Samson A O, Chill J H, Rodriguez E, Scherf T, Anglister J
Department of Structural Biology and Chemical Services, The Weizmann Institute of Science, Rehovot 76100, Israel.
Biochemistry. 2001 May 8;40(18):5464-73. doi: 10.1021/bi0022689.
The alpha-subunit of the nicotinic acetylcholine receptor (alphaAChR) contains a binding site for alpha-bungarotoxin (alpha-BTX), a snake-venom-derived alpha-neurotoxin. Previous studies have established that the segment comprising residues 173-204 of alphaAChR contains the major determinant interacting with the toxin, but the precise boundaries of this determinant have not been clearly defined to date. In this study, we applied NMR dynamic filtering to determine the exact sequence constituting the major alphaAChR determinant interacting with alpha-BTX. Two overlapping synthetic peptides corresponding to segments 179-200 and 182-202 of the alphaAChR were complexed with alpha-BTX. HOHAHA and ROESY spectra of these complexes acquired with long mixing times highlight the residues of the peptide that do not interact with the toxin and retain considerable mobility upon binding to alpha-BTX. These results, together with changes in the chemical shifts of the peptide protons upon complex formation, suggest that residues 184-200 form the contact region. At pH 4, the molecular mass of the complex determined by dynamic light scattering (DLS) was found to be 11.2 kDa, in excellent agreement with the expected molecular mass of a 1:1 complex, while at pH >5 the DLS measurement of 20 kDa molecular mass indicated dimerization of the complex. These results were supported by T(2) measurements. Complete resonance assignment of the 11.2 kDa complex of alpha-BTX bound to the alphaAChR peptide comprising residues 182-202 was obtained at pH 4 using homonuclear 2D NMR spectra measured at 800 MHz. The secondary structures of both alpha-BTX and the bound alphaAChR peptide were determined using 2D (1)H NMR experiments. The peptide folds into a beta-hairpin conformation, in which residues (R)H186-(R)V188 and (R)Y198-(R)D200 form the two beta-strands. Residues (R)Y189-(R)T191 form an intermolecular beta-sheet with residues (B)K38-(B)V40 of the second finger of alpha-BTX. These results accurately pinpoint the alpha-BTX-binding site on the alphaAChR and pave the way to structure determination of this important alphaAChR determinant involved in binding acetylcholine and cholinergic agonists and antagonists.
烟碱型乙酰胆碱受体(αAChR)的α亚基含有一个与α-银环蛇毒素(α-BTX)结合的位点,α-银环蛇毒素是一种源自蛇毒的α-神经毒素。先前的研究已确定,αAChR中包含第173 - 204位残基的片段含有与该毒素相互作用的主要决定因素,但该决定因素的确切边界迄今尚未明确界定。在本研究中,我们应用核磁共振动态过滤来确定构成与α-BTX相互作用的主要αAChR决定因素的确切序列。将与αAChR的第179 - 200位和第182 - 202位片段相对应的两个重叠合成肽与α-BTX复合。在长混合时间下获取的这些复合物的HOHAHA和ROESY谱突出了肽中不与毒素相互作用且在与α-BTX结合时仍保持相当大流动性的残基。这些结果,连同复合物形成时肽质子化学位移的变化,表明第184 - 200位残基形成了接触区域。在pH 4时,通过动态光散射(DLS)测定的复合物分子量为11.2 kDa,与预期的1:1复合物分子量非常吻合,而在pH > 5时,20 kDa分子量的DLS测量表明复合物发生了二聚化。这些结果得到了T(2)测量的支持。在pH 4时,使用800 MHz测量的同核二维核磁共振谱获得了与包含第182 - 202位残基的αAChR肽结合的α-BTX的11.2 kDa复合物的完全共振归属。使用二维(1)H NMR实验确定了α-BTX和结合的αAChR肽的二级结构。该肽折叠成β-发夹构象,其中残基(R)H186 - (R)V188和(R)Y198 - (R)D200形成两条β链。残基(R)Y189 - (R)T191与α-BTX第二指的残基(B)K38 - (B)V40形成分子间β-折叠。这些结果准确地确定了αAChR上的α-BTX结合位点,并为确定参与结合乙酰胆碱以及胆碱能激动剂和拮抗剂的这一重要αAChR决定因素的结构铺平了道路。
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