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基质辅助激光解吸电离诱导的亮氨酸脑啡肽、硝基酪氨酸亮氨酸脑啡肽和d(5)-苯丙氨酸-硝基酪氨酸亮氨酸脑啡肽的碎片化

MALDI-induced Fragmentation of Leucine enkephalin, Nitro-Tyr Leucine Enkaphalin, and d(5)-Phe-Nitro-Tyr Leucine Enkephalin.

作者信息

Zhan Xianquan, Desiderio Dominic M

机构信息

Charles B. Stout Neuroscience Mass Spectrometry Laboratory The University of Tennessee Health Science Center 847 Monroe Avenue, Room 117 Memphis, Tennessee 38163 USA.

出版信息

Int J Mass Spectrom. 2009 Oct 15;287(1-3):77-86. doi: 10.1016/j.ijms.2008.08.020.

Abstract

The long-term objective of this study is to use MALDI MS and MS/MS to study the fragmentation pattern of in vitro nitrotyrosine-containing peptides in order to assist the interpretation of MS-identification of endogenous nitroproteins in human tissues and fluids. The short-term objective is to study synthetic leucine enkephalin, nitro-Tyr-leucine enkephalin, and d(5)-Phe-nitro-Tyr-leucine enkephalin with a vacuum matrix-assisted laser desorption/ionization linear ion-trap mass spectrometer (vMALDI-LTQ). The results demonstrated the UV laser-induced photochemical decomposition of the nitro group. Although photochemical decomposition decreased the ion intensity and complicated the MS spectrum, the recognition of that unique decomposition pattern unambiguously identified a nitrotyrosine. The a(4)- and b(4)-ions were the most-intense fragment ions found in the MS/MS spectra for those three synthetic peptides. Compared to the unmodified peptides, more collision energy optimized the fragmentation of the nitropeptide, increased the intensity of the a(4)-ion, and decreased the intensity of the b(4)-ion. Optimized laser fluence maximized the fragmentation of the nitropeptide. MS(3) analysis confirmed the MS(2)-derived amino acid sequence, but required much more sample. To detect a nitropeptide, the sensitivity of vMALDI-LTQ is 1 fmol for MS detection and 10 fmol for MS(2) detection; the S/N ratio was ca. 50:1 in those studies. Those data are important for an analysis of low-abundance endogenous nitroproteins, where preferential enrichment of nitroproteins and optimized mass spectrometry parameters are used.

摘要

本研究的长期目标是使用基质辅助激光解吸电离质谱(MALDI MS)和串联质谱(MS/MS)研究体外含硝基酪氨酸肽段的碎裂模式,以辅助解释人体组织和体液中内源性硝基化蛋白质的质谱鉴定结果。短期目标是使用真空基质辅助激光解吸/电离线性离子阱质谱仪(vMALDI-LTQ)研究合成的亮氨酸脑啡肽、硝基酪氨酸-亮氨酸脑啡肽和d(5)-苯丙氨酸-硝基酪氨酸-亮氨酸脑啡肽。结果表明,紫外激光可诱导硝基的光化学分解。虽然光化学分解降低了离子强度并使质谱图复杂化,但对这种独特分解模式的识别明确鉴定出了硝基酪氨酸。对于这三种合成肽,a(4)离子和b(4)离子是MS/MS谱图中最强烈的碎片离子。与未修饰的肽相比,更多的碰撞能量优化了硝基肽的碎裂,增加了a(4)离子的强度,并降低了b(4)离子的强度。优化的激光能量密度使硝基肽的碎裂最大化。MS(3)分析证实了MS(2)推导的氨基酸序列,但需要更多的样品。为了检测硝基肽,vMALDI-LTQ的灵敏度在MS检测时为1 fmol,在MS(2)检测时为10 fmol;在这些研究中,信噪比约为50:1。这些数据对于分析低丰度内源性硝基化蛋白质很重要,在分析过程中会使用硝基化蛋白质的优先富集和优化的质谱参数。

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