Identification of Amino Acids of the Torpedo Nicotinic Acetylcholine Receptor Contributing to the Binding Site for the Noncompetitive Antagonist [3H]Tetracaine

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Vol. 56, Issue 2, 300-307, August 1999

Identification of Amino Acids of the Torpedo Nicotinic Acetylcholine Receptor Contributing to the Binding Site for the Noncompetitive Antagonist [³H]Tetracaine

Martin J. Gallagher¹ and Jonathan B. Cohen

Department of Neurobiology, Harvard Medical School, Boston, Massachusetts

	Summary

Top Summary Introduction Experimental Procedures Results Discussion References

[³H]Tetracaine is a noncompetitive antagonist of the Torpedo nicotinic acetylcholine receptor (nAChR) that binds with highaffinity in the absence of cholinergic agonist (K_eq = 0.5 µM)and weakly (K_eq = 30 µM) in the presence of agonist (i.e., tonAChR in the desensitized state). In the absence of agonist, irradiationat 302 nm of nAChR-rich membranes equilibrated with [³H]tetracaine results in specific photoincorporation of [³H]tetracaine into each nAChR subunit. In this report, we identifythe amino acids of each nAChR subunit specifically photolabeledby [³H]tetracaine that contribute to the high-affinity binding site.Subunits isolated from nAChR-rich membranes photolabeled with[³H]tetracaine were subjected to enzymatic digestion, and peptidescontaining ³H were purified by SDS-polyacrylamide gel electrophoresis followedby reversed phase HPLC. N-terminal sequence analysis of the isolatedpeptides demonstrated that [³H]tetracaine specifically labeled two sets of homologous hydrophobicresidues ( $alpha$ Leu²⁵¹, $beta$ Leu²⁵⁷, $gamma$ Leu²⁶⁰, and $delta$ Leu²⁶⁵; $alpha$ Val²⁵⁵ and $delta$ Val²⁶⁹) as well as $alpha$ Ile²⁴⁷ and $delta$ Ala²⁶⁸ within the M2 hydrophobic segments of each subunit. The labelingof these residues establishes that the high-affinity [³H]tetracaine-binding site is located within the lumen of the closedion channel and provides a definition of the surface of the M2helices facing the channellumen.

	Introduction

Top Summary Introduction Experimental Procedures Results Discussion References

The nicotinic acetylcholine receptor (nAChR) isolated from the electric organ of the marine ray Torpedo is the best characterizedligand-gated ion channel (for reviews, see Karlin and Akabas,1995; Hucho et al., 1996). The nAChR is composed of four homologoussubunits in the stoichiometry $alpha$ ₂ $beta$ $gamma$ $delta$ , which electron microscopicstudies show are arranged pseudosymmetrically about a centralaxis that is the ion channel (Unwin, 1993). The M2 hydrophobicsegments from each subunit line the lumen of the ion channel (Huchoet al., 1986; Imoto et al., 1988, 1991; Charnet et al., 1990;Revah et al., 1990) and undergo a conformational change when thenAChR binds agonist (White and Cohen, 1992; Akabas et al., 1994;Unwin, 1995). Within the M2 domain, a conserved leucine ( $alpha$ Leu²⁵¹ and the homologous position in the other subunits) appears tobe important for the gating of the ion channel. Cryoelectron microscopyreveals an agonist-dependent rotation of a kink in the M2 helicesnear the predicted position of these leucines (Unwin, 1995), referredto as position 9 with reference to the conserved Lys at the N-terminalend of each M2 segment, and site-directed mutagenesis demonstratesthat this position is an important determinant of the equilibriumbetween closed and open channel states (Filatov and White, 1995;Labarca et al., 1995). However, it is unclear whether this ringof leucines forms the permeability barrier in the closed channelbecause cysteine mutants below position 9 are accessible to water-solublesulfhydryl reagents in the absence of agonist (Akabas et al.,1994; Pascual and Karlin, 1998).

Noncompetitive antagonists (NCAs), which are compounds that block the permeability response without preventing the bindingof agonist, have also been used to characterize the structureof the ion channel pore. For nAChR in the desensitized state,[³H]chlorpromazine is photoincorporated into residues at position6 of each subunit's M2 segment as well as into position 2 in $beta$ M2and 9 in $beta$ M2 and $gamma$ M2 (Giraudat et al., 1986, 1987, 1989; Revahet al., 1990). The labeling of these residues establishes that[³H]chlorpromazine's binding site is within the lumen of the ionchannel toward the cytoplasmic end of the pore and helps to identifythe pore-lining faces of the M2 segments. In contrast, in thedesensitized nAChR, the NCA [³H]meproadifen mustard reacts specifically with $alpha$ Glu²⁶² at position 20 at the extracellular end of the pore (Pedersenet al., 1992).

Unlike chlorpromazine and meproadifen, the uncharged NCA 3-(trifluoromethyl)-3-(M-[¹²⁵I]iodophenyl)diazirine ([¹²⁵I]TID) binds with similar affinity to both the resting and desensitizedstates (White et al., 1991) and therefore is a useful probe ofthe channel in the absence as well as the presence of agonist.In the absence of agonist, [¹²⁵I]TID specifically photoincorporates into M2 residues at positions9 and 13, whereas in the desensitized state, it labels residuesdeeper in the pore (positions 2 and 6) as well as the residuesat 9 and 13 (White and Cohen, 1992). This study directly demonstrateda structural change in the pore between resting (closed channel)and desensitized states and suggested that the aliphatic residuesat position 9 from each subunit associate in the lumen to providethe permeability barrier in the closedchannel.

To better characterize the structure of the ion channel in the closed state, we identified the binding site of the NCA [³H]tetracaine, in the absence of agonist. Unlike the NCAs usedin previous photoaffinity labeling studies, tetracaine binds tothe nAChR with high affinity in the absence of agonist (K_eq =0.3 µM) and with 100-fold lower affinity in the presence of agonist(Blanchard et al., 1979). Middleton et al. (1999) establishedthat [³H]tetracaine binds with a 1:1 stochiometry to the nAChR and thatultraviolet irradiation at 302 nm resulted in specific [³H]tetracaine photoincorporation into each subunit. We report herethe identification of the individual amino acids of the nAChRthat photoincorporated [³H]tetracaine. These data show that the high-affinity [³H]tetracaine-binding site is located within the lumen of the ionchannel. The labeled amino acids define the surface of the M2helix extending one helical turn above and below position 9 fromeach subunit that lines the lumen of the channel in the absenceofagonist.

	Experimental Procedures

Top Summary Introduction Experimental Procedures Results Discussion References

Materials. [³H]Tetracaine was prepared at New England Nuclear Research Products (Boston, MA) by palladium/charcoal-catalyzed reductionin 3,5-dibromotetracaine with carrier-free ³H₂ gas. [³H]Tetracaine was purified from the tritium reduction productsby silica thin-layer chromatography (5:4:1 cyclohexane/chloroform/diethylamine;R_f = 0.17). The purity (>90%) and specific activity (48 Ci/mmol)were determined by silica HPLC (Hibar Si-60 10 µm, 200:1 acetonitrile/diethylamineisocratic elution). nAChR-rich membranes were isolated from electricorgans of Torpedo californica (Marinus Inc., Westchester, CA)as described previously (Pedersen et al., 1992) and stored at $-$ 80°C in 38% sucrose. Endoproteinase Lys-C (EKC) was obtainedfrom Boehringer-Mannheim (Indianapolis, IN). l-1-Tosylamido-2-phenylethylchloromethylketone-treatedtrypsin was obtained from Worthington Biochemical (Freehold, NJ).Staphylococcus aureus glutamyl endopeptidase (V8 protease) waspurchased from ICN Biomedical Inc. (Costa Mesa, CA). Oxidizedglutathione and tricine were from Sigma Chemical Co. (St. Louis,MO). o-Phthalaldehyde (OPA), 10% Genapol C-100, and trifluoroaceticacid (TFA) were obtained from Pierce Chemical Co. (Rockford, IL).1-Azidopyrene (1-AP) was purchased from Molecular Probes (Eugene,OR). dl-perhydrohistrionicotoxin (HTX) was kindly provided byDr. Y. Kishi (Harvard University, Cambridge,MA).

Photolabeling of nAChR-Rich Membranes with [³H]Tetracaine and Isolation of Labeled nAChR Subunits. Freshly thawed suspensions of nAChR-rich membranes (10-14 mg protein) were diluted 1:2 in Torpedo physiological saline (TPS;250 mM NaCl, 5 mM KCl, 3 mM CaCl₂, 2 mM MgCl₂, 5 mM NaPi, pH 7.0)and pelleted (15,000g) for 30 min at 4°C. The membrane pelletswere then resuspended at ~2 mg protein/ml in TPS supplementedwith 50 mM oxidized glutathione (Middleton et al., 1999). [³H]Tetracaine was then added at a final concentration of 5 µM,as well as 30 µM HTX for the samples used to define nonspecificphotolabeling. The suspensions (2.5-ml volumes) were incubatedfor 30 min at room temperature with stirring in covered glasscrystallization dishes (3 cm diameter) that were flushed withAr(g) for 15 min immediately before photolysis. The samples, containedin a water bath that served to keep the sample temperature below25°C, were then irradiated at 302 nm for 30 min with stirring.The lamp (Spectroline model EB-280C; Spectronics, Westbury, NY)was at a distance of 12 cm and had an intensity of ~1000 µW/cm² (as measured by a Spectroline DIX 300 digital radiometer). Afterirradiation, samples were pelleted, resuspended to ~2 mg/ml inTPS, and photolabeled as described (Blanton and Cohen, 1994) withthe fluorescent, hydrophobic probe 1-AP. The membranes were thenpelleted and resuspended in electrophoresis sample loading bufferfor isolation of nAChR subunits by SDS-polyacrylamide gel electrophoresis(PAGE). Labeling with 1-AP was used to facilitate the initialidentification and isolation of nAChR subunits and for the subsequentisolation of their hydrophobic fragments (Blanton and Cohen, 1994).

SDS-PAGE. nAChR subunits were resolved by SDS-PAGE using the Laemmli buffer system (Laemmli, 1970) with 1.5-mm-thick, 8% acrylamideslab gels containing 0.32% bisacrylamide. After electrophoresis,the unstained gels were illuminated on a 365-nm UV light box,and the nAChR subunits were visualized by 1-AP fluorescence. ThenAChR $beta$ , $gamma$ , and $delta$ subunits were excised from the gel and elutedin 10 ml of elution buffer (0.1 M NH₄HCO₃/0.1% SDS). The bandcontaining the nAChR $alpha$ subunit was excised from the gel and placedon top of the stacking portion of a 15% mapping gel for in geldigestion with S. aureus V8 protease (Pedersen et al., 1986).The $alpha$ subunit V8 protease fragments of 20 kDa ( $alpha$ V8-20, $alpha$ Ser¹⁷³- $alpha$ Glu³³⁸) and 10 kDa ( $alpha$ V8-10; $alpha$ Asn³³⁹- $alpha$ Gly⁴³⁷) were visualized by 1-AP fluorescence (Blanton and Cohen, 1994),excised from the gel, and eluted as above. After 4 days of elution,subunits (or subunit fragments) were concentrated with Centriprep-30(or -10) Microconcentrators (Amicon, Beverly, MA) to approximately400 µl, and excess SDS was removed by acetone precipitation at $-$ 20°C. The precipitates were resuspended in 15 mM Tris (pH 8.1)/0.1%SDS at 0.4 mg protein/ml. Protein concentration was measured usinga bicinchoninic acid-based protein assay (Micro BCA Protein Assay,Pierce Chemical Co.), and [³H]tetracaine incorporation was determined by scintillationcounting.

Purification of Proteolytic Digests of [³H]Tetracaine/1-AP -Labeled nAChR Subunits. nAChR $alpha$ V8-20 and $delta$ subunit at 0.4 to 0.6 mg protein/ml in 15 mM Tris (pH 8.1)/0.1% SDS were digested with 4 U/ml EKC or with1:1 (w/w) S. aureus V8 protease at ambient temperature. The $beta$ and $gamma$ subunits were digested with trypsin (25% w/w) at ambienttemperature in 15 mM Tris (pH 8.1)/0.1% SDS supplemented with0.5% Genapol C-100. The digestion times are indicated in the figurelegends. The proteolytic digests were fractionated by TricineSDS-PAGE as described (Schagger and von Jagow, 1987; Blanton andCohen, 1994). To identify regions of the gel that contained specificallylabeled fragments, an aliquot (5 µg) of each digest was run ina separate lane of the 1.5-mm-thick preparative gel, and anotherlane contained prestained molecular weight standards (Life Technologies,Gaithersburg, MD): insulin B (2300) and A (3400) chains, bovinetrypsin inhibitor (6200), lysozyme (14,300), $alpha$ -lactoglobulin (18,400),carbonic anhydrase (29,000), and ovalbumin (43,000). The analyticallanes were cut into 3-mm slices and placed into scintillationtubes. After dissolution of the acrylamide in 800 µl of 30% H₂O₂heated to 80°C for more than 1 h, the ³H in each sample was determined by scintillation counting in Dimiscint(National Diagnostics, Atlanta,GA).

Bands of the preparative gel were excised based on the observed distribution of ³H in the analytical lanes in relation to molecular weight markers,as well as the visualization of 1-AP fluorescence. The excisedbands were diced and passively eluted into 4 ml of elution buffer,and each eluate was concentrated using Centricon-3 Microconcentrators(Amicon).

[³H]Tetracaine/1-AP-labeled fragments were further purified by reversed phase HPLC on a Brownlee C4 Aquapore column (100 ×2.1 mm, 7-µm particle size) as described previously (Pedersenet al., 1992

). Solvent A consisted of 0.08% TFA in water, andsolvent B consisted of 60% acetonitrile/40% 2-propanol/0.05% TFA.The fragments were eluted at 0.2 ml/min with a linear gradientfrom 25 to 100% B in 80 min. The elution of peptides was monitoredby the absorbance at 210 nm and by fluorescence emission at 432nm (355-nm excitation), corresponding to the excitation and emissionmaxima of 1-AP. Fractions (0.5 ml) were collected in plastic tubes,and the distribution of ³H was determined by scintillation counting of 5% of eachfraction.

Sequence Analysis. N-terminal sequence analysis was performed on an ABI model 477A (Applied Biosystems, Foster City, CA) protein sequencer withgas phase cycles. HPLC fractions that contained specifically labeledmaterial were pooled and dried by vacuum centrifugation. The driedsamples were resuspended in 25 µl of 100 mM NH₄HCO₃/0.05% SDSand then loaded onto chemically modified glass-fiber disks (Beckman,Palo Alto, CA) that were used rather than polybrene-treated filtersto improve the sequencing yields of hydrophobic peptides (Pedersenet al., 1992). Before beginning the Edman degradation cycles,the sample in the sequencer cartridge was exposed to TFA vaporfor 4 min to fix the sample to the filter, and then SDS was removedby a 5-min wash of the filter with ethyl acetate. Approximately30% of each degradation cycle was injected into the on-line ABImodel 120 A amino acid analyzer to determine the identity of thereleased phenylthiohydantoin (PTH)-amino acid derivatives, and60% was delivered to a fraction collector for scintillation counting.During the sequencing of samples containing $beta$ -M1, sequencing ofcontaminating peptides was blocked by treatment of the sampleon the filter with OPA. OPA reacts with primary, but not secondaryamines, and can be used to block Edman degradation of any peptidenot containing an N-terminal proline (Brauer et al., 1984). OPAtreatment was carried out as described previously (Middleton andCohen, 1991). The Applied Biosystem model 610A Data Analysis ProgramVersion 1.2.1 was used to analyze the sequencer chromatogramsand calculate the background-subtracted amount of PTH-amino acidpresent in each cycle of Edman degradation. Initial peptide mass(I₀) and repetitive yield (R) were determined by nonlinear least-squaresregression (Sigma Plot) of the function I = I₀ × Rⁿ, where I is the observed mass of PTH-derivative at cycle n. Thebackground-subtracted mass of the PTH derivatives of Ser, Cys,Arg, His, and Trp were excluded from the fits because of knownproblems of measuring their massyields.

	Results

Top Summary Introduction Experimental Procedures Results Discussion References

To identify the amino acids of the nAChR that specifically photoincorporated [³H]tetracaine, we labeled nAChR-rich membranes (5 mg protein, 2mg/ml) equilibrated with 5 µM [³H]tetracaine in both the absence and presence of 30 µM HTX. ThenAChR subunits were purified in good yield (typically 100-200µg). Then $beta$ , $gamma$ , and $delta$ subunit preparations each incorporated about1800 to 2000 ³H cpm/µg protein, with $beta$ subunit labeling ~75% specific (i.e.,inhibitable by HTX) and $gamma$ and $delta$ subunit labeling ~55 and ~70%specific. Although intact $alpha$ subunit was not routinely isolated,preparations of $alpha$ V8-20 incorporated ~2500 ³H cpm/µg with an 80% reduction for $alpha$ V8-20 isolated from nAChRslabeled with [³H]tetracaine in the presence of HTX. The levels of HTX-inhibitable³H incorporation in each subunit indicated specific incorporationof [³H]tetracaine in ~0.1% of subunits, a level somewhat lower thanthat seen in the analytical experiments of Middleton et al. (1999).

[³H]Tetracaine Photoincorporation in $delta$ Subunit. In initial experiments, we performed a series of analytical scale digests (5-µg aliquots of labeled $delta$ subunit) with EKC thatwere analyzed both by the ³H distribution after Tricine SDS-PAGE and by the profile of ³H release when the total digest was sequenced. Digestion conditionsthat resulted in a fragment (or fragments) releasing ³H after 9 and 13 cycles of Edman degradation were identified (notshown). The digest contained a single, specifically labeled fragmentof ~10 kDa, as shown in Figure 1A, the analytical lanes (5-µgaliquots) of a preparative scale digest of $delta$ subunits (~150 µgprotein) isolated from nAChRs labeled in the absence or presenceof HTX. The peak of ³H corresponded to a band of 1-AP fluorescence in the preparativelanes and a 5-mm strip containing the fluorescent band, as wellas sections below and above the fluorescent band, were excisedfrom each preparative lane, and the protein in them was eluted.The eluates from the fluorescent band (band C) and the band above(band D) contained the highest amounts of ³H, which when combined accounted for 38% of the eluted cpm. Thematerial eluted from these two sections was pooled and is referredto as $delta$ EKC-10.

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Fig. 1. Proteolytic mapping of [³H]tetracaine incorporation in nAChR $delta$ subunit with endoproteinase Lys-C (A-C) or S. aureus V8 protease (D). All panels display results from parallel photolabelings of nAChR-rich membranes with [³H]tetracaine in the absence (

) or presence ( $open circle$ ) of HTX. Solutions (0.4 mg/ml) of [³H]tetracaine-labeled $delta$ subunit were digested with EKC (3U/ml) for 5 days at ambient temperature and fractionated by Tricine SDS-PAGE with 5-µg aliquots ( $-$ HTX, 10,780 cpm; +HTX, 3050 cpm) electrophoresed in analytical lanes adjacent to the bulk digests. A, distribution of ³H in the analytical lanes is shown in relation to molecular weight markers (above) and the strips (A-F) excised from the preparative lanes. For the $-$ HTX sample, 543,300 cpm was loaded onto the preparative lane, with 14,640, 17,000, 66,560, 31,640, 11,520, and 7600 cpm recovered from strips A to F, respectively. The eluates from strips C and D were combined and designated as $delta$ EKC-10. B, reversed phase HPLC purification of $delta$ EKC-10 (5% of the HPLC fractions) were assayed for ³H. Specifically labeled material (66% of loaded cpm) eluted in a single peak (fractions 20-23). Fractions 21 and 22 were pooled for sequence analysis. C, ³H and mass release on N-terminal sequencing of $delta$ EKC-10 purified by reversed phase HPLC. The only sequence detected in either sample began at $delta$ Met²⁵⁷, the N terminus of $delta$ M2 (

, $-$ HTX, I₀ = 10 pmol, R = 94%, 10,000 cpm loaded/1800 cpm remained on the filter; +HTX, I₀ = 11 pmol, R = 94%). The sequence of the identified peptide is shown above. D, ³H release from N-terminal sequencing of $delta$ V8-3. Solutions of [³H]tetracaine-labeled $delta$ subunit (0.6 mg/ml) were digested with an equal weight of S. aureus V8 protease for 14 days at ambient temperature and then separated by Tricine SDS-PAGE (not shown). A 3-kDa specifically labeled fragment ( $delta$ V8-3) was excised, purified by reversed phase HPLC (not shown), and sequenced ( $-$ HTX, 13,700 cpm loaded/2300 cpm remained on the filter). As many as five different PTH derivatives were identified in each cycle of Edman degradation.

When $delta$ EKC-10 was further purified by reversed phase HPLC (Fig. 1B), about 66% of ³H loaded on the column eluted in a single peak of ³H centered at 65% organic that was associated with two peaks offluorescence. For $delta$ EKC-10 from nAChRs labeled with [³H]tetracaine in the presence of HTX, the ³H in that peak was reduced by >95% (Fig. 1B), whereas the peaksof fluorescence were similar in magnitude (not shown). Sequenceanalysis (Fig. 1C) of the pooled fractions (f21-22) from boththe specifically and nonspecifically labeled $delta$ EKC-10 fragmentsrevealed the presence of a single peptide starting at $delta$ -Met²⁵⁷ at the N terminus of M2 ( $-$ HTX, I₀ = 10 pmol; +HTX, 11 pmol).No other sequences were identifiable, with other PTH amino acidspresent at less than 5% the level of the primary sequence. Themolecular weight of this fragment and its labeling by 1-AP (Blantonand Cohen, 1994

) indicated that it must extend through the M3hydrophobic segment. The ³H release profile revealed clear peaks of ³H release in cycles 9, 12, and 13 that were reduced by more than90% for the sample labeled in the presence of HTX. The releaseof ³H in those cycles correspond to [³H]tetracaine reaction with $delta$ Leu²⁶⁵, $delta$ Ala²⁶⁸, and $delta$ Val²⁶⁹.

Although only one fragment beginning at the N terminus of $delta$ M2 was identified in the sequence analysis of $delta$ EKC-10, it was possiblethat the observed ³H release originated from a contaminating peptide present at levelsbelow detection (<0.5 pmol). Therefore, we used a second digestionstrategy to verify that the ³H release in cycles 9, 12, and 13 originated from $delta$ Leu²⁶⁵, $delta$ Ala²⁶⁸, and $delta$ Val²⁶⁹ and not from a contaminating peptide. Digestion with V8 proteasecould result in cleavage at $delta$ Glu²⁵⁵ and at $delta$ Glu²⁸⁰ at the N and C termini of $delta$ M2, which would generate a ~2.9-kDafragment. Following cleavage after $delta$ Glu²⁵⁵, ³H release would be expected in cycles 10, 13, and 14 of Edmandegradation.

Aliquots (75 µg) of labeled $delta$ subunits were digested with an equal weight of V8 protease for 14 days at room temperature.The digestion products were then purified by Tricine SDS-PAGE,with 5-µg aliquots from each sample loaded in analytical lanes.The ³H distribution in the analytical lanes showed a specifically labeledband at 3 kDa (not shown). This band, referred to as $delta$ V8-3, waseluted and purified by reversed phase HPLC (not shown). Sequenceanalysis revealed the presence of at least five different peptidesin $delta$ V8-3. However, in the ³H release profile, there was specific release of ³H in cycles 10, 13, and 14 (Fig. 1D), a result consistent withlabeling at $delta$ Leu²⁶⁵, $delta$ Ala²⁶⁸, and $delta$ Val²⁶⁹ after V8 protease cleavage at $delta$ Glu²⁵⁵. The observed molecular weight of this labeled peptide as wellas the ³H release pattern were as predicted for specific [³H]tetracaine incorporation within $delta$ M2.

[³H]Tetracaine Photoincorporation in $beta$ Subunit. White and Cohen (1992) showed that digestion of [¹²⁵I]TID-labeled $beta$ subunit with trypsin generated a 7-kDa fragment beginningat the N terminus of $beta$ M2 and extending through the M3 segment,as well as 3- and 10-kDa fragments that also contained $beta$ M2. Therefore,we digested [³H]tetracaine-labeled $beta$ subunit (160 µg, 290,000 cpm) with trypsin[25% (w/w)] for 4 days at ambient temperature and then purifiedthe digestion products by Tricine SDS-PAGE. Aliquots (5 µg) wereelectrophoresed in analytical lanes adjacent to the bulk digest.The ³H distribution in these analytical lanes (Fig. 2A) showed thatspecifically labeled material migrated in bands at 7 and 3 kDa.Material was eluted from gel strips (bands A-G) that were excisedfrom the preparative lanes that spanned from below the 3-kDa markerto above the 14-kDa marker. Bands B and C, which contained 54,000cpm (19% of loaded counts), were combined and denoted $beta$ T-3, andbands E and F, which contained 52,000 cpm (18% of loaded counts),were combined and denoted $beta$ T-7.

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Fig. 2. Proteolytic mapping with trypsin of [³H]tetracaine incorporation in the nAChR $beta$ subunit. All panels display results from parallel photolabelings of nAChR-rich membranes with [³H]tetracaine in the absence (

) or presence ( $open circle$ ) of HTX. Solutions (0.7 mg/ml) of [³H]tetracaine-labeled $beta$ subunit were digested with trypsin (0.2 mg/ml) for 4 days at ambient temperature and then fractionated by Tricine SDS-PAGE with 5-µg aliquots ( $-$ HTX, 9000 cpm; +HTX, 2630 cpm) electrophoresed in analytical lanes adjacent to the bulk digests. A, distribution of ³H in the analytical lanes is shown in relation to molecular weight markers (above) and the strips (A-G) excised from the preparative lanes. For the $-$ HTX sample, 213,600 cpm was loaded on the preparative lane, with 19,200, 29,200, 25,000, 20,450, 25,650, 26,350, and 12,850 cpm recovered from strips A to G, respectively. The eluates from strips B and C (~3 kDa) were combined and designated as fragment $beta$ T-3, and the eluates from strips E and F (~7 kDa) were combined and designated as fragment $beta$ T-7. B and D, reversed phase HPLC purification of $beta$ T-7 and $beta$ T-3 (5% of the HPLC fractions were assayed for ³H). B, for $beta$ T-7 ( $-$ HTX), 46% of the 51,000 cpm injected was recovered in a single peak associated with two absorbance peaks. Fractions 22 to 24 were combined for sequence analysis. D, for $beta$ T-3 ( $-$ HTX), specifically labeled material eluted in three peaks that together accounted for 70% of the injected ³H. Fractions 13 to 15 ( $beta$ T-3a, 30% of injected ³H) and fractions 16 to 19 ( $beta$ T-3b, 20% of injected ³H) were pooled for sequence analysis. C, ³H and mass release on N-terminal sequencing of $beta$ T-7 purified by reversed phase HPLC. For both samples, the primary sequence began at $beta$ Met²⁴⁹, the N terminus of $beta$ M2 (

, $-$ HTX, I₀ = 13 pmol, R = 92%, 16,420 cpm loaded/3180 cpm remained on the filter; +HTX, I₀ = 12 pmol, R = 96%), and a secondary sequence began at $beta$ Lys²¹⁶, the N terminus of $beta$ M1 ( $-$ HTX, I₀ = 6 pmol, R = 92%; +HTX, I₀ = 8 pmol, R = 95%). The sequences of the identified peptides are shown above. Additional PTH derivatives were present at <20% the level the primary sequence. E, sequence analysis of $beta$ T-3b. After one cycle of Edman degradation, the sequencing filter was treated with OPA, which reacts selectively with the free N termini of amino acids other than proline, a secondary amine, blocking Edman degradation (Brauer et al., 1984

). After OPA block, the primary sequence in both samples began at $beta$ Lys²¹⁶, the N terminus of $beta$ M1 ( $-$ HTX, I₀ ~ 1 pmol, R = 95%, 10,400 cpm loaded/410 cpm remained on the filter). The sequence of the identified peptide is shown above.

The material eluted from $beta$ T-7 was further purified by HPLC (Fig. 2B). The specifically labeled material was recovered in asingle peak (fractions 22-24) that was associated with two peaksin absorbance. For the nonspecifically labeled sample, the ³H in those fractions was <10% that of the specifically labeledsample, whereas the absorbance peaks were similar to those forthe specifically labeledsample.

Sequence analysis of HPLC purified $beta$ T-7 (Fig. 2C) revealed the presence of a primary sequence beginning at $beta$ Met²⁴⁹ at the N terminus of $beta$ M2 (I₀ = 13 pmol) and a secondary sequencebeginning at $beta$ Lys²¹⁶ at the N terminus of $beta$ M1 (I₀ = 6 pmol). There was a clear peakof release of ³H in cycle 9 that was reduced by >95% for the sample labeled nonspecifically.If the release in cycle 9 originated from the primary sequence( $beta$ M2), it would indicate labeling of $beta$ Leu²⁵⁷, the amino acid homologous to the major site of labeling in $delta$ subunit ( $delta$ Leu²⁶⁵).

To test whether the ³H release in cycle 9 during the sequencing of $beta$ T-7 was from the $beta$ M2 or the $beta$ M1 domain, the $beta$ T-3 band wasalso analyzed. When the $beta$ T-3 band was purified by HPLC (Fig. 2D),material was recovered in three overlapping peaks of ³H. The largest peak (denoted $beta$ T-3a), which accounted for 35% ofthe loaded cpm, was centered at 52% organic, and a second peak(denoted $beta$ T-3b), which accounted for 22% of the loaded ³H, eluted at ~59% organic. $beta$ T-3a eluted in the HPLC gradient whereWhite and Cohen (1992)

previously recovered a 3-kDa fragment ofthe $beta$ M2 domain, whereas $beta$ T-3b eluted close to the reported positionof $beta$ M1 (Blanton and Cohen, 1994

Sequence analysis of $beta$ T-3a revealed ³H release only in cycle 9, as was seen for $beta$ T-7. However, the presence of at least fourdifferent sequences, including autodigestion products of trypsin,precluded direct fragment identification (not shown). For $beta$ T-3b,a sequencing protocol was used to determine whether any ³H release originated from the $beta$ M1 segment. To selectively sequence $beta$ M1 in a sample likely to contain other $beta$ subunit fragments, OPA,a compound that selectively blocks primary but not secondary amines(proline), was applied before the second sequencing cycle where $beta$ Pro²¹⁷ was expected to be exposed. This treatment will block the Edmandegradation of all peptides that do not contain an N-terminalproline residue. After OPA treatment at cycle 2, the only observedsequence began at $beta$ Pro²¹⁷ ( $beta$ M1) which was present at an initial mass of 1 pmol (Fig. 2E),and there was no ³H release above background. At this mass of $beta$ M1, one would haveexpected to see 70 cpm of ³H release at cycle 9 if the ³H release seen in the sequencing of $beta$ T-7 (Fig. 2C) correspondedto $beta$ Thr²²⁴ (in $beta$ -M1) and not $beta$ Leu²⁵⁷ (in $beta$ M2). Because the sequencing of $beta$ T-3b demonstrated that therewas no ³H release at cycle 9 in $beta$ M1, we conclude that $beta$ Leu²⁵⁷ (in $beta$ M2) is labeled and not $beta$ Thr²²⁴.

[³H]Tetracaine Photoincorporation in $alpha$ Subunit. The specific [³H]tetracaine photolabeling in the $alpha$ subunit is contained within $alpha$ V8-20 (Ser¹⁶²/Ser¹⁷³ to Glu³³⁸/Asn³³⁹), a proteolytic fragment produced by an "in gel" digest of $alpha$ subunit with V8 protease (Middleton et al., 1999). To determinewhether that specific labeling was within $alpha$ M2, [³H]tetracaine-labeled $alpha$ V8-20 was digested with endoproteinase Lys-C,which had been used previously (Pedersen et al., 1992) to generatean ~8-kDa fragment beginning at the N terminus of $alpha$ M2 in studiesof the site of labeling of [³H]meproadifen mustard. When the EKC digest was fractionated byTricine SDS-PAGE, the distribution of ³H in the analytical lanes (Fig. 3A) contained a peak of specificallylabeled material migrating at ~8 kDa, as well as material aggregatednear the top of the gel and a band of ~14 kDa. The preparativelanes of the gels were cut into strips (referred to as bands A-G),which together spanned the gel from below the 6-kDa marker toabove the 14-kDa molecular weight marker. For the digest of $alpha$ V8-20labeled in the absence of HTX, 14,000 cpm of the 74,000 cpm loadedon the gel was recovered from bands D and E. This material, whichwas combined and denoted as $alpha$ EKC-8, accounted for 40% of the ³H cpm eluted. When $alpha$ EKC-8 was further purified by HPLC (Fig. 3B),50% of the loaded cpm was recovered in a single peak (fractions25-27) associated with single peaks in fluorescence and absorbance.For the sample labeled in the presence of HTX, the ³H in that peak was reduced by >90%, whereas the peaks in fluorescenceand absorbance were similar in size to those seen for the specificallylabeled sample (not shown).

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Fig. 3. Proteolytic mapping of [³H]tetracaine incorporation in the nAChR $alpha$ subunit with endoproteinase Lys-C (A-C) or S. aureus V8 protease (D). All panels display results from parallel photolabelings of nAChR-rich membranes with [³H]tetracaine in the absence (

) or presence ( $open circle$ ) of HTX. Solutions (0.6 mg/ml) of $alpha$ V8-20 isolated from [³H]tetracaine-labeled $alpha$ subunit were digested with EKC (3 U/ml) for 6 days at ambient temperature and fractionated by Tricine SDS-PAGE with 5-µg aliquots ( $-$ HTX, 16,060 cpm; +HTX, 3315 cpm) electrophoresed in analytical lanes adjacent to the bulk digests. A, the distribution of ³H in the analytical lanes is shown in relation to molecular weight markers (above) and the strips (A-G) excised from the preparative lanes. For the $-$ HTX sample, 73,900 cpm was loaded on the preparative lane, with 1550, 2750, 2050, 7150, 7550, 2000, and 1850 cpm recovered from strips A to G, respectively. The eluates from strips D and E were combined and designated as $alpha$ EKC-8. B, reversed phase HPLC purification of $alpha$ EKC-8 (5% of the HPLC fractions were assayed for ³H). For the $-$ HTX sample, 50% of the 14,000 cpm injected was recovered in a single peak associated with a single peak in absorbance and fluorescence (not shown). Fractions 25 to 27 were combined for sequence analysis. C, ³H and mass released from N-terminal sequencing of $alpha$ EKC-8 purified by reversed phase HPLC. The only sequence detected in either sample began at $alpha$ Met²⁴³, the N terminus of $alpha$ M2 (

, $-$ HTX, I₀ = 11 pmol, R = 86%, 6740 cpm loaded/680 cpm remained on the filter; +HTX, I₀ = 27 pmol, R = 86%). The sequence of the identified peptide is shown above. This sequence was present at a 10-fold higher level than any secondary sequence. D, ³H release on N-terminal sequencing of an S. aureus V8 protease digest of $alpha$ V8-20. Solutions of [³H]tetracaine-labeled $alpha$ V8-20 (0.3 mg/ml) were further digested with equal weight of V8 protease for 28 days at ambient temperature and then separated by reversed phase HPLC (not shown). The ³H peak (43% of recovered ³H), which eluted at 88% organic, was sequenced ( $-$ HTX, 14,500 cpm loaded/3640 cpm remained on the filter). The presence of multiple PTH derivatives in each cycle of Edman degradation precluded the identification of peptides in this sample.

Sequence analysis of HPLC-purified $alpha$ EKC-8 (Fig. 3C) revealed the presence of a peptide beginning at $alpha$ Met²⁴³ at the N terminus of $alpha$ M2 ( $-$ HTX, I₀ = 11 pmol; +HTX, I₀ = 27 pmol),with any other sequence present at <10% that level. The majorpeak of ³H release was in cycle 9 ( $alpha$ Leu²⁵¹), with lower level ³H release in cycles 5 ( $alpha$ Ile247) and 13 ( $alpha$ Val-255). The observed³H release resulted from specific [³H]tetracaine photolabeling, since the ³H release was reduced by >90% in the sample isolated from nAChRphotolabeled in the presence of HTX.

An alternative digestion strategy using S. aureus V8 protease in conjunction with radiochemical sequencing also led to theconclusion that $alpha$ Ile²⁴⁷ and $alpha$ Leu²⁵¹ were the amino acids specifically photolabeled by [³H]tetracaine. There is a potential cleavage site for V8 proteaseat $alpha$ Glu²⁴¹ immediately preceding $alpha$ Lys²⁴² that was the site of cleavage by EKC. [³H]Tetracaine-labeled $alpha$ V8-20 was digested for 28 days with an equalweight of S. aureus V8 protease, and the digest was then fractionatedby HPLC. Radioactivity (34% of eluted cpm) was recovered in apeak centered at 88% organic that was sequenced for 25 cycles(Fig. 3D). Although the presence of multiple PTH derivatives ineach sequencing cycle prevented identification of the fragmentspresent, there was ³H release in cycles 6, 10, and 15. Release in cycles 6 and 10was consistent with the ³H release seen in cycles 5 and 9 in the sequencing of $alpha$ EKC-8.The lack of significant ³H release in cycle 14 was not surprising, based on the relativelevels of ³H release in cycles 9 and 13 in the sequencing of $alpha$ EKC-8. Releasein cycle 15 was unexpected. It might result from labeling of $alpha$ Val255with release in cycle 15 rather than 14 due to low repetitiveyield of Edman degradation, but it could also result from [³H]tetracaine photoincorporation in another, unidentifiedfragment.

[³H]Tetracaine Photoincorporation in $gamma$ Subunit. Attempts to isolate a labeled fragment of $gamma$ subunit were unsuccessful. Digestion of intact $gamma$ subunit with either endoproteinaseLys-C or trypsin resulted in specifically labeled fragment orfragments of <3 kDa, which when repurified by HPLC eluted in commonwith many peptides. After digestion of $gamma$ subunit (170 µg) withtrypsin, 31% of the specifically labeled material migrated ina band below 3 kDa ( $gamma$ T-3), a result consistent with the presenceof trypsin sites at the N and C termini of $gamma$ M2. When further purifiedby reversed phase HPLC, 34% of the specifically labeled cpm wererecovered in a peak centered at 48% organic, consistent with apreviously characterized 3-kDa peptide containing M2 (White andCohen, 1992). Sequence analysis of HPLC-purified $gamma$ T-3 revealedthe presence of a complex mixture of unidentifiable peptides.There was a peak of ³H release in cycle 9 (40 cpm), which, if it originated from $gamma$ M2,would correspond to $gamma$ Leu²⁶⁰, the amino acid homologous to the most highly labeled amino acidsin the othersubunits.

	Discussion

Top Summary Introduction Experimental Procedures Results Discussion References

In this report, we mapped the binding site for [³H]tetracaine in the closed channel state of the Torpedo nAChR by identifyingthe amino acids specifically photolabeled by this drug. N-terminalsequencing demonstrated that the specific photoincorporation withinthe $alpha$ , $beta$ , and $delta$ subunits was contained within proteolytic fragmentsthat included the M2 segments. Sites of specific ³H release in these fragments corresponded to labeling within theM2 segments of $alpha$ Ile²⁴⁷, $alpha$ Leu²⁵¹, $alpha$ Val²⁵⁵, $beta$ Leu²⁵⁷, $delta$ Leu²⁶⁵, $delta$ Ala²⁶⁸, and $delta$ Val²⁶⁹. Trypsin digestion of labeled $gamma$ subunit produced a labeled proteolyticfragment whose size and hydrophobicity were consistent with theknown properties of isolated M2 segments, and sequence analysisof this material showed release of ³H nine cycles after the N terminus that, if originating from $gamma$ M2,corresponds to $gamma$ Leu260.

Each of the labeled residues lies on a common helical face of the M2 segments (Fig. 4A). Because [³H]tetracaine binds to the nAChR with a 1:1 stoichiometry (Middletonet al., 1999), the photolabeling data provide clear evidence thatthis binding site is located within the lumen of the closed ionchannel and identify the amino acids within M2 that are in closeproximity to bound tetracaine. Although [¹²⁵I]TID labels many of the same residues (White and Cohen, 1992),the additional residues labeled by [³H]tetracaine ( $alpha$ Ile²⁴⁷, $delta$ Ala²⁶⁸) extend the definition of the surface of the M2 helix that isoriented toward the lumen of the closed ion channel (Fig. 4B;[³H]tetracaine: $delta$ arc = 100 degrees, $alpha$ arc = 80 degrees; [¹²⁵I]TID: $alpha$ , $beta$ , $delta$ arcs = 40 degrees).

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Fig. 4. The pattern of [³H]tetracaine photoincorporation defines the surface of the M2 segments lining the closed channel and suggests a model for tetracaine binding within the nAChR ion channel. A, space-filling, $alpha$ -helical models of each subunit's M2 segment and a model at the same scale of tetracaine in an extended conformation were made using the molecular modeling software Insight (Biosym, Inc.). The M2 residues labeled by [³H]tetracaine, which are shaded, lie on a single helical face. The presumed photoreactive aromatic atoms of tetracaine are positioned at the same level as the labeled residues of the M2 helices. In this orientation, tetracaine's dimethylaminoethyl group would be in proximity to the hydrophilic side chains at position M2-6, whereas its N-butyl group is aligned with the hydrophobic residues toward the C terminus of the M2-segment. B, when depicted on a helical wheel, the $alpha$ carbons of the labeled residues in the $alpha$ subunit (positions 5, 9, and 13) span 80 degrees of the helix cylinder, and those of the $delta$ subunit (positions 9, 12, and 13) span 100 degrees of the helical face. Thus, identification of amino acids labeled by [³H]tetracaine extends the definition of the surface of the M2 helices lining the lumen of the closed channel beyond those side labeled by [¹²⁵I]TID (residues 9 and 13; White and Cohen, 1992

The photochemistry of [³H]tetracaine is unknown. However, the photolysis products of para-aminobenzoic acid (Chignell et al.,1980; Gasparro, 1985) include reactive radicals at the aromaticnitrogen and on the adjacent carbon on the benzene ring. Thissuggests that reactive radicals should be produced at tetracaine'saromatic atoms as well. In the model in Figure 4A, tetracainehas been aligned with its benzene ring positioned at the levelof M2 position 9 (i.e., at the level of the amino acids that arethe most efficiently labeled in each M2 segment). In this orientation,tetracaine's benzene ring, as well as its aryl nitrogen and carboxyl,could interact with the labeled residues at positions 5, 9, 12,and 13 and account for all the specific photolabeling. With thebenzene ring at this position, chemical intuition suggests thatit would be energetically favorable for tetracaine to be orientedas shown with its N-butyl substituent interacting with the hydrophobicresidues at positions 16 and 17 (leucines, valines, and phenylalanines)and the dimethylamino group (probably protonated) interactingwith hydrophilic side chains (serines and threonines) at position6.

An orientation of tetracaine with its N-butyl group interacting with the hydrophobic residues at positions M2-16 and M2-17is consistent with structure-activity studies of tetracaine analogs.Procaine, a tetracaine analog that lacks the butyl group on thearyl nitrogen, is bound by the Torpedo nAChR in the absence ofagonist with 1000-fold lower affinity than tetracaine (Middletonet al., 1999). Although the hydrophobic side chains at M2-16 andM2-17 would form an energetically favorable environment for thebutyl group of tetracaine, no such stabilization would be expectedfor the unsubstituted aryl nitrogen of procaine. In addition,if the desensitized state of the nAChR has a more open pore structureat the level of positions 2, 6, and 9, as is required to accommodatedrugs such as trimethylphenylphosphonium and chlorpromazine and(Hucho et al., 1986; Revah et al., 1990; White and Cohen, 1992),then the dimethylamino of tetracaine may contribute less to theenergetics of binding in the desensitized state than does a diethylgroup. This interpretation is consistent with the analysis oftetracaine analogs by Middleton et al. (1999). This proposed orientationof bound tetracaine is also consistent with the observation thattetracaine is 10 times more potent as an antagonist of Torpedothan of mouse muscle nAChR (Eterovic et al., 1993). The Torpedoand mouse muscle nAChRs have nearly identical M2 segments, withsubstitutions at three positions in $beta$ subunit ( $beta$ S2G, $beta$ S6F, $beta$ A10T)and one in $gamma$ subunit ( $gamma$ S6N). The differences include an increasein hydrophobicity at position 6 in the mouse $beta$ subunit. If ourmodel of tetracaine's interaction with the Torpedo receptor iscorrect, then the mouse muscle nAChR may interact less stronglywith the charged dimethylamino group oftetracaine.

The positioning of tetracaine's dimethylamino group near position M2-6 is in apparent contrast to the proposed permeabilitybarrier. Previous mutagenesis (Revah et al., 1991; Filatov andWhite, 1995; Labarca et al., 1995), electron microscopy (Unwin,1993, 1995), and photolabeling (White and Cohen, 1992; Blantonet al., 1998) studies have suggested that the hydrophobic sidechains at M2-9 could form the permeability barrier in the closedchannel. However, the kinetics of [³H]tetracaine binding to the Torpedo nAChR in the absence of agonistare characterized by very low association (k₊ = 4 × 10⁴ M¹ min¹) and dissociation (k = 3 × 10⁴ s¹) rate constants at 4°C (Cohen et al., 1986; Strnad, 1988). Thisindicates that tetracaine's access to its high-affinity bindingsite in the closed channel, as well as its kinetics of dissociation,is greatly hindered and depend on slow changes in the structureof the pore region that are distinct from the movements requiredfor channel opening. In support of this interpretation, TID, whichhas a much greater association rate constant at 4°C (k₊ ~2 × 10⁶ M¹ min¹; Wu et al., 1994), is not in contact with (i.e., does not label)residues below M2-9 in the absence ofagonist.

An alternative model for the permeability barrier, based on the access from the extracellular side of water-soluble sulfhydrylreagents in the absence of agonist to positions as low as M2-2,places the permeability barrier below M2-2 (Akabas et al., 1994;Pascual and Karlin, 1998). However, for 2-aminoethyl methanethiosulfonate,the rate of reaction with a cysteine at position 2 in $alpha$ M2 was3 × 10⁴ M¹ min¹ (Pascual and Karlin, 1998), which is close to the observed associationrate constant for [³H]tetracaine binding to Torpedo nAChR, whereas the rates of reactionat positions 6, 9, and 10 were 1 to 3 × 10³ M¹ min¹. Although it is clear that factors other than the kinetics ofaccess do contribute to the rate constant for cysteine alkylation,the observed accessibility and reactivity of cysteines withinthe M2 channel domain in the absence of agonist are not incompatiblewith a structural barrier made up by the aliphatic residues atM2-9 that contributes to the hindered binding of tetracaine andto the permeability barrier to inorganic cations in the closedchannel. There is no reason to expect that the kinetics of tetracaineassociation and dissociation from the closed channel would bedetermined by a structural constraint below the level of position2 in the M2domain.

Tetracaine is an unusual NCA in that it binds with 100-fold higher affinity to the resting state than to the desensitizedstate, and this preferential binding in the absence of agonistemphasizes the restricted dimensions of drugs that can be accommodatedwithin the structure of the closed channel. In the absence ofagonist, a benzene ring (~6.5 Å) as well as the butylamino group(~4 Å wide in extended configuration) can be accommodated withinthe ion channel in a hydrophobic environment that does not existin the desensitized state of the nAChR. The hindered binding kineticsindicates that the structure of the pore must relax somewhat toaccommodate tetracaine, but the change in structure is far smallerthan that required for transitions to either the open channelor desensitized state. Although the width of tetracaine may belarger than the restriction in the closed channel in the absenceof drug, it is not nearly as large as the desensitizing NCAs suchas chlorpromazine that bind at the level of M2-2 and M2-6 in thedesensitized state (Revah et al., 1990). The hydrophobic ringmade up by the leucines at M2-9 must be more splayed apart inthe desensitized than in the resting state (White and Cohen, 1992),and there is no longer a domain within the pore with a structurefavorable for the high-affinity binding of a molecule with tetracaine'sdimensions.

	Acknowledgments

We thank Dr. David Chiara for his valuable guidance in protein sequencing strategies and for assistance with the preparationof the finalfigures.

	Footnotes

Received March 23, 1999; Accepted May 18, 1999

¹ Present address: Department of Neurology, Washington University School of Medicine, St. Louis, MO63110.

This work was supported in part by United States Public Health Service Grant NS19522 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

nAChR, nicotinic acetylcholine receptor; HTX, dl-perhydrohistrionicotoxin; PAGE, polyacrylamide gel electrophoresis; NCA, noncompetitive antagonist; EKC, endoproteinase Lys-C; 1-AP, 1-azidopyrene; V8 protease, Staphylococcus aureus glutamyl endopeptidase; TFA, trifluoroacetic acid; OPA, o-phthalaldehyde; PTH, phenylthiohydantoin; [¹²⁵I]TID, 3-(trifluoromethyl)-3-(M-[¹²⁵I]iodophenyl)diazirine; TPS, Torpedo physiological saline.

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