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Derivatization with 1-pyrenyldiazomethane enhances ionization of glycopeptides but not peptides in matrix-assisted laser desorption/ionization mass spectrometry.1-芘基重氮甲烷衍生化增强了糖肽而不是肽在基质辅助激光解吸/电离质谱中的离子化。
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基质辅助激光解吸电离(MALDI)样品中糖肽的甜蜜点与基质晶体多态性之间的相关性

Correlation between Sweet Spots of Glycopeptides and Polymorphism of the Matrix Crystal in MALDI Samples.

作者信息

Nishikaze Takashi, Okumura Hisako, Jinmei Hiroshi, Amano Junko

机构信息

Laboratory of Glycobiology, The Noguchi Institute.

出版信息

Mass Spectrom (Tokyo). 2012;1(1):A0006. doi: 10.5702/massspectrometry.A0006. Epub 2012 Aug 28.

DOI:10.5702/massspectrometry.A0006
PMID:24349907
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3775826/
Abstract

A standard dried-droplet preparation using 2,5-dihydroxybenzoic acid (2,5-DHBA) as the matrix results in a large variation in signal intensity and poor shot-to-shot reproducibility in matrix-assisted laser desorption/ionization (MALDI). We expected that the differences can be attributed to the nature of the crystal structures in the region of the "sweet spot" within the MALDI samples. 2,5-DHBA crystals with and without analytes on a target plate obtained by means of a dried-droplet preparation contain two polymorphs, which can be distinguished by Raman spectra. In comparing the Raman image with the MS image, a clear correlation between the signal distribution of glycopeptides and hydrophilic peptides and the specific crystal form of 2,5-DHBA could be made. The ionization of hydrophobic peptides appears to proceed in both types of polymorphic crystals. In addition, the derivatization of glycopeptides with a pyrene group enabled us to detect glycopeptides regardless the crystal form. As the result, the number of sweet spots increased and MS spectra with a high signal intensity were obtained. The results suggest that the introduction of a hydrophobic/aromatic moiety to glycopeptides results in a more successful MALDI analysis due to the effective incorporation of the analyte into matrix crystals.

摘要

以2,5 -二羟基苯甲酸(2,5 - DHBA)为基质的标准干滴制备法,在基质辅助激光解吸/电离(MALDI)中会导致信号强度的大幅变化以及逐次进样的重现性较差。我们预期这些差异可归因于MALDI样品中“最佳点”区域内晶体结构的性质。通过干滴制备法在靶板上获得的含有和不含有分析物的2,5 - DHBA晶体包含两种多晶型物,可通过拉曼光谱加以区分。在将拉曼图像与质谱图像进行比较时,可以发现糖肽和亲水肽的信号分布与2,5 - DHBA的特定晶型之间存在明显的相关性。疏水性肽的电离似乎在两种多晶型晶体中均可发生。此外,用芘基团对糖肽进行衍生化使我们能够检测糖肽,而无需考虑晶体形式。结果,最佳点的数量增加了,并且获得了具有高信号强度的质谱图。结果表明,由于分析物有效地掺入基质晶体中,向糖肽中引入疏水/芳香部分会使MALDI分析更成功。