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肌红蛋白:细胞色素b5相互作用及高铁肌红蛋白还原酶的动力学机制

Myoglobin: cytochrome b5 interactions and the kinetic mechanism of metmyoglobin reductase.

作者信息

Livingston D J, McLachlan S J, La Mar G N, Brown W D

出版信息

J Biol Chem. 1985 Dec 15;260(29):15699-707.

PMID:4066692
Abstract

Metmyoglobin (metMb) reduction by metMb reductase from heart muscle requires cytochrome b5 as electron-transfer mediator. The existence of a metMb-ferrous cytochrome b5 complex is demonstrated by mutual perturbation of the proteins' respective electrophoretic titration curves between pH 4 and 7. The same technique shows a preferential binding of cytochrome b5 over metMb by the enzyme. The paramagnetic hyperfine shifts in the cytochrome b5 1H NMR spectrum are perturbed by metMb, indicating the formation of a specific bimolecular complex with a 1:1 stoichiometry and a binding constant estimated to be less than 10 microM. The resonances assigned to the cytochrome b5 heme 6-propionate methylene group exhibit the largest complexation shifts. Computer modeling implicates lysines 47, 50, and 98 of metMb as contact points with cytochrome b5 carboxylate residues 43, 44, 60, and heme 6-propionate. The mechanism of the enzymatic reduction establishes metMb reductase as an NADH-cytochrome b5 oxidoreductase. Cytochrome b5 is reduced at near diffusion-controlled rates by the enzyme with a turnover number of 1000 min-1 X Km for the cytochrome is 0.9 microM versus 100 microM reported for the erythrocyte enzyme. Ferrous cytochrome b5 then reduces metMb nonenzymatically with an apparent rate constant of 4.9 X 10(4) M-1 min-1 X Acetylation of metMb, which does not affect its oxygen affinity or chemical reduction, renders it a poor substrate for enzymatic reduction. This study suggests a function for the three exterior lysine residues conserved in all mammalian myoglobin sequences: they are contact points for complexation with cytochrome b5.

摘要

心肌中的高铁肌红蛋白还原酶将高铁肌红蛋白(metMb)还原需要细胞色素b5作为电子传递介质。在pH 4至7之间,通过蛋白质各自的电泳滴定曲线相互干扰,证明了高铁肌红蛋白 - 亚铁细胞色素b5复合物的存在。相同技术显示该酶对细胞色素b5的结合优先于高铁肌红蛋白。高铁肌红蛋白会干扰细胞色素b5的1H NMR谱中的顺磁超精细位移,表明形成了化学计量比为1:1的特定双分子复合物,其结合常数估计小于10 microM。归属于细胞色素b5血红素6 - 丙酸亚甲基的共振显示出最大的络合位移。计算机建模表明高铁肌红蛋白的赖氨酸47、50和98是与细胞色素b5羧酸盐残基43、44、60以及血红素6 - 丙酸的接触点。酶促还原机制将高铁肌红蛋白还原酶确定为一种NADH - 细胞色素b5氧化还原酶。细胞色素b5被该酶以接近扩散控制的速率还原,周转数为1000 min-1,细胞色素的Km为0.9 microM,而红细胞酶的Km报道为100 microM。亚铁细胞色素b5然后以4.9×10(4) M-1 min-1的表观速率常数非酶促地还原高铁肌红蛋白。高铁肌红蛋白的乙酰化不影响其氧亲和力或化学还原,但使其成为酶促还原的不良底物。这项研究表明在所有哺乳动物肌红蛋白序列中保守的三个外部赖氨酸残基具有一种功能:它们是与细胞色素b5络合的接触点。

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