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Rapid De-O-Glycosylation Concomitant with Peptide Labeling Using Microwave Radiation and an Alkyl Amine Base

机译:快速脱O-糖基化与使用微波辐射和烷基胺碱进行肽标记

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摘要

Procedures are detailed for a quantitative release of O-linked glycans from peptides that now provide a shorter reaction time, a possible identification of O-linked sites, and a quantification of all reaction products. The release was initiated by a mild base, dimethylamine, and accelerated by microwave radiation. Differential analysis using standard glycoproteins has shown improved release efficiency concurrent with facile incorporation of dimethylamine into the former O-linked sites. In situ glycan reduction insures protection against peeling and is synchronous with subsequent studies by high performance MS~(n) sequencing. The protocols were established with a synthetic O-GlcNAc peptide that would mimic the linkage chemistry and applied to a well characterized glycoprotein bovine fetuin with both N- and O-linked glycans and a highly glycosylated swine mucin.
机译:详细介绍了从肽中定量释放O-连接聚糖的方法,该方法现在可以缩短反应时间,可能确定O-连接位点,并对所有反应产物进行定量。释放是由温和的碱二甲胺引发的,并通过微波辐射加速释放。使用标准糖蛋白进行的差异分析表明,在将二甲胺轻松掺入到以前的O-连接位点的同时,释放效率得到了提高。原位聚糖的减少确保了对脱皮的保护,并且与随后通过高性能MS〜(n)测序进行的研究同步。用合成的O-GlcNAc肽建立了该方案,该肽可模拟连接化学,并应用于具有N-和O-连接的聚糖以及高度糖基化的猪粘蛋白的特征明确的糖蛋白牛胎球蛋白。

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