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Comparison of Three Glycoproteomic Methods for the Analysis of the Secretome of CHO Cells Treated with 134-

机译:三种糖蛋白方法对134-施用CHO细胞沉淀的三种糖蛋白方法的比较

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摘要

Comprehensive analysis of the glycoproteome is critical due to the importance of glycosylation to many aspects of protein function. The tremendous complexity of this post-translational modification, however, makes it difficult to adequately characterize the glycoproteome using any single method. To overcome this pitfall, in this report we compared three glycoproteomic analysis methods; first the recently developed N-linked glycans and glycosite-containing peptides (NGAG) chemoenzymatic method, second, solid-phase extraction of N-linked glycoproteins (SPEG), and third, hydrophilic interaction liquid chromatography (HILIC) by characterizing N-linked glycosites in the secretome of Chinese hamster ovary (CHO) cells. Interestingly, the glycosites identified by SPEG and HILIC overlapped considerably whereas NGAG identified many glycosites not observed in the other two methods. Further, utilizing enhanced intact glycopeptide identification afforded by the NGAG workflow, we found that the sugar analog 1,3,4-O-Bu3ManNAc, a “high flux” metabolic precursor for sialic acid biosynthesis, increased sialylation of secreted proteins including recombinant human erythropoietin (rhEPO).
机译:由于糖基化对蛋白质功能的许多方面的重要性,甘油膜综合分析至关重要。然而,这种翻译后修饰的巨大复杂性使得难以使用任何单一方法充分表征糖蛋白酶。为了克服这一陷阱,在本报告中,我们比较了三种糖蛋白分析方法;首先,最近开发的N-连接的聚糖和含甘甘油肽(NgAG)化学酶方法,第二,通过表征N-连接的综合血液复合材料,第二,固相提取N-连接的糖蛋白(SPEG)和第三,亲水相互作用液相色谱(HILIC)在中国仓鼠卵巢(CHO)细胞的秘书中。有趣的是,由Speg和HILIC鉴定的血糖含量大大重叠,而NGAG鉴定了在另外两种方法中未观察到的许多糖基。此外,利用由NgAG工作流程提供增强的完整糖肽鉴定,我们发现糖类似物1,3,4-O-Bu3mannAc,“高通量”代谢前体用于唾液酸生物合成,分泌蛋白质的唾液酸唾液化增加,包括重组人促红细胞生成素(rhepo)。

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