece was overlaidwith 350 µl of buffer (5% sucrose, 125 mM Tris-HCl, 0.1% SDS,pH 6.8) containing 250 µg of Staphylococcus aureus V8 protease.Electrophoresis was carried out overnight at 15 mA constantcurrent.

1-AP/[³H]promegestone-labeled proteolytic fragments were isolated from the excised gel pieces by a passive elution protocolas described in (Blanton and Cohen, 1994

). The eluate was filtered(Whatman 1), and the protein concentrated with a Centriprep-10(Amicon, Inc., Beverly, MA). Excess SDS was removed by acetoneprecipitation (overnight at $-$ 20°C).

Purification of Proteolytic Digests of [³H]Promegestone/1-AP-Labeled AChR Subunits. For EKC digestion, the acetone-precipitated 20-kDa V8 protease fragment of the $alpha$ -subunit ( $alpha$ V8-20; Ser-173-Glu-338) was resuspendedin 15 mM Tris-HCl, 0.1% SDS (pH 8.1), at 1-2 mg/ml protein. Approximately1.5 U of EKC were added and incubated at room temperature for6 days. The $beta$ - and $delta$ -subunits and the 10-kDa fragment of the $alpha$ -subunit( $alpha$ V8-10) (Asn-339-Gly-437) were digested with trypsin exactlyas described (Blanton et al., 1998). Both trypsin and EKC digestswere separated on individual 1.5-mm thick 16.5% T, 6% C tricineSDS-PAGE gels (Schagger and von Jagow, 1987; Blanton et al., 1998).

Proteolytic fragments containing either the M2 or M4 region of each of the receptor subunits were identified and isolatedby two different sets of criteria: Under conditions nearly identicalwith those used here, it has been previously determined whereproteolytic fragments containing the M2 and M4 regions migraterelative to Life Technologies (GIBCO/BRL, Gaithersburg, MD) prestainedmolecular weight standards (White and Cohen, 1992

; Pedersen etal., 1992

; Blanton et al., 1998

). In addition, fragments wereselected that contain both the M2 and M3 region so that incorporationof 1-AP into the M3 segment (Blanton and Cohen, 1994

) could beused to visualize the fragments by illuminating the tricine SDS-PAGEgel at 365 nm on a UV-light box. Incorporation of 1-AP into theM4 segment was also used as an aid in identifying fragments containingthisregion.

1-AP/[³H]promegestone-labeled fragments were further purified by reverse-phase high-pressure liquid chromatography (HPLC) asdescribed (Blanton et al., 1998

) with a Brownlee Aquapore C₄ column(100 × 2.1 mm). Solvent A was 0.08% trifluoroacetic acid in water,and solvent B was 0.05% trifluoroacetic acid in 60% acetonitrile/40%2-propanol. The elution of [³H]promegestone was monitored by scintillation counting of an aliquot(25 µl) of each 0.5-mlfraction.

Sequence Analysis. Amino-terminal sequence analysis was performed on a ABI model 477A (Applied Biosystems, Foster City, CA) protein sequencerwith gas phase cycles. Pooled HPLC samples were dried by vacuumcentrifugation, resuspended in a small volume of 0.05% SDS (~20µl), and immobilized on chemically modified glass fiber disks(Beckman Instruments). Approximately 30% of the released phenylthiohydantoin(PTH)-amino acids were separated by an on-line model 120A PTH-aminoacid analyzer, and ~60% was collected for determination of released³H by scintillation counting of each sample for three 5-min intervals.Initial yield (I_o) and repetitive yield (R) were calculated bynonlinear least-squares regression of the observed release (M)for each cycle (n): M = I_oRⁿ (PTH-derivatives of Ser, Thr, Cys, and His were omitted fromthefit).

	Results

Top Summary Introduction Materials and methods Results Discussion References

To determine whether promegestone was an antagonist of Torpedo AChRs, we tested it as an inhibitor of AChRs expressed in Xenopusoocytes. When coapplied for 5 s with ACh, promegestone produceda dose-dependent and reversible inhibition of the ACh-inducedcurrents (Fig. 2A). In the absence of promegestone, the ACh concentration-responserelation was characterized by K_ap = 20 µM and a Hill coefficientof 1.8 (data not shown). When applied in the presence of 3 µMACh, 30 µM promegestone produced ~50% reduction of the peak currentresponse, whereas that same concentration resulted in a 90% reductionof the current seen after 5 s exposure. After a 1-min wash afterexposure to 30 µM promegestone, there was a 50% recovery of theACh peak current and a full recovery within 5 min. The potencyof promegestone as well as its kinetics of inhibition were similarto that of progesterone (Fig. 2B). Although the time-dependentdecrease of the ACh-response could indicate that both steroidsincrease the rate of agonist-dependent desensitization, it wasalso possible that neither steroid equilibrated with its bindingsite during the 5 s exposure. To determine whether kinetic factorswere important determinants of the extent of inhibition seen forthese drugs, ACh responses were determined after preincubationwith progesterone. When oocytes were perfused with 1 µM progesteronefor 5 min, there was a dramatic, time-dependent increase in progesteronepotency, with 50% inhibition of the peak current seen after a60-s preincubation (Fig. 2C). After 5 min, the peak current wasreduced by 65%, and after a 2.5-min wash, there was a 40% recoveryof the peak response (not shown). Although further experimentationis required to analyze the time and concentration dependence ofthe observed inhibition, these first experiments established thatpromegestone was in fact an AChR antagonist similar in potencyand action to progesterone.

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Fig. 2. Inhibition of ACh-evoked currents of Torpedo AChRs expressed in Xenopus oocytes by promegestone and progesterone. Currents elicited by ACh from Torpedo AChRs expressed in Xenopus oocytes were measured with a standard two-electrode voltage clamp at a holding potential of $-$ 70 mV. A, once a stable response was observed for 3 µM ACh, responses were measured when ACh was applied simultaneously for 5 s with 10 and then 30 µM promegestone, or B, with 1, 3, and then 10 µM progesterone. Inhibition by promegestone and progesterone was reversible, because peak responses to ACh returned to control levels after exposure to 30 µM promegestone or to 10 µM progesterone (not shown). C, current response was recorded when 3 µM ACh was applied for 5 sec (Control), and then progesterone (1 µM) was applied continuously for 5 min, with test pulses of 3 µM ACh (and progesterone) at the indicated times. After 5 min exposure, the peak current was reduced to 35% of control, and after a 2.5 min wash there was a recovery to 60% of control (not shown).

Effects of Promegestone on [³H]ACh and ³H-Noncompetitive Antagonist Binding to Torpedo Membranes. Equilibrium binding of [³H]ACh was assayed at a concentration sufficient to occupy ~20% of sites. At this subsaturating concentration,the assay is sensitive to drugs that either increase or decreaseACh binding affinity (Boyd and Cohen, 1984). Promegestone at concentrationsup to 100 µM did not inhibit the equilibrium binding of [³H]ACh, and, in fact, at concentrations between 1 and 30 µM itincreased binding by 50% (Fig. 3A). In comparison, proadifen,an aromatic amine noncompetitive antagonist known to stabilizethe desensitized state of the AChR (Boyd and Cohen, 1984), increased[³H]ACh binding by 300%.

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Fig. 3. Effects of promegestone on the equilibrium binding of [³H]ACh, [³H]histrionicotoxin, [³H]phencyclidine, and [³H]tetracaine. A, AChR-rich membranes suspensions (50 µg protein/ml, 50 nM ACh binding sites), pretreated with diisopropylphosphofluoridate, were equilibrated at 4°C for 30 min with [³H]ACh (50 nM) and promegestone ( $bullet$ ) or proadifen ( $black-triangle$ ), and bound [³H]ACh was determined by a centrifugation assay. B, AChR membranes (0.5 mg/ml, 0.6 µM ACh binding sites) were equilibrated at room temperature for 2 to 3 h with 10 nM [³H]HTX in the absence (

) or presence ( $black-square$ ) of carbamylcholine, with 6 nM [³H]PCP in the presence of carbamylcholine ( $bullet$ ), or with 2 nM [³H]tetracaine ( $black-triangle$ ) and the indicated concentrations of promegestone. Specific binding was determined as the difference between the total binding and the nonspecific binding in the presence of either 200 µM tetracaine (for [³H]tetracaine) or 200 µM meproadifen. In the absence of promegestone, [³H]HTX total binding was 4000 ³H cpm in the absence and 4200 in the presence of carbamylcholine, and 350 ³H cpm were bound nonspecifically. For [³H]PCP, total and nonspecific binding were 15,000 and 2,500 ³H cpm, respectively, and for [³H]tetracaine they were 69,200 and 22,500 cpm.

Promegestone was also tested as an inhibitor of the equilibrium binding of radiolabeled, positively charged AChR noncompetitiveantagonists (NCAs) (Fig. 3B). [³H]HTX is bound at equilibrium with high affinity to a single sitein the AChR in the absence (resting state, K_eq = 1 µM) or presenceof agonist (desensitized state, K_eq = 0.3 µM) (Heidmann et al.,1983

). [³H]Phencyclidine ([³H]PCP) binds with high affinity (K_eq = 1 µM) to a single siteper AChR in the desensitized state (Heidmann et al., 1983

). [³H]Tetracaine binds with high affinity (K_eq = 0.3 µM) in the absenceof agonist to a single site per AChR and it is bound only weakly(K_eq = 30 µM) in the desensitized state (Cohen et al., 1985

).Based on photoaffinity labeling, the [³H]tetracaine binding site has been localized within M2 ion channeldomain (Gallagher and Cohen, 1994

; Gallagher, 1996

). In the presenceof agonist, promegestone was a potent inhibitor of [³H]PCP binding. High concentrations inhibited specific bindingby >95%, and the concentration dependence of inhibition couldbe modeled as competitive with IC₅₀ = 9 µM (Fig. 3B). In contrast,100 µM promegestone did not inhibit [³H]HTX binding in the absence of agonist and produced only partialinhibition in the presence of agonist. For [³H]tetracaine in the absence of agonist, high concentrations ofpromegestone inhibited binding by at least 80% with an IC₅₀ of75 µM.

Photoincorporation of [³H]Promegestone in the AChR. Experiments were first designed to characterize the general pattern of [³H]promegestone photoincorporation into Torpedo AChR-rich membranes,as well as to test the sensitivity of the photoincorporation tocholinergic ligands. Membranes (2 mg/ml) were equilibrated with80 nM [³H]promegestone in the absence and in the presence of 200 µM carbamylcholine.This promegestone concentration provided a sufficient level ofradioactivity to detect AChR subunit labeling even though onlya small amount of the total ³H (~2%) was incorporated. After irradiation, membrane suspensionswere pelleted and resuspended in electrophoresis sample buffer,and the pattern of incorporation was monitored by SDS-PAGE followedby fluorography. As is evident in the fluorograph of an 8% polyacrylamidegel (Fig. 4), there was incorporation of [³H]promegestone into each of the AChR subunits. Neither the patternof incorporation into individual AChR subunits nor the overalllabeling pattern was affected by the inclusion of 200 µM carbamylcholine(Fig. 4, lane 2). The additional presence of nonradioactive progesterone(1.2 µM, 12 µM, and 100 µM) had no observable effect on the extentof incorporation into any of the AChR subunits either in the presenceor absence of agonist (data not shown). Based upon quantificationof ³H incorporation in excised gel slices, ~0.1% of $alpha$ -subunits werelabeled with the relative incorporation within subunits: $alpha$ / $beta$ / $gamma$ / $delta$ :1.6/1.1/1.2/1in the absence of agonist. Similar ratios were seen for photolabelingin the presence of agonist as well as from the amount of ³H present in subunits isolated from preparative scale labelings.

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Fig. 4. Photoincorporation of [³H]promegestone into AChR-rich membranes in the absence and in the presence of carbamylcholine. AChR-rich membranes were equilibrated with 80 nM [³H]promegestone in the absence (lane 1) or presence (lane 2) of 200 µM carbamylcholine and irradiated at 312 nm for 7 min. After photolysis, polypeptides were resolved on a 8% polyacrylamide gel and processed for fluorography (5-week exposure). The bulk of the labeled lipid and free photolysis products were electrophoresed from the gel with the tracking dye. AChR subunits and the Na⁺/K⁺ ATPase $alpha$ -subunit ( $alpha$ _NK) are indicated on the left.

The distribution of [³H]promegestone incorporation within the AChR $alpha$ -subunit was examined by determining the amount of labelingin two large proteolytic fragments generated by limited S. aureusV8 protease digestion on a mapping gel: $alpha$ V8-20 (Ser-173-Glu-338),containing the membrane spanning segments M1-M3, and $alpha$ V8-10 (Asn-339-Gly-439),containing the membrane spanning segment M4 (Pedersen et al.,1986

; White and Cohen, 1988

). In the fluorograph of an analyticalmapping gel all the visible labeling was contained within $alpha$ V8-10.However, scintillation counting of the material contained withinthese two $alpha$ -subunit fragments, isolated from preparative scalelabelings, indicated that ~70% of ³H cpm was incorporated in $alpha$ V8-10 and 30% was in $alpha$ V8-20. The relativeincorporation of [³H]promegestone into $alpha$ V8-10 was similar for labelings carried outin the absence (74%) and in the presence (70%) of 200 µMcarbamylcholine.

Identification of the Sites of [³H]Promegestone Incorporation in the M4 Segments of the $alpha$ , $beta$ , and $gamma$ AChR Subunits. The M4 segments from AChRs labeled with [³H]promegestone in the presence of 200 µM carbamylcholine were isolated from trypticdigests of either the intact subunit ( $beta$ , $gamma$ , ~250 µg) or $alpha$ V8-10(~125 µg). When the tryptic digest of $alpha$ -V8-10 was purified byreverse-phase HPLC, ³H counts eluted in a peak centered at ~82% solvent B (Fig. 5A)along with the peak of 1-AP fluorescence (data not shown). Amino-terminalsequence analysis (Fig. 6A) of the pool of HPLC fractions 31-35revealed the presence of a primary sequence beginning at $alpha$ Tyr-401(initial yield, 129 pmol) present at 15-fold higher level thana secondary sequence that began at $alpha$ Ser-388. In the pattern of³H release shown in Fig. 6A, there were 620 cpm released in thefirst cycle, equivalent to 1.5% of loaded cpm and similar in magnitudeto the 1.3% of ³H cpm washed off the filter by acid treatment before the firstcycle of Edman degradation (data not shown). The progressivelydeclining ³H release seen in the first 4 cycles of Edman degradation waslikely to result either from release of peptide poorly adsorbedon the glass support or chemical instability of some incorporated³H. A stable baseline of ³H release was achieved by cycle 5, and, in addition to the prominent³H release in cycle 12, there was also clear, but lower level,release in cycles 8 and 18. Comparison of the pattern of releasewith the corresponding amino acids in the primary sequence indicatesthat the labeled amino acids include His-408 (0.7 cpm/pmol), Cys-412(9 cpm/pmol), and Cys-418 (2 cpm/pmol). These same three residueswere found to have incorporated [³H]promegestone when the M4 region was isolated from membraneslabeled in the absence of agonist (data not shown). Cys-412 isthe residue in $alpha$ M4 at the lipid interface that is labeled mostefficiently by the hydrophobic probes 3-(trifluoromethyl)-3(m-[¹²⁵I]iodophenyl)diazirine[¹²⁵I](TID) and [³H]diazofluorene; Cys-418 is labeled by both probes, and His-408is labeled only by [³H]diazofluorene (Blanton and Cohen, 1994; Blanton et al., 1998).

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Fig. 5. Reverse-phase HPLC purification of proteolytic fragments of [³H]promegestone-labeled AChR subunits containing M4 and M2 hydrophobic segments. AChR subunits were isolated from AChR-rich membranes (12 mg protein) labeled with [³H]promegestone in the presence of carbamylcholine and in the absence ( $bullet$ ) or presence ( $open circle$ ) of 60 µM phencyclidine. Proteolytic digests of subunits were purified by SDS-PAGE and reverse-phase HPLC as described under Materials and Methods. A, trypsin digests of $alpha$ V8-10 (Asn-339-Gly-437) were purified directly; B, purification of a 10-kDa band ( $alpha$ -K-10K) isolated by tricine-SDS-PAGE from Endoproteinase-Lys C digests of $alpha$ V8-20 (Ser-173-Glu-338). Trypsin digests of $beta$ -, $gamma$ -, and $delta$ -subunits were fractionated by tricine-SDS-PAGE to isolate from $beta$ -subunit 5 kDa ( $beta$ -T-5K) and 7-kDa ( $beta$ -T-7K) bands, from $gamma$ -subunit a 5-kDa band ( $gamma$ -T-5K), and from $delta$ -subunit a 5 kDa band ( $delta$ -T-5K). C and D, reversed-phase HPLC purification of $beta$ -T-5K and $beta$ -T-7K, respectively. E and F, purification of $gamma$ -T-5K and $delta$ -T-5K respectively.

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Fig. 6. Radioactivity and mass release upon amino-terminal sequence analysis of the M4 region of the $alpha$ -, $beta$ -, and $gamma$ -subunits. For AChRs labeled with [³H]promegestone in the presence of agonist, the M4 regions of the $alpha$ - $beta$ -, and $gamma$ -subunits were isolated from tryptic digests of $alpha$ V8-10 (Asn-339-Gly-437) and intact $beta$ - and $gamma$ -subunits. M4 containing proteolytic fragments $alpha$ -T-4K, $beta$ -T-4K, and $gamma$ -T-5K were purified by reverse-phase HPLC (Fig. 5, A, C, and E) and the fractions containing the peaks of ³H were pooled (fractions 28-32, 28-32, and 31-35, respectively) and sequenced. For each sample 60% of each cycle of Edman degradation was analyzed for released ³H ( $bullet$ ) and 30% for PTH-amino acids (

) with the dashed lines corresponding to the exponential decay fit of the amount of detected PTH-amino acids for the peptides containing M4. The amino acid sequence of the sequenced peptide containing the M4 region is shown above each panel. A, ³H release from $alpha$ -T-4K [I_o = 129 pmol; r = 89%; 44,000 cpm loaded/5800 remaining on filter]. B, ³H release from $beta$ -T-4K [I_o = 129 pmol; r = 95%; 7700 cpm loaded/2100 remaining on filter]. C, ³H release from $gamma$ -T-5K [I_o = 116 pmol; r = 88%; 7800 cpm loaded/1950 remaining on filter].

Tryptic digestion of the intact $beta$ -subunit produced on a tricine SDS-PAGE gel a fluorescent and radioactive band migratingwith an apparent molecular mass of 4 kDa ( $beta$ T-4K), known to containthe $beta$ M4 region (Blanton et al., 1998

), which was further purifiedby HPLC (Fig. 5C). Amino-terminal sequence analysis (Fig. 6B)of the pooled fractions (28-32) revealed the presence of a primarysequence beginning at $beta$ Asp-427 (129 pmol) as well as a secondarysequence beginning at the amino terminus of $beta$ M1 ( $beta$ Lys-216, 40pmol). As with $alpha$ M4, recovery of ³H in the acid prewash and in cycle 1 were each equal to 1% of³H cpm loaded. A stable baseline of ³H release was seen in cycles 5-14, followed by prominent ³H release in cycle 15 with additional release in cycle 21. A comparisonof the pattern of ³H release with the corresponding amino acids identified in thepeptide beginning at $beta$ Asp-427 indicate that Tyr-441 (0.5 cpm/pmol)and Cys-447 (0.2 cpm/pmol) are labeled, the same residues in $beta$ M4that were labeled nonspecifically by [¹²⁵I]TID (Blanton and Cohen, 1994

) and by [³H]diazofluorene (Blanton et al., 1998

When the tryptic digest of the intact [³H]promegestone-labeled $gamma$ -subunit was resolved on a tricine SDS-PAGE gel, a band offluorescence and ³H migrated with an apparent molecular mass of 5 kDa ( $gamma$ T-5K). Materialeluted from the $gamma$ T-5K band was further purified by reverse-phaseHPLC (Fig. 5E) with peaks of both 1-AP fluorescence and ³H counts eluting at 75% solvent B. Amino-terminal sequence analysisof the pool of fractions 28-32 revealed the presence of a primarysequence (Fig. 6C) beginning at $gamma$ Val-446 and extending through $gamma$ M4 (116 pmol) that was present at 10-fold higher level than secondarysequences that began at $gamma$ Lys-218 (amino terminus of $gamma$ M1, 10 pmol)and at $gamma$ Val-273 (amino terminus of $gamma$ M3, 12 pmol). The ³H released in cycles 6 and 8 indicated that [³H]promegestone was incorporated into $gamma$ Cys-451 (2 cpm/pmol)and $gamma$ Trp-453 (~0.4 cpm/pmol) within $gamma$ -M4. Incorporation into $gamma$ Cys-451was also evident in the amino-terminal sequence analysis of $gamma$ T-5Kisolated from membranes labeled in the absence of carbamylcholine(data notshown).

Radiochemical Sequence Analysis of M2 Segments of AChR $alpha$ -, $beta$ -, and $delta$ -subunits. Subunit proteolytic fragments beginning at the amino termini of the M2 segments of AChR $alpha$ -, $beta$ -, and $delta$ -subunits were isolatedfrom AChRs labeled with [³H]promegestone in the presence of carbamylcholine. For $alpha$ -subunit,an EKC digest of $alpha$ V8-20 (~280 µg) was fractionated by tricineSDS-PAGE, and an ~10- kDa fragment ( $alpha$ -K-10K), previously shownto contain the M2-M3 region (Pedersen et al., 1992), was isolatedfrom the gel (see Materials and Methods). When the material elutedfrom the $alpha$ -K-10K fragment was further purified by reversed-phaseHPLC (Fig. 5B), the majority of ³H counts eluted in a peak centered at 84% solvent B. HPLC fractions32-35 were pooled and sequenced (Fig. 7A). The primary sequence,which began at $alpha$ Met-243, the amino terminus of the M2 region (85pmol), was present at 10-fold higher level than a secondary sequencebeginning at the amino terminus of $alpha$ M3 ( $alpha$ Tyr-277, 7 pmol). Nosignificant ³H release above background was observed in any of the 21 sequencingcycles.

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Fig. 7. Radioactivity and mass release upon amino-terminal sequence analysis of the M2 regions of $alpha$ -, $beta$ -, and $delta$ -subunits. For AChRs labeled with [³H]promegestone in the presence of agonist, proteolytic fragments beginning at the amino termini of the M2 regions of the $alpha$ - $beta$ -, and $delta$ -subunits were isolated from either an EKC digest of $alpha$ V8-20 (Ser-173-Glu-338) or tryptic digests of intact $beta$ - and $delta$ -subunits. The $alpha$ -K-10K, $beta$ -T-7K, and $delta$ T-5K fragments containing M2 segments isolated by tricine SDS-PAGE were further purified by reverse-phase HPLC (Figs. 5B, D, and F, respectively) and the fractions containing the peaks of ³H were pooled (fractions 32-35, 30-34, and 30-33, respectively) and sequenced. For each sample 60% of each cycle of Edman degradation was analyzed for released ³H( $bullet$ ) and 30% for PTH-amino acids (

) with the dashed lines corresponding to the exponential decay fit of the amount of detected PTH-amino acids for the each of the M2 containing peptides. The amino acid sequence of the sequenced peptides containing the M2 region is shown above each panel. A, ³H release from $alpha$ -K-10K [I_o = 85 pmol; r = 85.8%; 6200 cpm loaded/2000 cpm remaining on filter]. B, ³H release from $beta$ -T-7K [I_o = 86 pmol; r = 90%; 3,600 cpm loaded/1000 cpm remaining on filter]. C, ³H release from $delta$ -T-5K [I_o = 90 pmol; r = 91%; 7,700 cpm loaded/1,200 cpm remaining on filter].

To identify potential sites of [³H]promegestone photoincorporation in the M2 regions of $beta$ - and $delta$ -subunits, trypsin digestsof the subunits (~250 µg) were first fractionated by tricine SDS-PAGE.For the $beta$ -subunit, a 7-kDa fragment ( $beta$ -T-7K), known to containboth the M2 and M3 region, was identified as a band of weak fluorescencebetween two strongly fluorescent bands of 10 and 5.5 kDa whenthe tricine SDS-PAGE gel was illuminated at 365 nm (data not shown).The material eluted from the $beta$ -T-7K band was further purifiedby reverse-phase HPLC (Fig. 5D), with the majority of ³H counts eluting in a peak centered at 80% solvent B. Sequenceanalysis of the pool of HPLC fractions 30 to 34 (Fig. 7B) revealedthe presence of a peptide beginning at $beta$ -Met-249, the amino terminusof the $beta$ M2 (86 pmol), along with secondary sequences beginningat the amino termini of $beta$ M1 ( $beta$ Lys-216, 15 pmol) and $beta$ M4 ( $beta$ Asp-427,10 pmol). No ³H release above background was seen in any of the 21 sequencingcycles. Similarly, no [³H]promegestone incorporation was evident in the ³H release profile obtained upon sequencing the $beta$ -T-7K fragmentlabeled in the absence of agonist (data notshown).

When the trypsin digest of [³H]promegestone-labeled $delta$ -subunit was resolved by tricine SDS-PAGE, a 5-kDa fragment ( $delta$ -T-5K),known to contain the M2-M3 region, was identified by the use ofprestained molecular weight standards and by the fluorescenceassociated with 1-azidopyrene incorporation into M3. When thematerial eluted from the $delta$ -T-5K band was further purified by reverse-phaseHPLC (Fig. 5F), the majority of ³H counts eluted in a peak centered at 82% solvent B. When HPLCfractions 30 to 33 were pooled and sequenced (Fig. 7C), a primarysequence was identified beginning at $delta$ Met-257, the amino terminusof the $delta$ M2 (90 pmol), along with a secondary sequence beginningat the amino terminus of $delta$ M4 ( $delta$ Asn-447, 7 pmol). No clear ³H release above background wasdetected.

	Discussion

Top Summary Introduction Materials and methods Results Discussion References

We have shown that the synthetic progestin, promegestone, is a NCA of the Torpedo AChR. Promegestone reversibly inhibits ACh-elicitedcurrents for Torpedo AChRs expressed in Xenopus oocytes with thesame potency as progesterone. Because promegestone concentrationsup to 100 µM increase the [³H]ACh equilibrium binding affinity to AChR-rich membranes, promegestoneis a desensitizing NCA. Interestingly, although it is only a weakinhibitor (IC₅₀ ~ 100 µM) of [³H]HTX binding to AChRs in the desensitized state, it is a potentinhibitor (IC₅₀ = 9 µM) of [³H]PCP binding. Because binding of HTX and PCP appear formallycompetitive (Heidmann et al., 1983; White et al., 1991), thisresult appears at first surprising. However, studies with TID,an uncharged, photoactivatable NCA, provide clear evidence thatthe binding sites for PCP and HTX can be differentiated (Whiteet al., 1991; White and Cohen, 1992): TID is a potent, competitiveinhibitor of [³H]PCP binding to AChRs in the desensitized state, whereas it isan allosteric inhibitor of [³H]HTX binding. Although HTX and PCP are presumed to bind withinthe lumen of the ion channel, their site(s) of high-affinity bindinghave not been mapped directly. The high-affinity binding sitefor [³H]tetracaine in the AChR in the resting state has been shown bydirect photoaffinity labeling to overlap with the [¹²⁵I]TID site in the M2 ion channel domain (White and Cohen, 1992;Gallagher and Cohen, 1994; Gallagher, 1996). Although promegestoneat high concentrations (IC₅₀ ~75 µM) inhibits [³H]tetracaine binding, that inhibition probably occurs becausepromegestone stabilizes the AChR desensitized state that binds[³H]tetracaine only weakly. Although promegestone clearly can bea potent inhibitor of NCA binding, the results of the radioligandassays provide no clear indication of the nature of the promegestonebinding site(s) in theAChR.

When [³H]promegestone was photoincorporated into AChR-rich membranes, its incorporation was readily detected in residues inthe M4 segments of the $alpha$ -, $beta$ -, and $gamma$ -subunits that previous workhas shown are exposed to lipid (Fig. 8; Blanton and Cohen, 1994;Blanton et al., 1998). In contrast, no incorporation was detectedin the sequence analysis of the $alpha$ -, $beta$ -, or $delta$ -M2 segments isolatedfrom AChRs labeled in either the absence or presence of agonist.The simplest interpretation of the photolabeling data is that,consistent with its lipophilicity, the steroid promegestone bindsto and interacts with the AChR at the lipid-protein interface.The inability of increasing doses of progesterone to affect thephotoincorporation of [³H]promegestone, at least at the subunit level, is also consistentwith "nonspecific" binding at the lipid-protein interface. Althoughpromegestone interaction at the AChR-lipid protein interface doesnot meet the classical criteria for a specific drug-receptor bindingsite, this does not preclude this promegestone-AChR interactionfrom affecting AChR function. Additional studies are requiredto determine whether promegestone interactions at the AChR-lipidinterface result in the observed inhibition of NCA binding orof ACh-induced ion currents. Also, additional studies are requiredto determine whether promegestone is interacting at sites on theAChR surface normally occupied by cholesterol, which is presentat 15% (w/w) in the AChR-rich membranes and at an effective concentrationof 1 mM. There is strong evidence that cholesterol interacts directlywith AChRs and that neutral lipids are required to maintain theAChR in a state responsive to agonist (Rankin et al., 1997 andreferences therein). Inhibition by promegestone (or progesterone)might occur because it displaces cholesterol from a functionallyimportant site.

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Fig. 8. Corey-Pauling-Koltun models of the $alpha$ -M4 helix. The amino acids labeled by [³H]promegestone (His-408, Cys-412, and Cys-418) are also labeled by the hydrophobic probe [³H]diazofluorene (as is Met-415 (Blanton et al., 1998

)) and by [¹²⁵I]TID [which also reacts with Thr-422 and Val-425 (Blanton and Cohen, 1994

)].

Although our studies have found no evidence that [³H]promegestone binds within the M2 ion channel domain, it remains possiblethat it binds within the channel but is incapable of photoincorporatinginto the predominantly aliphatic residues contained within eachof the M2 segments. Promegestone photoincorporation proceeds througha "triplet state" biradical, which should readily incorporateinto C-H bonds (Benisek, 1977). However, although very limited,the residues that have been shown to react with [³H]promegestone [Met-759 and Met-909 (human progestin receptor);Met-622 and Cys-754 (rat glucocorticoid receptor) (Stromstedtet al., 1990); His-408, Cys-412, and Cys-418 ( $alpha$ M4); Tyr-441, Cys-447( $beta$ M4); and Cys-451, Trp-453 ( $gamma$ M4) AChR, this report] do not includeany aliphatic residues. In addition, it is also possible thatthere is an extracellular binding site for promegestone, but thatthe efficiency of [³H]promegestone photoincorporation into this region was too lowfor us to detect. Finally, it also remains to be determined whether[³H]promegestone is photoincorporated in the M1 or M3 hydrophobicsegments (or in the AChR extracellular domain) because the subunitfragmentation strategies used in this study were chosen specificallyto identify possible sites of incorporation in M2 and M4segments.

By interacting with residues situated at the lipid-protein interface of the AChR, promegestone could allosterically alterthe structure of the ion channel, effecting both ion conductanceand binding of NCAs. Several recent reports provide support forthis conclusion. Mutations at lipid-exposed residues in the M4segment dramatically affect open channel lifetimes (Bouzat etal., 1994, 1998; Lee et al., 1994; Lasalde et al., 1996), anda mutation within the M2 ion channel domain that increases channellifetime also increases hydrocortisone potency (Bouzat and Barrantes,1996).

Finally, progesterone inhibits AChR activity but potentiates GABA_A receptor currents in the same concentration range (EC₅₀= 26 µM, Wu et al., 1990). Given the emerging evidence of structuralhomology between these two receptors (reviewed in Sigel and Buhr,1997), this raises the possibility that steroids may differentiallymodulate the activities of these two receptors (as well as othermembers of the AChR family) by interacting with residues at acommon site, potentially at the lipid-protein interface. On theother hand the ACh and GABA_A receptors have different steroidstructure-activity relationships (Wu et al., 1990). Although thesedifferences may simply reflect the different modulatory affectsprogesterone and other steroids have on these two receptors, itmay also indicate separate steroid binding domains. In this respect,future studies will be aimed at identifying the site(s) of [³H]promegestone incorporation in GABA_A receptorsubunits.

	Acknowledgements

We thank Martin Gallagher for helpful comments andsuggestions.

	Footnotes

Received August 24, 1998; Accepted October 30, 1998

¹ Current address: Department of Pharmacology, Texas Tech University of Health Sciences Center, Lubbock, TX79430.

² Current address: Millenium Pharmaceuticals, Cambridge, MA02139.

³ Current address: Protein Chemistry Laboratory, Department of Chemistry, Texas A&M University, College Station TX77842.

This research was supported in part by U.S. Public Health Service Grant GM 15904 and by an award in Structural Neurobiologyfrom the KeckFoundation.

Send reprint requests to: Dr. Jonathan B. Cohen. Department of Neurobiology, Harvard Medical School, 220 Longwood Ave., Boston MA 02115. E-mail: jonathan-cohen{at}hms.harvard.edu

	Abbreviations

ACh, acetylcholine; AChR, nicotinic acetylcholine receptor; Promegestone, 17,21-dimethyl-19-nor-pregn-4,9-diene-3,20-dione; 1-AP, 1-azidopyrene; PAGE, polyacrylamide gel electrophoresis; HPLC, high-performance liquid chromatography; NCA, noncompetitive antagonist; HTX, d,l-perhydrohistrionicotoxin; [¹²⁵I]TID, 3-(trifluoromethyl)-3(m-[¹²⁵I]iodophenyl)diazirine; EKC, endoproteinase Lys-C; PCP, phencyclidine; PTH, phenylthiohydantoin; TPS, Torpedo physiological saline (250 mM NaCl, 3 mM CaCl₂, 2 mM MgCl₂, 5 mM sodium phosphate, pH 7.0); T, total acrylamide concentration; C, bis-acrylamide cross-linker concentration relative to total acrylamide concentration; GABA AChR, $gamma$ -aminobutyric acid; $alpha$ V8-20, 20-kDa V8 protease fragment of the AChR $alpha$ -subunit; $alpha$ V8-10, 10-kDa V8 protease fragment of the $alpha$ -subunit.

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