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对溶菌酶衍生物中酰胺氢交换行为的二维核磁共振研究——该衍生物在Glu35和Trp108之间存在额外交联——协同波动的猝灭及其对蛋白质稳定性的影响。

A two-dimensional NMR study of exchange behavior of amide hydrogens in a lysozyme derivative with an extra cross-link between Glu35 and Trp108--quenching of cooperative fluctuations and effects on the protein stability.

作者信息

Noda Y, Fukuda Y, Segawa S

机构信息

School of Science, Department of Physics, Kwansei Gakuin University, Nishinomiya, Japan.

出版信息

Biopolymers. 1997 Feb;41(2):131-43. doi: 10.1002/(SICI)1097-0282(199702)41:2<131::AID-BIP2>3.0.CO;2-U.

DOI:10.1002/(SICI)1097-0282(199702)41:2<131::AID-BIP2>3.0.CO;2-U
PMID:9004550
Abstract

Two-dimensional nmr spectra [correlated spectroscopy (COSY), homonuclear Hartmann-Hahn (HOHAHA), nuclear Overhauser effect spectroscopy (NOESY)] have been observed for cross-linked lysozyme, a chemically modified lysozyme derivative with an extra ester cross-link between residues E35 and W108. Eight shifted cross-peaks were found in the fingerprint region of COSY spectra. By searching COSY, HOHAHA and NOESY spectra, they have been assigned to A32, E35, S36, 158, A107, W108, V109, and A110. The NOE connectivities (dNN and d alpha N) found for the cross-linked lysozyme are quite similar to those for the intact lysozyme. Exchange behavior of amide hydrogens has been studied for both intact and cross-linked lysozymes by observing the fingerprint region of COSY spectra. Hydrogen exchange reactions were carried out at pH 7.0 and at several temperatures. There exist 41 amide hydrogens whose exchange reactions are detectable under this experimental condition. Not only exchange rates but also their activation enthalpies were determined for individual amide hydrogens. They are classified into two groups, which are called categories III and IV. Category III hydrogens are distributed in relatively flexible peripheral parts of protein, and category IV hydrogens are deeply buried in the core region of protein. Category III hydrogens are exchanged through localized unfolding around their sites with a low activation enthalpy ranging from 10 to 25 kcal/mol. The formation of an extra cross-link affects neither the exchange rate nor the activation enthalpy of category III hydrogens. However, amide hydrogens of residues 34-39 in the vicinity of the hinge are exceptions. They are easily exchanged in the intact lysozyme but their exchange rates are drastically retarded by cross-linking. In the intact lysozyme, structural fluctuations mediating the exchange of category IV hydrogens are highly cooperative with a large activation enthalpy. These large-scale structural fluctuations are the global unfolding of the overall structure and also concerted motions within a domain. Especially near 38 degrees C, it was found that the dominant fluctuation occurring in the alpha-domain is different from that in the beta-domain. However, these concerted motions are strongly quenched by the formation of the cross-link because of the cooperativity of such a large-scale fluctuation. The stabilization of a localized area of protein by cross-linking results in the great suppression of large-scale and concerted motions. The exchange rates of category IV hydrogens are extremely retarded in the cross-linked lysozyme, so that they are exchanged through the so-called penetration mechanism characterized by a low activation enthalpy. These experimental results are discussed with regard to the contribution of cross-linking to the stabilization of the folded structure of protein.

摘要

已对交联溶菌酶进行了二维核磁共振谱(相关光谱法(COSY)、同核哈特曼-哈恩法(HOHAHA)、核Overhauser效应光谱法(NOESY))的观测,交联溶菌酶是一种化学修饰的溶菌酶衍生物,在E35和W108残基之间有一个额外的酯交联。在COSY谱的指纹区发现了8个位移交叉峰。通过搜索COSY、HOHAHA和NOESY谱,它们被归属为A32、E35、S36、I58、A107、W108、V109和A110。交联溶菌酶的NOE连接性(dNN和dαN)与完整溶菌酶的非常相似。通过观测COSY谱的指纹区,研究了完整和交联溶菌酶中酰胺氢的交换行为。在pH 7.0和几个温度下进行了氢交换反应。在该实验条件下,有41个酰胺氢的交换反应可被检测到。不仅测定了各个酰胺氢的交换速率,还测定了它们的活化焓。它们被分为两组,分别称为III类和IV类。III类氢分布在蛋白质相对灵活的外围部分,IV类氢深埋在蛋白质的核心区域。III类氢通过其位点周围的局部展开进行交换,活化焓较低,范围为10至25千卡/摩尔。额外交联的形成既不影响III类氢的交换速率,也不影响其活化焓。然而,铰链附近34 - 39残基的酰胺氢是例外。它们在完整溶菌酶中很容易交换,但交联会使其交换速率急剧减慢。在完整溶菌酶中,介导IV类氢交换的结构波动具有高度协同性,活化焓较大。这些大规模的结构波动是整体结构的全局展开以及结构域内的协同运动。特别是在38℃附近,发现α结构域中发生的主要波动与β结构域中的不同。然而,由于这种大规模波动的协同性,这些协同运动因交联的形成而被强烈抑制。交联导致蛋白质局部区域的稳定,从而极大地抑制了大规模和协同运动。交联溶菌酶中IV类氢的交换速率极其缓慢,因此它们通过以低活化焓为特征的所谓渗透机制进行交换。关于交联对蛋白质折叠结构稳定化的贡献,对这些实验结果进行了讨论。

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