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质谱分析法鉴定出微管蛋白上的多个有机磷酸化位点。

Mass spectrometry identifies multiple organophosphorylated sites on tubulin.

作者信息

Grigoryan Hasmik, Schopfer Lawrence M, Peeples Eric S, Duysen Ellen G, Grigoryan Marine, Thompson Charles M, Lockridge Oksana

机构信息

University of Nebraska Medical Center, Eppley Institute for Cancer Research, 986805 Nebraska Medical Center, Omaha, NE 68198-6805, USA.

出版信息

Toxicol Appl Pharmacol. 2009 Oct 15;240(2):149-58. doi: 10.1016/j.taap.2009.07.020. Epub 2009 Jul 24.

Abstract

Acute toxicity of organophosphorus poisons (OP) is explained by inhibition of acetylcholinesterase in nerve synapses. Low-dose effects are hypothesized to result from modification of other proteins, whose identity is not yet established. The goal of the present work was to obtain information that would make it possible to identify tubulin as a target of OP exposure. Tubulin was selected for study because live mice injected with a nontoxic dose of a biotinylated organophosphorus agent appeared to have OP-labeled tubulin in brain as determined by binding to avidin beads and mass spectrometry. The experiments with live mice were not conclusive because binding to avidin beads could be nonspecific. To be convincing, it is necessary to find and characterize the OP-labeled tubulin peptide. The search for OP-labeled tubulin peptides was begun by identifying residues capable of making a covalent bond with OP. Pure bovine tubulin (0.012 mM) was treated with 0.01-0.5 mM chlorpyrifos oxon for 24 h at 37 degrees C in pH 8.3 buffer. The identity of labeled amino acids and percent labeling was determined by mass spectrometry. Chlorpyrifos oxon bound covalently to tyrosines 83, 103, 108, 161, 224, 262, 272, 357, and 399 in bovine alpha tubulin, and to tyrosines 50, 51, 59, 106, 159, 281, 310, and 340 in bovine beta tubulin. The most reactive were tyrosine 83 in alpha and tyrosine 281 in beta tubulin. In the presence of 1 mM GTP, percent labeling increased 2-fold. Based on the crystal structure of the tubulin heterodimer (PDB 1jff) tyrosines 83 and 281 are well exposed to solvent. In conclusion seventeen tyrosines in tubulin have the potential to covalently bind chlorpyrifos oxon. These results will be useful when searching for OP-labeled tubulin in live animals.

摘要

有机磷毒物(OP)的急性毒性是由神经突触中乙酰胆碱酯酶的抑制作用所解释的。低剂量效应被假定是由其他蛋白质的修饰引起的,而这些蛋白质的身份尚未确定。本研究的目的是获取能够将微管蛋白鉴定为OP暴露靶点的信息。选择微管蛋白进行研究是因为,通过与抗生物素蛋白珠结合及质谱分析确定,给活小鼠注射无毒剂量的生物素化有机磷试剂后,其大脑中似乎存在OP标记的微管蛋白。对活小鼠进行的实验并不具有决定性,因为与抗生物素蛋白珠的结合可能是非特异性的。为了令人信服,有必要找到并鉴定OP标记的微管蛋白肽段。通过鉴定能够与OP形成共价键的残基,开始了对OP标记的微管蛋白肽段的寻找。将纯牛微管蛋白(0.012 mM)在pH 8.3缓冲液中于37℃用0.01 - 0.5 mM毒死蜱氧磷处理24小时。通过质谱分析确定标记氨基酸的身份和标记百分比。毒死蜱氧磷与牛α微管蛋白中的酪氨酸83、103、108、161、224、262、272、357和399共价结合,与牛β微管蛋白中的酪氨酸50、51、59、106、159、281、310和340共价结合。反应性最强的是α微管蛋白中的酪氨酸83和β微管蛋白中的酪氨酸281。在1 mM GTP存在下,标记百分比增加了2倍。基于微管蛋白异二聚体的晶体结构(PDB 1jff),酪氨酸83和281很好地暴露于溶剂中。总之,微管蛋白中的17个酪氨酸具有与毒死蜱氧磷共价结合的潜力。这些结果在寻找活体动物中OP标记的微管蛋白时将很有用。

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