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使用[12C]/[13C]苯胺和ZIC-HILIC-ESI-TOF-MS对酶解释放的N-聚糖进行稳定同位素标记,以实现糖基化变体的相对定量。

Relative quantitation of glycosylation variants by stable isotope labeling of enzymatically released N-glycans using [12C]/[13C] aniline and ZIC-HILIC-ESI-TOF-MS.

作者信息

Giménez Estela, Sanz-Nebot Victòria, Rizzi Andreas

机构信息

Department of Analytical Chemistry, University of Barcelona, Diagonal 647, 08028, Barcelona, Spain.

出版信息

Anal Bioanal Chem. 2013 Sep;405(23):7307-19. doi: 10.1007/s00216-013-7178-5. Epub 2013 Jul 12.

DOI:10.1007/s00216-013-7178-5
PMID:23846592
Abstract

Glycan reductive isotope labeling (GRIL) using [(12)C]- and [(13)C]-coded aniline was used for relative quantitation of N-glycans. In a first step, the labeling method by reductive amination was optimized for this reagent. It could be demonstrated that selecting aniline as limiting reactant and using the reductant in excess is critical for achieving high derivatization yields (over 95 %) and good reproducibility (relative standard deviations ∼1-5 % for major and ∼5-10 % for minor N-glycans). In a second step, zwitterionic-hydrophilic interaction liquid chromatography in capillary columns coupled to electrospray mass spectrometry with time-of-flight analyzer (μZIC-HILIC-ESI-TOF-MS) was applied for the analysis of labeled N-glycans released from intact glycoproteins. Ovalbumin, bovine α1-acid-glycoprotein and bovine fetuin were used as test glycoproteins to establish and evaluate the methodology. Excellent separation of isomeric N-glycans and reproducible quantitation via the extracted ion chromatograms indicate a great potential of the proposed methodology for glycoproteomic analysis and for reliable relative quantitation of glycosylation variants in biological samples.

摘要

使用[(12)C]和[(13)C]编码的苯胺进行聚糖还原同位素标记(GRIL)用于N-聚糖的相对定量。第一步,针对该试剂优化了还原胺化标记方法。结果表明,选择苯胺作为限量反应物并过量使用还原剂对于实现高衍生化产率(超过95%)和良好的重现性(主要N-聚糖的相对标准偏差约为1-5%,次要N-聚糖的相对标准偏差约为5-10%)至关重要。第二步,将毛细管柱中的两性离子亲水相互作用液相色谱与带飞行时间分析仪的电喷雾质谱联用(μZIC-HILIC-ESI-TOF-MS)用于分析从完整糖蛋白释放的标记N-聚糖。卵清蛋白、牛α1-酸性糖蛋白和牛胎球蛋白用作测试糖蛋白以建立和评估该方法。通过提取离子色谱图对异构体N-聚糖进行了出色的分离和可重现的定量,表明该方法在糖蛋白质组分析以及生物样品中糖基化变体的可靠相对定量方面具有巨大潜力。

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