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T4溶菌酶折叠与功能的结构及遗传学分析

Structural and genetic analysis of the folding and function of T4 lysozyme.

作者信息

Matthews B W

机构信息

Institute of Molecular Biology, Howard Hughes Medical Institute, Eugene, Oregon, USA.

出版信息

FASEB J. 1996 Jan;10(1):35-41. doi: 10.1096/fasebj.10.1.8566545.

Abstract

The combination of directed mutagenesis with high-resolution structure analysis has made it possible to systematically address fundamental questions of protein folding and stability. Here we briefly review some recent results in this area based on studies of the lysozyme of bacteriophage T4. Extended segments of the polypeptide chain can be substituted with alanine, suggesting that about 50%, or perhaps less, of the overall amino acid sequence protein is necessary to define the 3-dimensional structure of the protein. It is the internal residues that seem to be most important for folding and stability (although not necessarily for function). Substitutions within the core of the protein of large nonpolar side chains with smaller ones have been used to better understand the nature of hydrophobic stabilization. Mutants that produce the largest cavities within the protein tend to be most destabilizing, allowing the energy cost of cavity formation to be estimated. Small, nonpolar ligands bind within such cavities and restore some stability to the protein. Analogous, nonpolar ligands do not bind, however, providing evidence that water molecules do not bind with high occupancy within nonpolar cavities. In a further series of studies it has been possible to re-engineer the active site region of T4 lysozyme to change the catalytic mechanism of the enzyme.

摘要

定向诱变与高分辨率结构分析相结合,使得系统地解决蛋白质折叠和稳定性的基本问题成为可能。在此,我们基于对噬菌体T4溶菌酶的研究,简要回顾该领域的一些最新成果。多肽链的延伸片段可用丙氨酸替代,这表明定义蛋白质三维结构大约需要50%或更少的总氨基酸序列。似乎是内部残基对折叠和稳定性最为重要(尽管不一定对功能重要)。用较小的非极性侧链取代蛋白质核心内较大的非极性侧链,已被用于更好地理解疏水稳定作用的本质。在蛋白质内部产生最大空洞的突变体往往最不稳定,从而可以估算形成空洞的能量成本。小的非极性配体结合在这些空洞内并恢复蛋白质的一些稳定性。然而,类似的非极性配体不结合,这证明水分子不会以高占有率结合在非极性空洞内。在另一系列研究中,已能够对T4溶菌酶的活性位点区域进行重新设计,以改变该酶的催化机制。

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