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缓激肽类似物的193纳米光解离与TOF-TOFMS分析的比较研究:电荷位点和碎裂时间尺度的影响

Comparative studies of 193-nm photodissociation and TOF-TOFMS analysis of bradykinin analogues: the effects of charge site(s) and fragmentation timescales.

作者信息

Morgan Joseph W, Russell David H

机构信息

Laboratory for Biological Mass Spectrometry, Department of Chemistry, Texas A and M University, College Station, Texas, USA.

出版信息

J Am Soc Mass Spectrom. 2006 May;17(5):721-9. doi: 10.1016/j.jasms.2006.02.004. Epub 2006 Mar 15.

DOI:10.1016/j.jasms.2006.02.004
PMID:16540342
Abstract

The dissociation reactions of [M + H]+, [M + Na]+, and [M + Cu]+ ions of bradykinin (amino acid sequence RPPGFSPFR) and three bradykinin analogues (RPPGF, RPPGFSPF, PPGFSPFR) are examined by using 193-nm photodissociation and post-source decay (PSD) TOF-TOF-MS techniques. The photodissociation apparatus is equipped with a biased activation cell, which allows us to detect fragment ions that are formed by dissociation of short-lived (<1 mus) photo-excited ions. In our previously reported photodissociation studies, the fragment ions were formed from ions dissociating with lifetimes that exceeded 10 mus; thus these earlier photofragment ion spectra and post-source decay (PSD) spectra [composite of both metastable ion (MI) and collision-induced dissociation (CID)] were quite similar. On the other hand, short-lived photo-excited ions dissociate by simple bond cleavage reactions and other high-energy dissociation channels. We also show that product ion types and abundances vary with the location of the charge on the peptide ion. For example, H+ and Na+ cations can bind to multiple polar functional groups (basic amino acid side chains) of the peptide, whereas Cu+ ions preferentially bind to the guanidino group of the arginine side-chain and the N-terminal amine group. Furthermore, when Cu+ is the charge carrier, the abundances of non-sequence informative ions, especially loss of small neutral molecules (H2O and NH3) is decreased for both photofragment ion and PSD spectra relative to that observed for [M + H]+ and [M + Na]+ peptide ions.

摘要

利用193纳米光解离和源后衰变(PSD)串联飞行时间质谱技术,研究了缓激肽(氨基酸序列为RPPGFSPFR)及其三种类似物(RPPGF、RPPGFSPF、PPGFSPFR)的[M + H]+、[M + Na]+和[M + Cu]+离子的解离反应。光解离装置配备了一个偏置激活池,这使我们能够检测由短寿命(<1微秒)光激发离子解离形成的碎片离子。在我们之前报道的光解离研究中,碎片离子是由寿命超过10微秒的解离离子形成的;因此,这些早期的光碎片离子光谱和源后衰变(PSD)光谱[亚稳离子(MI)和碰撞诱导解离(CID)的组合]非常相似。另一方面,短寿命的光激发离子通过简单的键断裂反应和其他高能解离通道解离。我们还表明,产物离子的类型和丰度随肽离子上电荷的位置而变化。例如,H+和Na+阳离子可以与肽的多个极性官能团(碱性氨基酸侧链)结合,而Cu+离子优先与精氨酸侧链的胍基和N端胺基结合。此外,当Cu+作为电荷载体时,相对于[M + H]+和[M + Na]+肽离子,光碎片离子光谱和PSD光谱中非序列信息离子的丰度,特别是小中性分子(H2O和NH3)的损失都减少了。

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