TY - JOUR
T1 - Asymmetric and independent contribution of the second transmembrane segment 12' residues to diliganded gating of acetylcholine receptor channels
T2 - A single-channel study with choline as the agonist
AU - Grosman, Claudio
AU - Auerbach, Anthony
PY - 2000/5
Y1 - 2000/5
N2 - Mutagenesis studies have suggested that the second transmembrane segment (M2) plays a critical role during acetylcholine receptor liganded gating. An adequate description of the relationship between gating and structure of the M2 domain, however, has been hampered by the fact that many M2 mutations increase the opening rate constant to levels that, in the presence of acetylcholine, are unresolvably fast. Here, we show that the use of saturating concentrations of choline, a low-efficacy agonist, is a convenient tool to circumvent this problem. In the presence of 20 mM choline: (a) single-channel currents occur in clusters; (b) fast blockade by choline itself reduces the single-channel conductance by ~50%, yet the excess open- channel noise is only moderate; (c) the kinetics of gating are fitted best by a single-step, C mutually implies O model; and (d) opening and closing rate constants are within a well resolvable range. Application of this method to a series of recombinant adult mouse muscle M2 12' mutants revealed that: (a) the five homologous M2 12' positions make independent and asymmetric contributions to diliganded gating, the δ subunit being the most sensitive to mutation; (b) mutations at δ12' increase the diliganded gating equilibrium constant in a manner that is consistent with the sensitivity of the transition state to mutation being ~30% like that of the open state and ~70% like that of the closed state; (c) the relationship between δ12' amino acid residue volume, hydrophobicity or α-helical tendency, and the gating equilibrium constant of the corresponding mutants is not straightforward; however, (d) rate and equilibrium constants for the mutant series are linearly correlated (on log-log plots), which suggests that the conformational rearrangements upon mutation are mostly local and that the position of the transition state along the gating reaction coordinate is unaffected by these mutations.
AB - Mutagenesis studies have suggested that the second transmembrane segment (M2) plays a critical role during acetylcholine receptor liganded gating. An adequate description of the relationship between gating and structure of the M2 domain, however, has been hampered by the fact that many M2 mutations increase the opening rate constant to levels that, in the presence of acetylcholine, are unresolvably fast. Here, we show that the use of saturating concentrations of choline, a low-efficacy agonist, is a convenient tool to circumvent this problem. In the presence of 20 mM choline: (a) single-channel currents occur in clusters; (b) fast blockade by choline itself reduces the single-channel conductance by ~50%, yet the excess open- channel noise is only moderate; (c) the kinetics of gating are fitted best by a single-step, C mutually implies O model; and (d) opening and closing rate constants are within a well resolvable range. Application of this method to a series of recombinant adult mouse muscle M2 12' mutants revealed that: (a) the five homologous M2 12' positions make independent and asymmetric contributions to diliganded gating, the δ subunit being the most sensitive to mutation; (b) mutations at δ12' increase the diliganded gating equilibrium constant in a manner that is consistent with the sensitivity of the transition state to mutation being ~30% like that of the open state and ~70% like that of the closed state; (c) the relationship between δ12' amino acid residue volume, hydrophobicity or α-helical tendency, and the gating equilibrium constant of the corresponding mutants is not straightforward; however, (d) rate and equilibrium constants for the mutant series are linearly correlated (on log-log plots), which suggests that the conformational rearrangements upon mutation are mostly local and that the position of the transition state along the gating reaction coordinate is unaffected by these mutations.
KW - Allosteric proteins
KW - Bronsted plot
KW - Double- mutant cycles
KW - Kinetics
KW - Nicotinic receptors
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U2 - 10.1085/jgp.115.5.637
DO - 10.1085/jgp.115.5.637
M3 - Article
C2 - 10779320
AN - SCOPUS:0034064135
SN - 0022-1295
VL - 115
SP - 637
EP - 651
JO - Journal of General Physiology
JF - Journal of General Physiology
IS - 5
ER -