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Site-Specific Synthesis of Cysteine-Bridged Glycoproteins via Expressed Protein Glycoligation

机译:通过表达蛋白质缩斗特异性合成半胱氨酸桥糖蛋白

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摘要

Site-specific glycosylation of a functional recombinant protein thioester is reported. The thioester functionalized protein sfGFP-Y151ThioD, prepared by genetic code expansion, underwent native chemical ligation with the cysteine-conjugated glycans H-Cys-NH-GIcNAc and H-Cys-NH-(GlcNAc)(2)(Man)(3) to give the corresponding cysteine-bridged glycoproteins. The intact glycoproteins, which retained their fluorescence, were characterized by top-down mass spectrometry and gel electrophoresis. The bridging cysteine provided a convenient handle for affinity chromatography purification of the glycoproteins via a removable biotin tag. Given the influence that specific glycoforms can have on a protein's function, the ability to attach a homogeneous glycan to an intact protein in a functional group controlled yet sequon-independent manner could find widespread application. These preliminary results set the stage for development of the expressed protein glycoligation (EPG) concept.
机译:报道了官能重组蛋白酯的特异性糖基化。 通过遗传代码扩张制备的硫酯官能化蛋白SFGFP-Y151周期,用半胱氨酸 - 缀合的聚糖H-Cys-NH-Gicnac和H-Cys-NH-(GlcNAc)(2)(3)(3) 给予相应的半胱氨酸桥糖蛋白。 保留其荧光的完整糖蛋白,其特征在于通过自上而下的质谱和凝胶电泳。 桥接半胱氨酸提供了通过可去除的生物素标签的亲和色谱纯化糖蛋白的亲和层析纯化。 鉴于特定糖型可以对蛋白质的功能具有的影响,以官能团控制又激发的独立式方式将均质聚集剂与完整蛋白质附着到完整的蛋白质的能力可以找到广泛的应用。 这些初步结果设定了表达蛋白质糖精(EPG)概念的发展阶段。

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