Identification of a novel bond between a histidine and the essential tyrosine in catalase HPII of Escherichia coli

被引:54
作者
Bravo, J
Fita, I
Ferrer, JC
Ens, W
Hillar, A
Switala, J
Loewen, PC
机构
[1] UNIV MANITOBA,DEPT MICROBIOL,WINNIPEG,MB R3T 2N2,CANADA
[2] UNIV MANITOBA,DEPT PHYS,WINNIPEG,MB R3T 2N2,CANADA
[3] UNIV BARCELONA,FAC QUIM,DEPT BIOQUIM & BIOL MOL,E-08028 BARCELONA,SPAIN
[4] CSIC,CTR INVEST & DESARROLLO,ES-08034 BARCELONA,SPAIN
关键词
catalase; crystal structure; Escherichia coli; heme; histidine-tyrosine linkage; protein modification; LASER-DESORPTION IONIZATION; MIRABILIS PR CATALASE; 3-DIMENSIONAL STRUCTURE; CRYSTAL-STRUCTURE; RESOLUTION; SEQUENCE; PROTEIN; KATE;
D O I
10.1002/pro.5560060507
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
A bond between the N-delta of the imidazole ring of His 392 and the C-beta of the essential Tyr 415 has been found in the refined crystal structure at 1.9 Angstrom resolution of catalase HPII of Escherichia coli. This novel type of covalent linkage is clearly defined in the electron density map of HPII and is confirmed by matrix-assisted Laser desorption/ionization mass spectrometry analysis of tryptic digest mixtures. The geometry of the bond is compatible with both the sp(3) hybridization of the C-beta atom and the planarity of the imidazole ring. Two mutated variants of HPII active site residues, H128N and N201H, do not contain the His 392-Tyr 415 bond, and their crystal structures show that the imidazole ring of His 392 was rotated, in both cases, by 80 degrees relative to its position in HPII. These mutant forms of HPII are catalytically inactive and do not convert heme b to heme d, suggesting a relationship between the self-catalyzed heme conversion reaction and the formation of the His-Tyr linkage. A model coupling the two processes and involving the reaction of one molecule of H2O2 on the proximal side of the heme with compound I is proposed.
引用
收藏
页码:1016 / 1023
页数:8
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