STRUCTURAL FEATURES OF ISOLATED M2 HELICES OF NICOTINIC RECEPTORS - SIMULATED ANNEALING VIA MOLECULAR-DYNAMICS STUDIES

被引：19

作者：

SANKARARAMAKRISHNAN, R ^{[1
]}

SANSOM, MSP ^{[1
]}

机构：

[1] UNIV OXFORD,MOLEC BIOPHYS LAB,OXFORD OX1 3QU,ENGLAND

来源：

BIOPHYSICAL CHEMISTRY | 1995年 / 55卷 / 03期

基金：

英国惠康基金;

关键词：

ION CHANNEL; TRANSMEMBRANE HELICES; MOLECULAR DYNAMICS; ELECTROSTATICS; SALT-BRIDGE; SIDE-CHAIN CONFORMATION;

D O I：

10.1016/0301-4622(95)00006-J

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

The nicotinic acetylcholine receptor is an integral membrane protein and a ligand-gated cation channel. It has stoichiometry alpha(2) beta gamma delta, the subunits arranged symmetrically around an approximate five-fold axis. Five M2 helices, one from each subunit, form a parallel helix bundle surrounding a central pore. Simulated annealing via restrained molecular dynamics (SA/MD) has been employed to generate ensembles of isolated M2 transmembrane helices. Four ensembles of two different M2 helix sequences, M2 delta and M2 gamma, have been generated by SA/MD. The ensembles differed in their treatment of electrostatic interactions. Analysis of the simulated structures showed that intra-helical H-bonds were more strongly conserved in the C-terminal (and more hydrophobic) segment of M2 helices. Conformations of polar sidechains have been analyzed, placing particular emphasis on EK (and QK) pairs at the N-termini of M2 delta (and M2 gamma) helices. Conformations of EK sidechain pairs were obtained for the high resolution structures in the protein database in order to guide our analysis of simulated structures. Serine and threonine sidechain conformations in the M2 models also have been determined. Implications of studies of isolated M2 helices for models of the intact pore region of the nicotinic receptor are discussed.

引用

页码：215 / 230

页数：16

共 47 条

[1] AN EVALUATION OF IMPLICIT AND EXPLICIT SOLVENT MODEL SYSTEMS FOR THE MOLECULAR-DYNAMICS SIMULATION OF BACTERIOPHAGE-T4 LYSOZYME
ARNOLD, GE
ORNSTEIN, RL
[J]. PROTEINS-STRUCTURE FUNCTION AND GENETICS, 1994, 18 (01): : 19 - 33
[2] HYDROGEN-BONDING IN GLOBULAR-PROTEINS
BAKER, EN
HUBBARD, RE
[J]. PROGRESS IN BIOPHYSICS & MOLECULAR BIOLOGY, 1984, 44 (02) : 97 - 179
[3] BECHINGER B, 1991, Journal of Biomolecular NMR, V1, P167, DOI 10.1007/BF01877228
[4] PROTEIN DATA BANK - COMPUTER-BASED ARCHIVAL FILE FOR MACROMOLECULAR STRUCTURES
BERNSTEIN, FC
KOETZLE, TF
WILLIAMS, GJB
MEYER, EF
BRICE, MD
RODGERS, JR
KENNARD, O
SHIMANOUCHI, T
TASUMI, M
[J]. JOURNAL OF MOLECULAR BIOLOGY, 1977, 112 (03) : 535 - 542
[5] CHARMM - A PROGRAM FOR MACROMOLECULAR ENERGY, MINIMIZATION, AND DYNAMICS CALCULATIONS
BROOKS, BR
BRUCCOLERI, RE
OLAFSON, BD
STATES, DJ
SWAMINATHAN, S
KARPLUS, M
[J]. JOURNAL OF COMPUTATIONAL CHEMISTRY, 1983, 4 (02) : 187 - 217
[6] Brooks III C. L., 1988, PROTEINS THEORETICAL
[7] SLOW-COOLING PROTOCOLS FOR CRYSTALLOGRAPHIC REFINEMENT BY SIMULATED ANNEALING
BRUNGER, AT
KRUKOWSKI, A
ERICKSON, JW
[J]. ACTA CRYSTALLOGRAPHICA SECTION A, 1990, 46 : 585 - 593
[8] BRUNGER AT, 1991, ACCOUNTS CHEM RES, V24, P54
[9] BRUNGER AT, 1992, X PLOR VERSION 3 0
[10] NEUTRON-DIFFRACTION STUDIES ON PHOSPHATIDYLCHOLINE MODEL MEMBRANES .1. HEAD GROUP CONFORMATION
BULDT, G
GALLY, HU
SEELIG, J
ZACCAI, G
[J]. JOURNAL OF MOLECULAR BIOLOGY, 1979, 134 (04) : 673 - 691

← 1 2 3 4 5 →