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通过对糖肽富集、定量、质谱方法和数据分析策略的系统评估改进糖蛋白质组学分析工作流程

Improving Glycoproteomic Analysis Workflow by Systematic Evaluation of Glycopeptide Enrichment, Quantification, Mass Spectrometry Approach, and Data Analysis Strategies.

作者信息

Sun Zhenyu, Lih T Mamie, Woo Jongmin, Jiao Liyuan, Hu Yingwei, Wang Yuefan, Liu Hongyi, Zhang Hui

出版信息

Anal Chem. 2024 Dec 31;96(52):20481-20490. doi: 10.1021/acs.analchem.4c04466. Epub 2024 Dec 16.

DOI:10.1021/acs.analchem.4c04466
PMID:39679613
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12039365/
Abstract

Glycosylation is one of the most prevalent and crucial protein modifications. Quantitative site-specific characterization of glycosylation usually requires sophisticated intact glycopeptide analysis using glycoproteomics. Recent efforts have focused on the interrogation of intact glycopeptide analyses using tandem mass spectrometry. However, a systematic evaluation of the quantitative glycoproteomic workflow is still lacking. This study compared different strategies for glycopeptide enrichment alongside glycopeptide quantitation, as well as mass spectrometry and data analysis strategies, providing a comprehensive assessment of their efficacy. The ZIC-HILIC enrichment method demonstrated superior performance, representing a 26% improvement in identified glycopeptiudes compared to the MAX enrichment method. Quantification using TMT provided high precision and throughput with an average CV of 8%. Through systematic evaluation, this study established that the ZIC-HILIC enrichment method, quantification with TMT, and collision energies of 25, 35, and 45 using tandem mass spectrometry are the optimal workflow for higher-energy collisional dissociation (HCD) fragmentation, significantly enhancing the analysis of intact glycopeptides. Precise energy adjustment is crucial for the identification of certain glycans. Intact glycopeptides were analyzed using different software tools to investigate the identification and quantification of glycopeptides. By applying optimal settings, 5514 unique intact glycopeptides were in luminal and basal patient-derived xenograft (PDX) characterized models, highlighting distinct glycosylation profiles that may influence tumor behavior. This study offers a systematic approach to evaluate glycoproteomic analysis workflow.

摘要

糖基化是最普遍且关键的蛋白质修饰之一。糖基化的定量位点特异性表征通常需要使用糖蛋白质组学进行复杂的完整糖肽分析。近期的工作重点是利用串联质谱对完整糖肽分析进行探究。然而,目前仍缺乏对定量糖蛋白质组学工作流程的系统评估。本研究比较了糖肽富集以及糖肽定量的不同策略,以及质谱和数据分析策略,对它们的功效进行了全面评估。ZIC-HILIC富集方法表现出卓越的性能,与MAX富集方法相比,鉴定出的糖肽数量提高了26%。使用TMT进行定量提供了高精度和高通量,平均变异系数为8%。通过系统评估,本研究确定ZIC-HILIC富集方法、TMT定量以及串联质谱中25、35和45的碰撞能量是用于高能碰撞解离(HCD)碎裂的最佳工作流程,显著增强了对完整糖肽的分析。精确的能量调整对于某些聚糖的鉴定至关重要。使用不同的软件工具对完整糖肽进行分析,以研究糖肽的鉴定和定量。通过应用最佳设置,在管腔和基底患者来源异种移植(PDX)特征模型中鉴定出5514种独特的完整糖肽,突出了可能影响肿瘤行为的不同糖基化谱。本研究提供了一种评估糖蛋白质组学分析工作流程的系统方法。

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本文引用的文献

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Maximal performance of intact N-glycopeptide enrichment using sequential HILIC and MAX columns.使用顺序 HILIC 和 MAX 柱实现完整 N-糖肽富集的最大性能。
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