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通过傅里叶变换质谱法对高质量分子进行基质辅助激光解吸/电离

Matrix-assisted laser desorption/ionization of high-mass molecules by Fourier-transform mass spectrometry.

作者信息

Castro J A, Köster C, Wilkins C

机构信息

Department of Chemistry, University of California Riverside 92521.

出版信息

Rapid Commun Mass Spectrom. 1992 Apr;6(4):239-41. doi: 10.1002/rcm.1290060403.

DOI:10.1002/rcm.1290060403
PMID:1315178
Abstract

Following the first demonstrations of high-mass analysis using time-of-flight matrix-assisted laser desorption/ionization (MALDI) techniques by Hillenkamp, Tanaka and their co-workers, there have been significant efforts in a number of laboratories to adapt the new methodology to Fourier-transform mass spectrometry (FTMS). The motivation for this research is obvious. Namely, it would be desirable to couple the unparalleled high mass resolution of FTMS with the extended mass range provided by MALDI, particularly for analysis of polymers and biomolecules. Unfortunately, prior to the present work, attempts to mate FTMS and MALDI have met with limited success. The highest mass matrix-assisted laser-desorption-FTMS result previously obtained appears to be the unpublished low resolution spectrum of bovine insulin recently reported by Russell and co-workers. We, Campana and co-workers, and Hettich and Buchanan have had some success with MALDI-FTMS of biomolecules with masses lower than 3000 Da, including melittin, a variety of lower mass peptides, and oligonucleotides with masses lower than 1800 Da. Furthermore, with the single exception of Campana's report of obtaining mass resolution of 5000 for the molecular ion of melittin, such spectra have not displayed high resolution. Here, we report successful development of MALDI-FTMS, demonstrated with spectra obtained from a variety of high-mass polymer and biomolecule samples, using 355 nm radiation from an excimer-pumped dye laser for desorption/ionization and sinapinic acid as matrix. Some of these spectra are of much higher mass resolution than is possible with current time-of flight mass spectrometers.

摘要

在Hillenkamp、田中及其同事首次展示使用飞行时间基质辅助激光解吸/电离(MALDI)技术进行高质量分析之后,许多实验室付出了巨大努力,试图将这种新方法应用于傅里叶变换质谱(FTMS)。这项研究的动机显而易见。也就是说,将FTMS无与伦比的高质量分辨率与MALDI提供的扩展质量范围相结合是很有必要的,特别是对于聚合物和生物分子的分析。不幸的是,在本研究之前,将FTMS与MALDI结合的尝试取得的成功有限。此前获得的最高质量的基质辅助激光解吸-FTMS结果似乎是Russell及其同事最近报道的未发表的牛胰岛素低分辨率光谱。我们、Campana及其同事,以及Hettich和Buchanan在对质量低于3000 Da的生物分子进行MALDI-FTMS分析方面取得了一些成功,这些生物分子包括蜂毒肽、各种低质量肽以及质量低于1800 Da的寡核苷酸。此外,除了Campana报道的蜂毒肽分子离子的质量分辨率达到5000之外,这类光谱都没有显示出高分辨率。在此,我们报告了MALDI-FTMS的成功开发,通过从受准分子泵浦的染料激光获得的355 nm辐射进行解吸/电离,并使用芥子酸作为基质,从各种高质量聚合物和生物分子样品获得的光谱证明了这一点。其中一些光谱的质量分辨率比当前的飞行时间质谱仪所能达到的要高得多。

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