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采用 204Hg-同位素甲硫氨酸硫代水杨酸盐的动态标记策略进行绝对肽和蛋白质定量。

Dynamic labeling strategy with 204Hg-isotopic methylmercurithiosalicylate for absolute peptide and protein quantification.

出版信息

Anal Chem. 2010 Mar 1;82(5):1616-20. doi: 10.1021/ac902902y.

DOI:10.1021/ac902902y
PMID:20143794
Abstract

The methylmercury ion (CH(3)Hg(+)) demonstrated a high efficiency for directly labeling peptide/protein based on its specific and strong interaction with the sulfhydryl(s) in the peptide/protein and because of its smallest size among monofunctional organic mercurials studied, including methylmercury, ethylmercury, 4-(hydroxymercuric)benzoic acid, and 2,7-dibromo-4-hydroxymercurifluoresceine disodium. A simple 1:1 stoichiometry between CH(3)Hg(+) and sulfhydryl, confirmed with electrospray ionization-mass spectrometry (ESI-MS) and matrix-assisted laser desorption ionization-time-of-flight-mass spectrometry (MALDI-TOF-MS) studies, made it easy to calibrate the stoichiometry of Hg in the peptide/protein. In order to avoid the direct use of the harmful CH(3)Hg(+), in this study a CH(3)Hg(+)-equivalent tag, methylmercurithiosalicylate (CH(3)Hg-THI), and its (204)Hg-enriched homologue (CH(3)(204)Hg-THI) were synthesized, and then CH(3)Hg(+) and/or CH(3)(204)Hg(+) released from CH(3)Hg-THI and/or CH(3)(204)Hg-THI in solution were utilized to demonstrate the dynamic labeling of glutathione (GSH) and two model proteins, beta-lactoglobulin (BLG) and ovalbumin (OVA), for the first time. Furthermore, the CH(3)(204)Hg-THI isotopical labeled GSH, BLG, and OVA standards (CH(3)(204)Hg-GSH, CH(3)(204)Hg-BLG, and CH(3)(204)Hg-OVA) were used to demonstrate the feasibility of absolute peptide/protein quantification using label-specific isotope dilution inductively coupled plasma mass spectrometry (ICPMS). On the basis of the accurate and sensitive determination of Hg using ICPMS, the detection limits of GSH, BLG, and OVA could reach 45.4, 45.4, and 15.1 pmol L(-1), respectively, suggesting the possibility for low-abundance peptide/protein quantification alongside the surefire quantification of moderate and highly abundant peptide/protein.

摘要

甲基汞离子 (CH(3)Hg(+)) 因其与肽/蛋白质中的巯基(-SH)具有特异性和强相互作用,以及在研究的单功能有机汞中,包括甲基汞、乙基汞、4-(羟基汞基)苯甲酸和 2,7-二溴-4-羟基汞荧光素二钠盐,其尺寸最小,因此对基于肽/蛋白质的直接标记具有高效性。电喷雾电离质谱 (ESI-MS) 和基质辅助激光解吸电离飞行时间质谱 (MALDI-TOF-MS) 研究证实,CH(3)Hg(+)与巯基之间的简单 1:1 化学计量比使得很容易校准肽/蛋白质中的 Hg 化学计量比。为了避免直接使用有害的 CH(3)Hg(+),本研究合成了 CH(3)Hg(+)-等效标签甲基汞硫代水杨酸酯 (CH(3)Hg-THI) 及其 (204)Hg 富集同系物 (CH(3)(204)Hg-THI),然后利用溶液中 CH(3)Hg-THI 和/或 CH(3)(204)Hg-THI 释放的 CH(3)Hg(+) 和/或 CH(3)(204)Hg(+),首次动态标记谷胱甘肽 (GSH) 和两种模型蛋白,β-乳球蛋白 (BLG) 和卵清蛋白 (OVA)。此外,首次使用 (204)Hg 同位素标记的 CH(3)(204)Hg-THI 标记的 GSH、BLG 和 OVA 标准品 (CH(3)(204)Hg-GSH、CH(3)(204)Hg-BLG 和 CH(3)(204)Hg-OVA) 证明了使用标记特异性同位素稀释电感耦合等离子体质谱法 (ICPMS) 进行绝对肽/蛋白质定量的可行性。基于 ICPMS 对 Hg 的准确和灵敏测定,GSH、BLG 和 OVA 的检测限可分别达到 45.4、45.4 和 15.1 pmol L(-1),这表明可以进行低丰度肽/蛋白质定量,同时还可以可靠地定量中等和高丰度的肽/蛋白质。

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