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MICROHETEROGENEITY OF ERYTHROPOIETIN CARBOHYDRATE STRUCTURE

机译:促红细胞生成素碳酸盐结构的微均质性

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The microheterogeneity of the carbohydrate structures on recombinant human erythropoietin (rHuEPO) expressed in Chinese hamster ovary cells has been evaluated by electrospray ionization (ESI) mass spectrometry (MS) of glycopeptide fragments. The microheterogeneity is largely associated with the presence or absence of terminal N-acetylneuraminic acid (Neu5Ac) residues, varying amounts of O-acetylation of the Neu5Ac residues, and the presence or absence of N-acetyllactosamine extensions. The N-linked carbohydrate structures were structurally diverse; 52 different N-linked oligosaccharide structures were identified. Consistent structural assignments could be made from data obtained using different proteolytic digests, ESI solvent systems (aqueous/methanol systems with acetic or formic acid), and on-line or off-line LC/MS analysis. All glycosylation sites exhibited some level of O-acetylation of Neu5Ac residues. Interestingly, glycosylation site asparagine-83 exhibits mono-O-acetyl and di-O-acetyl Neu5Ac residues, while the other sites, asparagine-24, asparagine-38, and serine-126, exhibit mainly mono-O-acetyl Neu5Ac derivatization. This difference in O-acetylation may be site specific or due to sample handling of labile structures, However, mild base treatment of rHuEPO with NaOH on ice removed the O-acetyl groups associated with a given carbohydrate structure, without adversely affecting the underlying oligosaccharide structure, resulting in a simplified mass spectra. Nuclear magnetic resonance spectroscopy of Neu5Ac residues released by neuraminidase treatment of total rHuEPO indicated that Neu5,9Ac2 residues were present, Additional resonances were also observed that were consistent with other Neu5Ac O-acetyl linkages; these O-acetyl resonances could be removed by mild base hydrolysis of rHuEPO.
机译:已通过糖肽片段的电喷雾电离(ESI)质谱(MS)评估了中国仓鼠卵巢细胞中表达的重组人促红细胞生成素(rHuEPO)上碳水化合物结构的微异质性。微异质性主要与存在或不存在末端N-乙酰神经氨酸(Neu5Ac)残基,Neu5Ac残基的O-乙酰化量不同以及是否存在N-乙酰基乳糖胺延伸有关。 N-连接的碳水化合物结构在结构上是多样的。鉴定出52种不同的N-连接的寡糖结构。可以使用不同的蛋白水解消化物,ESI溶剂系统(含乙酸或甲酸的水/甲醇系统)以及在线或离线LC / MS分析获得的数据进行一致的结构分配。所有糖基化位点均显示Neu5Ac残基的O-乙酰化水平。有趣的是,糖基化位点天冬酰胺83显示出单-O-乙酰基和二-O-乙酰基Neu5Ac残基,而其他位点,天冬酰胺24,天冬酰胺-38和丝氨酸-126,主要表现出单-O-乙酰基Neu5Ac衍生化。 O-乙酰化的这种差异可能是特定于位点的,或者是由于不稳定结构的样品处理所致。但是,在冰上用NaOH对rHuEPO进行温和的碱处理会除去与给定碳水化合物结构相关的O-乙酰基,而不会不利地影响潜在的低聚糖结构,从而简化了质谱图。神经氨酸酶处理的总rHuEPO释放的Neu5Ac残基的核磁共振波谱表明存在Neu5,9Ac2残基,还观察到与其他Neu5Ac O-乙酰基键合一致的共振。这些O-乙酰基共振可以通过rHuEPO的轻度碱水解而消除。

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