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从变性状态下氢/氘交换获得的剩余结构中研究人酸性成纤维细胞生长因子 (hFGF-1) 的重折叠途径。

Investigating the refolding pathway of human acidic fibroblast growth factor (hFGF-1) from the residual structure(s) obtained by denatured-state hydrogen/deuterium exchange.

机构信息

Department of Chemistry, National Tsing-Hua University, Hsin-Chu, Taiwan, Republic of China.

出版信息

Biophys J. 2011 Jan 5;100(1):154-64. doi: 10.1016/j.bpj.2010.11.027.

Abstract

Human fibroblast growth factor 1 (hFGF-1) consists of 12 anti-parallel β-strands arranged into a β-trefoil architecture. We directly measured hydrogen/deuterium exchange rates on the urea-denatured hFGF-1 to obtain the information with regard to the persistent residual interaction(s) in the unfolded hFGF-1. Thirty-eight residues whose heteronuclear single quantum coherence cross-peaks can be observed after exchange show higher protections than those predicted for the same residues in a random coil conformation, suggesting the existence of residual structure(s). The urea-denaturation of hFGF-1 tested by both circular dichroism and fluorescence spectroscopy indicated that the unfolding process is a cooperative two-state process and that the residual structures observed did not originate from the existence of a partially structured intermediate. The coincident disappearance of the native heteronuclear single quantum coherence cross-peaks during the urea-denaturation process suggests that the residual structures observed contain no nativelike interactions. The protected residues (fold ons) in the urea-denatured state are mostly those that exchange slowly in the native state H/D exchange. The distribution of these fold ons in the native structure of hFGF-1 suggests that the refolding starts by collisions between the residual structures (microdomains) between the β-strands VI and VII, and between the β-strands II and III, which appear to be two independent refolding coordinates during the refolding process.

摘要

人成纤维细胞生长因子 1(hFGF-1)由 12 个反平行β-折叠组成β-三叶折叠结构。我们直接测量了尿素变性 hFGF-1 的氢/氘交换速率,以获得关于未折叠 hFGF-1 中持久残留相互作用的信息。在交换后可以观察到异核单量子相干峰的 38 个残基比在无规卷曲构象中相同残基的预测具有更高的保护作用,这表明存在残留结构。圆二色性和荧光光谱测试的 hFGF-1 尿素变性表明,展开过程是协同的两态过程,观察到的残留结构不是来自部分结构化中间产物的存在。在尿素变性过程中,天然异核单量子相干峰的同时消失表明观察到的残留结构不包含天然相互作用。在尿素变性状态下受保护的残基(折叠点)主要是在天然状态 H/D 交换中交换缓慢的残基。这些折叠点在 hFGF-1 天然结构中的分布表明,重折叠首先发生在β-链 VI 和 VII 之间以及β-链 II 和 III 之间的残留结构(微域)之间的碰撞,这两个结构在重折叠过程中似乎是两个独立的重折叠坐标。

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