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Characterization of gel-separated glycoproteins using two-step proteolytic digestion combined with sequential microcolumns and mass spectrometry

机译:凝胶分离的糖蛋白的表征,采用两步蛋白水解消化结合顺序微柱和质谱

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摘要

Protein glycosylation can be vital for changing the function or physiochemical properties of a protein. Abnormal glycosylation can lead to protein malfunction, resulting in severe diseases. Therefore, it is important to develop techniques for characterization of such modifications in proteins at a sensitivity level comparable with state-of-the-art proteomics. Whereas techniques exist for characterization of high abundance glycoproteins, no single method is presently capable of providing information on both site occupancy and glycan structure on a single band excised from an electrophoretic gel. We present a new technique that allows characterization of low amounts of glycoproteins separated by gel electrophoresis. The method takes advantage of sequential specific and nonspecific enzymatic treatment followed by selective purification and characterization of the glycopeptides using graphite powder microcolumns in combination with mass spectrometry. The method is faster and more sensitive than previous approaches and is compatible with proteomic studies.
机译:蛋白质糖基化对于改变蛋白质的功能或理化特性至关重要。糖基化异常会导致蛋白质功能异常,从而导致严重疾病。因此,重要的是开发用于以与现有蛋白质组学相当的灵敏度水平表征蛋白质中此类修饰的技术。尽管存在用于表征高丰度糖蛋白的技术,但是目前尚无一种方法能够提供从电泳凝胶上切下来的单条带上的位点占有率和聚糖结构的信息。我们提出了一种新技术,该技术可以表征通过凝胶电泳分离的少量糖蛋白。该方法利用顺序特异性和非特异性酶处理的优势,随后使用石墨粉末微柱结合质谱对糖肽进行选择性纯化和表征。该方法比以前的方法更快,更灵敏,并且与蛋白质组学研究兼容。

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