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选择性 351nm 光解半胱氨酸肽,用于区分 IgG 片段在自上而下的液相色谱-串联质谱工作流程中的抗原结合区域。

Selective 351 nm photodissociation of cysteine-containing peptides for discrimination of antigen-binding regions of IgG fragments in bottom-up liquid chromatography-tandem mass spectrometry workflows.

机构信息

Department of Chemistry and Biochemistry, The University of Texas at Austin, 1 University Station A5300, Austin, TX 78712, USA.

出版信息

Anal Chem. 2013 Jun 4;85(11):5577-85. doi: 10.1021/ac400851x. Epub 2013 May 16.

Abstract

Despite tremendous inroads in the development of more sensitive liquid chromatography-tandem mass spectrometry (LC-MS/MS) strategies for mass spectrometry-based proteomics, there remains a significant need for enhancing the selectivity of MS/MS-based workflows for streamlined analysis of complex biological mixtures. Here, a novel LC-MS/MS platform based on 351 nm ultraviolet photodissociation (UVPD) is presented for the selective analysis of cysteine-peptide subsets in complex protein digests. Cysteine-selective UVPD is mediated through the site-specific conjugation of reduced cysteine residues with a 351 nm active chromogenic Alexa Fluor 350 (AF350) maleimide tag. Only peptides containing the AF350 chromophore undergo photodissociation into extensive arrays of b- and y-type fragment ions, thus providing a facile means for differentiating cysteine-peptide targets from convoluting peptide backgrounds. With the use of this approach in addition to strategic proteolysis, the selective analysis of diagnostic heavy-chain complementarity determining regions (CDRs) of single-chain antibody (scAb) fragments is demonstrated.

摘要

尽管在开发更灵敏的基于液相色谱-串联质谱(LC-MS/MS)的策略方面取得了巨大进展,用于基于质谱的蛋白质组学,但仍然需要显著提高基于 MS/MS 的工作流程的选择性,以实现对复杂生物混合物的简化分析。在这里,提出了一种基于 351nm 紫外光解(UVPD)的新型 LC-MS/MS 平台,用于选择性分析复杂蛋白质消化物中的半胱氨酸肽亚组。通过将还原半胱氨酸残基与 351nm 活性生色 Alexa Fluor 350(AF350)马来酰亚胺标签进行特异性缀合,实现半胱氨酸选择性 UVPD。只有含有 AF350 生色团的肽经历光解,形成广泛的 b-和 y-型片段离子,从而提供了一种从复杂的肽背景中区分半胱氨酸肽靶标的简便方法。通过使用这种方法以及策略性蛋白水解,可以选择性分析单链抗体(scAb)片段的诊断重链互补决定区(CDRs)。

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