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在色谱时间尺度上对全蛋白质进行特征分析的紫外线光解。

Ultraviolet photodissociation for characterization of whole proteins on a chromatographic time scale.

机构信息

Department of Chemistry, University of Texas at Austin , 1 University Station A5300, Austin, Texas 78712, United States.

出版信息

Anal Chem. 2014 Feb 18;86(4):2185-92. doi: 10.1021/ac403859a. Epub 2014 Jan 29.

Abstract

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.

摘要

目前,使用质谱技术对完整蛋白质进行特征分析的方法虽然已经成熟,但在通量方面仍存在一些限制。本研究介绍了一种新的方法,即使用 193nm 紫外光解(UVPD)在线分析复杂混合物中的蛋白质,实现从顶部到底部的鉴定和特征分析。在完整蛋白质水平上进行液相色谱分离,结合快速 UVPD 和高分辨率检测,可以对 46 个独特的序列进行可靠鉴定,而使用 HCD 则只能鉴定出 44 个序列。重要的是,与优化的 HCD 分析相比,UVPD 和优化的 HCD 分析鉴定的几乎所有蛋白质的鉴定置信度都有了显著提高(定义为平均 E 值降低了约 40 个数量级),这是因为匹配的片段离子数量增加了。本研究还展示了通过对酿酒酵母裂解物的分子量基分数进行液相色谱(LC)-UVPD-MS 分析,实现高通量完整蛋白质特征分析的潜力。总共鉴定到来自 215 个基因的蛋白质产物,并发现了 292 种不同的蛋白形式,其中 168 种含有某种类型的翻译后修饰。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/450c/3958131/959699474141/ac-2013-03859a_0002.jpg

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