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结合增强的多磷酸盐激酶驱动的 UDP-葡萄糖再生系统与关键糖基转移酶的筛选以高效合成核苷二糖。

Combining an Enhanced Polyphosphate Kinase-Driven UDP-Glucose Regeneration System with the Screening of Key Glycosyltransferases for Efficient Synthesis of Nucleoside Disaccharides.

机构信息

State Key Laboratory of Bioreactor Engineering, East China University of Science and Technology, 130 Meilong Road, Shanghai 200237, China.

Shanghai Collaborative Innovation Center for Biomanufacturing Technology, 130 Meilong Road, Shanghai 200237, China.

出版信息

J Agric Food Chem. 2024 Sep 18;72(37):20557-20567. doi: 10.1021/acs.jafc.4c05329. Epub 2024 Sep 9.

Abstract

Nucleoside disaccharides are essential glycosides that naturally occur in specific living organisms. This study developed an enhanced UDP-glucose regeneration system to facilitate the multienzyme synthesis of nucleoside disaccharides by integrating it with nucleoside-specific glycosyltransferases. The system utilizes maltodextrin and polyphosphate as cost-effective substrates for UDP-glucose supply, catalyzed by α-glucan phosphorylase (αGP) and UDP-glucose pyrophosphorylase (UGP). To address the low activity of known polyphosphate kinases (PPKs) in the UDP phosphorylation reaction, a sequence-driven screening identified RhPPK with high activity against UDP (>1000 U/mg). Computational design further led to the creation of a double mutant with a 2566-fold increase in thermostability at 50 °C. The enhanced UDP-glucose regeneration system increased the production rate of nucleoside disaccharide synthesis by 25-fold. In addition, our UDP-glucose regeneration system is expected to be applied to other glycosyl transfer reactions.

摘要

核苷二糖是在特定生物体中天然存在的必需糖苷。本研究开发了一种增强的 UDP-葡萄糖再生系统,通过将其与核苷特异性糖基转移酶集成,促进多酶合成核苷二糖。该系统利用麦芽糊精和多聚磷酸盐作为 UDP-葡萄糖供应的经济有效的底物,由α-葡聚糖磷酸化酶(αGP)和 UDP-葡萄糖焦磷酸化酶(UGP)催化。为了解决已知多聚磷酸激酶(PPKs)在 UDP 磷酸化反应中活性低的问题,通过序列驱动筛选鉴定出对 UDP 具有高活性的 RhPPK(>1000 U/mg)。计算设计进一步导致创建了一个在 50°C 时热稳定性提高 2566 倍的双突变体。增强的 UDP-葡萄糖再生系统将核苷二糖合成的生产速率提高了 25 倍。此外,我们的 UDP-葡萄糖再生系统有望应用于其他糖基转移反应。

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