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使用蛋白质溶液作为解吸电喷雾电离质谱中的喷雾液对非挥发性分析物进行灵敏的离子化。

Sensitive ionization of non-volatile analytes using protein solutions as spray liquid in desorption electrospray ionization mass spectrometry.

机构信息

Jiangxi Key Laboratory for Mass Spectrometry and Instrumentation, East China Institute of Technology, Nanchang, Jiangxi Province, 330013, PR China.

出版信息

Rapid Commun Mass Spectrom. 2012 Dec 15;26(23):2770-6. doi: 10.1002/rcm.6387.

DOI:10.1002/rcm.6387
PMID:23124668
Abstract

RATIONALE

Desorption electrospray ionization (DESI) is the most popular ambient ionization technique for direct analysis of complex samples without sample pretreatment. However, for many applications, especially for trace analysis, it is of interest to improve the sensitivity of DESI-mass spectrometry (MS).

METHODS

In traditional DESI-MS, a mixture of methanol/water/acetic acid is usually used to generate the primary ions. In this article, dilute protein solutions were electrosprayed in the DESI method to create multiply charged primary ions for the desorption ionization of trace analytes on various surfaces (e.g., filter paper, glass, Al-foil) without any sample pretreatment. The analyte ions were then detected and structurally characterized using a LTQ XL mass spectrometer.

RESULTS

Compared with the methanol/water/acetic acid (49:49:2, v/v/v) solution, protein solutions significantly increased the signal levels of non-volatile compounds such as benzoic acid, TNT, o-toluidine, peptide and insulin in either positive or negative ion detection mode. For all the analytes tested, the limits of detection (LODs) were reduced to about half of the original values which were obtained using traditional DESI. The results showed that the signal enhancement is highly correlated with the molecular weight of the proteins and the selected solid surfaces.

CONCLUSIONS

The proposed DESI method is a universal strategy for rapid and sensitive detection of trace amounts of strongly bound and/or non-volatile analytes, including explosives, peptides, and proteins. The results indicate that the sensitivity of DESI can be further improved by selecting larger proteins and appropriate solid surfaces.

摘要

原理

解吸电喷雾电离(DESI)是最流行的无需样品预处理即可直接分析复杂样品的环境离子化技术。然而,对于许多应用,特别是痕量分析,提高 DESI-质谱(MS)的灵敏度是很有意义的。

方法

在传统的 DESI-MS 中,通常使用甲醇/水/乙酸的混合物来产生初级离子。在本文中,将稀释的蛋白质溶液在 DESI 方法中进行电喷雾,以在没有任何样品预处理的情况下,在各种表面(例如滤纸、玻璃、铝箔)上产生用于痕量分析物解吸电离的多电荷初级离子。然后使用 LTQ XL 质谱仪对分析物离子进行检测和结构表征。

结果

与甲醇/水/乙酸(49:49:2,v/v/v)溶液相比,蛋白质溶液显著提高了非挥发性化合物(如苯甲酸、TNT、邻甲苯胺、肽和胰岛素)的信号水平,无论是正离子检测模式还是负离子检测模式。对于所有测试的分析物,检测限(LOD)降低到使用传统 DESI 获得的原始值的约一半。结果表明,信号增强与蛋白质的分子量和所选固体表面高度相关。

结论

所提出的 DESI 方法是一种快速、灵敏检测痕量强结合和/或非挥发性分析物(包括爆炸物、肽和蛋白质)的通用策略。结果表明,通过选择较大的蛋白质和适当的固体表面,可以进一步提高 DESI 的灵敏度。

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