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蛋白质局部稳定性与整体稳定性之间的关系:细胞色素c的定点突变体和化学修饰衍生物

Relationship between local and global stabilities of proteins: site-directed mutants and chemically-modified derivatives of cytochrome c.

作者信息

Schejter A, Luntz T L, Koshy T I, Margoliash E

机构信息

Department of Biological Sciences, University of Illinois, Chicago 60607.

出版信息

Biochemistry. 1992 Sep 8;31(35):8336-43. doi: 10.1021/bi00150a030.

DOI:10.1021/bi00150a030
PMID:1326327
Abstract

The methionine 80 sulfur-heme iron bond of rat cytochrome c, whose stability is decreased by mutating the phylogenetically invariant residue proline 30 to alanine and increased when tyrosine 67 is changed to phenylalanine, recovers its wild-type characteristics when both substitutions are performed on the same molecule. Titrations with urea, analyzed according to the heteropolymer theory [Alonso, D. O. V., & Dill, K. A. (1991) Biochemistry 30, 5974-5985], indicate that both single mutations increase the solvent exposure of hydrophobic groups in the unfolded state, while in the double mutant this conformational perturbation disappears. Similar increases in solvent exposure of hydrophobic groups are observed when the sulfur-iron bond of the wild-type protein is broken by alkylation of the methionine sulfur, by high pH, or by binding the heme iron with cyanide. The compensatory effects of the two single mutations do not extend to the overall stability of the protein. The added loss of conformational stability due to the single mutations amounts to 7.3 kcal/mol out of the 9 kcal/mol representing the overall free energy of stabilization of the native conformation of the wild-type protein. The folded conformation of the doubly mutated protein is only 2 kcal/mol less stable than that of the wild type. These results indicate that the double mutant protein is able to retain the essential folding pattern of cytochrome c and the thermodynamic stability of the methionine sulfur-heme iron bond, in spite of structural differences that weaken the overall stability of the molecule.

摘要

大鼠细胞色素c的甲硫氨酸80与硫-血红素铁键,其稳定性会因将系统发育上不变的脯氨酸30突变为丙氨酸而降低,而当酪氨酸67变为苯丙氨酸时则会增加。当在同一分子上进行这两种取代时,该键恢复其野生型特征。根据杂聚物理论[阿隆索,D.O.V.,& 迪尔,K.A.(1991年)《生物化学》30,5974 - 5985]对尿素滴定进行分析,结果表明,这两个单突变都会增加未折叠状态下疏水基团的溶剂可及性,而在双突变体中这种构象扰动消失。当野生型蛋白质的硫-铁键通过甲硫氨酸硫的烷基化、高pH值或用氰化物结合血红素铁而断裂时,也观察到疏水基团溶剂可及性有类似增加。这两个单突变的补偿效应并未扩展到蛋白质的整体稳定性。由于单突变导致的构象稳定性额外损失在代表野生型蛋白质天然构象稳定化总自由能的9千卡/摩尔中占7.3千卡/摩尔。双突变蛋白质的折叠构象仅比野生型低2千卡/摩尔的稳定性。这些结果表明,尽管结构差异削弱了分子的整体稳定性,但双突变蛋白质仍能够保留细胞色素c的基本折叠模式以及甲硫氨酸硫-血红素铁键的热力学稳定性。

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