首页> 外文期刊>Journal of mass spectrometry: JMS >Peptide backbone fragmentation initiated by side-chain loss at cysteine residue in matrix-assisted laser desorption/ionization in-source decay mass spectrometry
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Peptide backbone fragmentation initiated by side-chain loss at cysteine residue in matrix-assisted laser desorption/ionization in-source decay mass spectrometry

机译:基质辅助激光解吸/电离源内衰减质谱法中半胱氨酸残基侧链损失引发的肽骨架断裂

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摘要

Matrix-assisted laser desorption/ionization in-source decay (MALDI-ISD) is initiated by hydrogen transfer from matrix molecules to the carbonyl oxygen of peptide backbone with subsequent radical-induced cleavage leading to c'/? fragments pair. MALDI-ISD is a very powerful method to obtain long sequence tags from proteins or to do de novo sequencing of peptides. Besides classical fragmentation, MALDI-ISD also shows specific fragments for which the mechanism of formation enlightened the MALDI-ISD process. In this study, the MALDI-ISD mechanism is reviewed, and a specific mechanism is studied in details: the N-terminal side of Cys residue (Xxx-Cys) is described to promote the generation of c' and w fragments in MALDI-ISD. Our data suggest that for sequences containing Xxx-Cys motifs, the N-C_α bond cleavage occurs following the hydrogen attachment to the thiol group of Cys side-chain. The ?/w fragments pair is formed by side-chain loss of the Cys residue with subsequent radical-induced cleavage at the N-C_α bond located at the left side (N-terminal direction) of the Cys residue. This fragmentation pathway preferentially occurs at free Cys residue and is suppressed when the cysteines are involved in disulfide bonds. Hydrogen attachment to alkylated Cys residues using iodoacetamide gives free Cys residue by the loss of ?CH_2CONH_2 radical. The presence of alkylated Cys residue also suppress the formation of ?/w fragments pair via the (C_β)-centered radical, whereas w fragment is still observed as intense signal. In this case, the ? fragment formed by hydrogen attachment of carbonyl oxygen followed side-chain loss at alkylated Cys leads to a w fragment. Hydrogen attachment on peptide backbone and side-chain of Cys residue occurs therefore competitively during MALDI-ISD process.
机译:基质辅助的激光解吸/电离源内衰减(MALDI-ISD)是通过将氢从基质分子转移到肽主链的羰基氧开始的,随后自由基诱导的裂解导致c'/?发生。片段对。 MALDI-ISD是一种非常强大的方法,可以从蛋白质中获得长序列标签或对肽进行从头测序。除经典片段化以外,MALDI-ISD还显示了特定的片段,其形成机理启发了MALDI-ISD过程。在这项研究中,对MALDI-ISD机理进行了综述,并详细研究了一种特殊的机理:描述了Cys残基(Xxx-Cys)的N端侧促进MALDI-ISD中c'和w片段的产生。我们的数据表明,对于含有Xxx-Cys基序的序列,N-C_α键裂解发生在氢附着到Cys侧链的硫醇基团之后。 α/ w片段对由Cys残基的侧链丢失和随后在Cys残基的左侧(N-末端方向)的N-C_α键的自由基诱导的切割形成。该片段化途径优先发生在游离的Cys残基上,并且当半胱氨酸参与二硫键时被抑制。使用碘乙酰胺将氢附着至烷基化的Cys残基,可通过丢失?CH_2CONH_2自由基获得游离的Cys残基。烷基化的Cys残基的存在也抑制了经由(C_β)中心的自由基形成的ω/ w片段对,而w片段仍被视为强信号。在这种情况下,?由羰基氧的氢连接形成的α片段,随后在烷基化的Cys上侧链损失,导致形成w片段。因此,在MALDI-ISD过程中竞争性地发生氢附着在肽主链和Cys残基的侧链上。

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