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Chromogenic Chemical Probe for Protein Structural Characterization via Ultraviolet Photodissociation Mass Spectrometry

机译:用于紫外光解离质谱分析蛋白质结构特征的生色化学探针

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摘要

A chemical probe/ultraviolet photodissociation (UVPD) mass spectrometry strategy for evaluating structures of proteins and protein complexes is reported, as demonstrated for lysozyme and beta-lactoglobulin with and without bound ligands. The chemical probe, NN, incorporates a UV chromophore that endows peptides with high cross sections at 351 nm, a wavelength not absorbed by unmodified peptides. Thus, NN-modified peptides can readily be differentiated from nonmodified peptides in complex tryptic digests created upon proteolysis of proteins after their exposure to the NN chemical probe. The NN chemical probe also affords two diagnostic reporter ions detected upon UVPD of the NN-modified peptide that provides a facile method for the identification of NN peptides within complex mixtures. Quantitation of the modified and unmodified peptides allows estimation of the surface accessibilities of lysine residues based on their relative reactivities with the NN chemical probe.
机译:已报道了用于评估蛋白质和蛋白质复合物结构的化学探针/紫外光解离(UVPD)质谱策略,已证明溶菌酶和β-乳球蛋白有或没有结合的配体。化学探针NN掺入了一种紫外线发色团,该发色团赋予了351 nm高横截面的肽,该波长未被未修饰的肽吸收。因此,在蛋白质暴露于NN化学探针后通过蛋白水解产生的复杂胰蛋白酶消化物中,NN修饰的肽可以很容易地与未修饰的肽区分开。 NN化学探针还提供了NN修饰肽的UVPD后检测到的两个诊断报告离子,为鉴定复杂混合物中的NN肽提供了一种简便的方法。修饰的和未修饰的肽的定量允许基于其与NN化学探针的相对反应性来估计赖氨酸残基的表面可及性。

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