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稳定同位素标记的疏水性酰肼试剂用于电喷雾电离质谱法相对定量 N-连接聚糖。

Stable-isotope labeled hydrophobic hydrazide reagents for the relative quantification of N-linked glycans by electrospray ionization mass spectrometry.

机构信息

W. M. Keck FT-ICR Mass Spectrometry Laboratory, North Carolina State University, Raleigh, North Carolina 27695, USA.

出版信息

Anal Chem. 2011 Sep 1;83(17):6738-45. doi: 10.1021/ac201376q. Epub 2011 Aug 1.

Abstract

This study presents the development of stable-isotope labeled hydrophobic, hydrazide reagents for the relative quantification of N-linked glycans. The P2GPN "light" ((12)C) and "heavy" ((13)C(6)) pair are used to differentially label two N-linked glycan samples. The samples are combined 1:1, separated using HILIC, and then mass differentiated and quantified using mass spectrometry. These reagents have several benefits: (1) impart hydrophobic character to the glycans affording an increase in electrospray ionization efficiency and MS detection; (2) indistinguishable chromatographic, MS, and MS/MS performance of the "light" and "heavy" reagents affording relative quantification; and (3) analytical variability is significantly reduced due to the two samples being mixed together after sample preparation. Obtaining these analytical benefits only requires ~4 h of sample preparation time. It is shown that these reagents are capable of quantifying changes in glycosylation in simple mixtures, and the analytical variability of the reagents in pooled plasma samples is shown to be less than ±30%. Additionally, the incorporation of an internal standard allows one to account for the difference in systematic error between the two samples due to the samples being processed in parallel and not mixed until after derivatization.

摘要

本研究开发了稳定同位素标记的疏水、酰肼试剂,用于相对定量分析 N 连接聚糖。使用 P2GPN“轻”((12)C)和“重”((13)C(6))对来分别标记两种 N 连接聚糖样品。将样品以 1:1 的比例混合,使用亲水相互作用色谱法(HILIC)分离,然后通过质谱法进行质量差异和定量分析。这些试剂具有以下几个优点:(1)赋予聚糖疏水性,提高电喷雾电离效率和 MS 检测;(2)“轻”和“重”试剂的色谱、MS 和 MS/MS 性能完全相同,可进行相对定量;(3)由于样品制备后混合在一起,分析变异性显著降低。仅需约 4 小时的样品制备时间即可获得这些分析优势。结果表明,这些试剂能够定量分析简单混合物中的糖基化变化,并且在混合血浆样品中,试剂的分析变异性小于±30%。此外,通过加入内标,可以考虑到由于样品平行处理而导致的两个样品之间系统误差的差异,直到衍生化后才混合。

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