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使用高分辨率质谱对鸟枪法蛋白质组学数据集进行高速数据缩减、特征检测和串联质谱(MS/MS)谱图质量评估。

High-speed data reduction, feature detection, and MS/MS spectrum quality assessment of shotgun proteomics data sets using high-resolution mass spectrometry.

作者信息

Hoopmann Michael R, Finney Gregory L, MacCoss Michael J

机构信息

Department of Genome Sciences, University of Washington, Seattle, Washington 98195, USA.

出版信息

Anal Chem. 2007 Aug 1;79(15):5620-32. doi: 10.1021/ac0700833. Epub 2007 Jun 21.

Abstract

Advances in Fourier transform mass spectrometry have made the acquisition of high-resolution and accurate mass measurements routine on a chromatographic time scale. Here we report an algorithm, Hardklör, for the rapid and robust analysis of high-resolution mass spectra acquired in shotgun proteomics experiments. Our algorithm is demonstrated in the analysis of an Escherichia coli enriched membrane fraction. The mass spectrometry data of the respective peptides are acquired by microcapillary HPLC on an LTQ-orbitrap mass spectrometer with data-dependent acquisition of MS/MS spectra. Hardklör detects 211,272 total peptide isotope distributions over a 2-h analysis (75-min gradient) in only a small fraction of the time required to acquire the data. From these data there are 13,665 distinct, chromatographically persistent peptide isotope distributions. Hardklör is also used to assess the quality of the product ion spectra and finds that more than 11.2% of the MS/MS spectra are composed of fragment ions from multiple different molecular species. Additionally, a method is reported that enzymatically labels N-linked glycosylation sites on proteins, creating a unique isotope signature that can be detected with Hardklör. Using the protein invertase, Hardklör identifies 18O-labeled peptide isotope distributions of four glycosylation sites. The speed and robustness of the algorithm create a versatile tool that can be used in many different areas of mass spectrometry data analysis.

摘要

傅里叶变换质谱技术的进步使得在色谱时间尺度上进行高分辨率和精确质量测量成为常规操作。在此,我们报告一种名为Hardklör的算法,用于快速、稳健地分析鸟枪法蛋白质组学实验中获取的高分辨率质谱图。我们的算法在对大肠杆菌富集膜组分的分析中得到了验证。各个肽段的质谱数据通过微毛细管高效液相色谱在LTQ-轨道阱质谱仪上采集,并采用数据依赖型采集方式获取串联质谱(MS/MS)谱图。Hardklör在仅一小部分采集数据所需的时间内,就能在2小时的分析(75分钟梯度)中检测到211,272个总肽段同位素分布。从这些数据中,有13,665个不同的、色谱上持续存在的肽段同位素分布。Hardklör还用于评估产物离子谱的质量,发现超过11.2%的MS/MS谱由来自多个不同分子物种的碎片离子组成。此外,还报告了一种方法,该方法通过酶促标记蛋白质上的N-连接糖基化位点,产生一种独特的同位素特征,可被Hardklör检测到。利用蛋白质转化酶,Hardklör识别出四个糖基化位点的18O标记肽段同位素分布。该算法的速度和稳健性创造了一种通用工具,可用于质谱数据分析的许多不同领域。

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