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多级质谱(MS(4))对人中性粒细胞髓过氧化物酶中活性依赖的血红素共价修饰的解构。

Deconstruction of activity-dependent covalent modification of heme in human neutrophil myeloperoxidase by multistage mass spectrometry (MS(4)).

机构信息

Pfizer Worldwide Research, Groton, Connecticut 06340, United States.

出版信息

Biochemistry. 2012 Mar 13;51(10):2065-77. doi: 10.1021/bi201872j. Epub 2012 Mar 1.

DOI:10.1021/bi201872j
PMID:22352991
Abstract

Myeloperoxidase (MPO) is known to be inactivated and covalently modified by treatment with hydrogen peroxide and agents similar to 3-(2-ethoxypropyl)-2-thioxo-2,3-dihydro-1H-purin-6(9H)-one (1), a 254.08 Da derivative of 2-thioxanthine. Peptide mapping by liquid chromatography and mass spectrometry detected modification by 1 in a labile peptide-heme-peptide fragment of the enzyme, accompanied by a mass increase of 252.08 Da. The loss of two hydrogen atoms was consistent with mechanism-based oxidative coupling. Multistage mass spectrometry (MS(4)) of the modified fragment in an ion trap/Orbitrap spectrometer demonstrated that 1 was coupled directly to heme. Use of a 10 amu window delivered the full isotopic envelope of each precursor ion to collision-induced dissociation, preserving definitive isotopic profiles for iron-containing fragments through successive steps of multistage mass spectrometry. Iron isotope signatures and accurate mass measurements supported the structural assignments. Crystallographic analysis confirmed linkage between the methyl substituent of the heme pyrrole D ring and the sulfur atom of 1. The final orientation of 1 perpendicular to the plane of the heme ring suggested a mechanism consisting of two consecutive one-electron oxidations of 1 by MPO. Multistage mass spectrometry using stage-specific collision energies permits stepwise deconstruction of modifications of heme enzymes containing covalent links between the heme group and the polypeptide chain.

摘要

髓过氧化物酶 (MPO) 已知可通过与过氧化氢和类似 3-(2-乙氧基丙基)-2-硫代-2,3-二氢-1H-嘌呤-6(9H)-酮 (1) 的试剂发生反应而被失活和共价修饰,1 是 2-硫代黄嘌呤的 254.08 Da 衍生物。通过液相色谱和质谱的肽图谱检测到该酶的不稳定肽-血红素-肽片段发生了 1 的修饰,伴随着 252.08 Da 的质量增加。失去两个氢原子与基于机制的氧化偶联一致。在离子阱/轨道阱质谱仪中对修饰片段进行多级质谱分析 (MS(4)) 表明 1 直接与血红素偶联。使用 10 amu 窗口将每个前体离子的完整同位素包络传输到碰撞诱导解离,通过多级质谱的连续步骤保留含铁片段的明确同位素分布。铁同位素特征和精确质量测量支持结构分配。晶体学分析证实了血红素吡咯 D 环的甲基取代基与 1 的硫原子之间的连接。1 垂直于血红素环平面的最终取向表明该机制由 MPO 对 1 进行的两个连续单电子氧化组成。使用特定于阶段的碰撞能量进行多级质谱分析,允许逐步解构含有血红素基团和多肽链之间共价连接的血红素酶的修饰。

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