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用荧光素标记的岩藻糖检测岩藻糖基转移酶的底物糖,并介绍糖电泳的方法。

Detecting substrate glycans of fucosyltransferases with fluorophore-conjugated fucose and methods for glycan electrophoresis.

机构信息

Bio-techne, R&D Systems, Inc., 614 McKinley Place N.E., Minneapolis, MN 55413, USA.

出版信息

Glycobiology. 2020 Dec 9;30(12):970-980. doi: 10.1093/glycob/cwaa030.

Abstract

Like sialylation, fucose usually locates at the nonreducing ends of various glycans on glycoproteins and constitutes important glycan epitopes. Detecting the substrate glycans of fucosyltransferases is important for understanding how these glycan epitopes are regulated in response to different growth conditions and external stimuli. Here we report the detection of these glycans on glycoproteins as well as in their free forms via enzymatic incorporation of fluorophore-conjugated fucose using FUT2, FUT6, FUT7, FUT8 and FUT9. Specifically, we describe the detection of the substrate glycans of these enzymes on fetal bovine fetuin, recombinant H1N1 viral neuraminidase and therapeutic antibodies. The detected glycans include complex and high-mannose N-glycans. By establishing a series of precursors for the synthesis of Lewis X and sialyl Lewis X structures, we not only provide convenient electrophoresis methods for studying glycosylation but also demonstrate the substrate specificities and some kinetic features of these enzymes. Our results support the notion that fucosyltransferases are key targets for regulating the synthesis of Lewis X and sialyl Lewis X structures.

摘要

与唾液酸化一样,岩藻糖通常位于糖蛋白上各种聚糖的非还原末端,并构成重要的聚糖表位。检测岩藻糖基转移酶的底物糖对于了解这些糖基表位如何响应不同的生长条件和外部刺激而受到调节非常重要。在这里,我们通过使用 FUT2、FUT6、FUT7、FUT8 和 FUT9 将荧光素缀合的岩藻糖酶促掺入到糖蛋白及其游离形式中来报告这些糖的检测。具体而言,我们描述了这些酶在胎牛胎球蛋白、重组 H1N1 病毒神经氨酸酶和治疗性抗体上的底物糖的检测。检测到的聚糖包括复杂的和高甘露糖 N-聚糖。通过建立一系列用于合成 Lewis X 和唾液酸化 Lewis X 结构的前体,我们不仅提供了用于研究糖基化的便利电泳方法,而且还证明了这些酶的底物特异性和一些动力学特征。我们的结果支持这样一种观点,即岩藻糖基转移酶是调节 Lewis X 和唾液酸化 Lewis X 结构合成的关键靶标。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4007/7724747/5514e2a90567/cwaa030f1.jpg

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