Chemoenzymatic synthesis of human natural killer-1-containing glycans and application as serum antibodies probes

聚糖 低聚糖 表位 抗体 化学 糖基 单克隆抗体 生物化学 唾液酸 糖蛋白 生物 免疫学
作者
Mehman Bunyatov,Margreet A. Wolfert,Lin Liu,Ruth Huizinga,Marco W.J. Schreurs,Bart C. Jacobs,Geert‐Jan Boons
出处
期刊:Nature Synthesis [Springer Nature]
卷期号:3 (1): 85-98 被引量:8
标识
DOI:10.1038/s44160-023-00394-4
摘要

Despite the versatility of enzyme-mediated oligosaccharide assembly, it has as a limitation that not all glycosyl transferases or glycan-modifying enzymes are readily available to install all natural occurring terminal epitopes. Here a chemoenzymatic strategy is described in which a core oligosaccharide is assembled enzymatically that is subjected to chemical manipulations to install complex terminal epitopes. It provided an unprecedented panel of human natural killer-1 (HSO3–3GlcAβ1–3Galβ1–4GlcNAc)-containing oligosaccharides and derivatives thereof. The compounds were printed as a microarray to examine binding specificities of serum antibodies of patients suffering from anti-myelin-associated glycoprotein neuropathy. All samples required glucuronic acid for antibody binding; however, variable dependence was observed for the length of the LacNAc chain and sulfation of glucuronic acid. Most serum samples required a lacto-neohexaose backbone indicating glycosphingolipids are being targeted. The clinical spectrum of immunoglobulin M monoclonal gammopathy varies, and the glycan microarray provides a more reliable platform for disease diagnosis and prognosis. While enzyme-mediated oligosaccharide synthesis is versatile, it is often limited by the availability of glycosyl transferases. Now a chemoenzymatic strategy is reported, comprising enzymatic assembly of a core oligosaccharide followed by chemical manipulations, to produce a library of glycans that reveal binding specificities of serum antibodies.
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