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一种通过选择的电子转移反应监测进行定量肽分析的新方法。

A novel approach for quantitative peptides analysis by selected electron transfer reaction monitoring.

机构信息

Institute of Molecular Biology, National Chung Hsing University, Taichung, Taiwan.

出版信息

J Chromatogr A. 2010 Oct 29;1217(44):6927-31. doi: 10.1016/j.chroma.2010.08.068. Epub 2010 Sep 17.

DOI:10.1016/j.chroma.2010.08.068
PMID:20850119
Abstract

Liquid chromatography coupled to tandem mass spectrometry (LC-MS/MS) with selective reaction monitoring (SRM) is a selective and sensitive method for quantitation of peptides. SRM is achieved via MS/MS utilizing collision-induced dissociation (CID) while monitoring unique precursor-product ion transitions. Low-energy CID tandem mass spectrometry has been, by far, the most common method used to dissociate peptide ions for sequence analysis. However, collisional scattering of product ions in CID results in decreased intensity of the primary product ion. The lower intensity of the targeted product ion can lead to a reduction in the sensitivity of a quantitative method that uses SRM. Electron transfer dissociation (ETD) is a fragmentation method that is complementary to CID. During the ETD reaction for doubly protonated peptides (M+2H), there is a significant shift toward nondissociative electron transfer (ET) product species (M+2H). We utilized that particular defect in ETD to develop a new quantitative method for monitoring the transition of unique precursors (M+2H) to charge-reduced ions (M+2H). We refer to this method as selective electron transfer reaction monitoring (SETRM). In ESI-MS, trypsin-digested peptides tend to generate doubly protonated peptide precursors. We found that SETRM was more suitable than SRM for these doubly charged tryptic peptides with nano-LC-MS/MS. The quantitative capabilities of SETRM provide a more sensitive way of performing quantitative experiments using the same instrument, thereby improving the application of electron transfer dissociation in proteomics.

摘要

液相色谱-串联质谱(LC-MS/MS)与选择反应监测(SRM)相结合,是一种定量分析肽类的选择性和灵敏性方法。通过 MS/MS 利用碰撞诱导解离(CID)实现 SRM,同时监测独特的前体-产物离子跃迁。到目前为止,低能 CID 串联质谱一直是用于肽离子序列分析的最常用方法。然而,CID 中产物离子的碰撞散射导致主要产物离子的强度降低。靶向产物离子的强度降低会导致使用 SRM 的定量方法的灵敏度降低。电子转移解离(ETD)是一种与 CID 互补的碎裂方法。对于双质子化肽(M+2H),在 ETD 反应过程中,非解离性电子转移(ET)产物物种([M+2H](+))的比例显著增加。我们利用 ETD 的这一特殊缺陷,开发了一种新的定量方法,用于监测独特前体(M+2H)向电荷减少离子([M+2H](+))的跃迁。我们将这种方法称为选择性电子转移反应监测(SETRM)。在 ESI-MS 中,胰蛋白酶消化的肽往往会生成双质子化的肽前体。我们发现,与 SRM 相比,SETRM 更适合于这些带双电荷的胰蛋白酶肽与纳升 LC-MS/MS 的联用。SETRM 的定量能力提供了一种更灵敏的方法,可在相同仪器上进行定量实验,从而提高了电子转移解离在蛋白质组学中的应用。

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