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Ultraviolet Photodissociation for Characterizationof Whole Proteins on a Chromatographic Time Scale

机译:紫外光解离用于表征蛋白质在色谱时间尺度上的分布

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摘要

Intact protein characterization using mass spectrometry thus far has been achieved at the cost of throughput. Presented here is the application of 193 nm ultraviolet photodissociation (UVPD) for top down identification and characterization of proteins in complex mixtures in an online fashion. Liquid chromatographic separation at the intact protein level coupled with fast UVPD and high-resolution detection resulted in confident identification of 46 unique sequences compared to 44 using HCD from prepared Escherichia coli ribosomes. Importantly, nearly all proteins identified in both the UVPD and optimized HCD analyses demonstrated a substantial increase in confidence in identification (as defined by an average decrease in E value of ∼40 orders of magnitude) due to the higher number of matched fragment ions. Also shown is the potential for high-throughput characterization of intact proteins via liquid chromatography (LC)–UVPD-MS of molecular weight-based fractions of a Saccharomyces cerevisiae lysate. In total, protein products from 215 genes were identified and found in 292 distinct proteoforms, 168 of which contained some type of post-translational modification.
机译:迄今为止,已经以使用质谱法完成了完整的蛋白质表征,但是却以通量为代价。此处介绍的是193 nm紫外光解离(UVPD)在网上以自上而下的方式识别和表征复杂混合物中蛋白质的应用。使用完整的蛋白质水平进行液相色谱分离,再加上快速的UVPD和高分辨率检测,可以确定地鉴定出46个独特的序列,而使用HCD从制备的大肠杆菌核糖体中鉴定出的独特序列为44个。重要的是,由于匹配的碎片离子数量增加,几乎所有在UVPD分析和优化的HCD分析中鉴定出的蛋白质都显示出鉴定可信度的大幅提高(定义为E值平均降低约40个数量级)。还显示了通过液相色谱(LC)–酿酒酵母裂解物基于分子量的馏分的UVPD-MS对完整蛋白进行高通量表征的潜力。总共鉴定出来自215个基因的蛋白质产物,并在292种不同的蛋白形式中发现,其中168种包含某种类型的翻译后修饰。

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