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工程化一种祖先糖基转移酶用于合成 2-苯乙基-β-d-葡萄糖苷和红景天苷。

Engineering an Ancestral Glycosyltransferase for Biosynthesis of 2-Phenylethyl-β-d-Glucopyranoside and Salidroside.

机构信息

College of Biotechnology and Pharmaceutical Engineering, Nanjing Tech University, Nanjing 211816, China.

出版信息

J Agric Food Chem. 2024 Sep 11;72(36):19966-19976. doi: 10.1021/acs.jafc.4c04381. Epub 2024 Aug 27.

Abstract

Phenylethanoid glycosides (PhGs) are naturally occurring glycosides derived from plants with various biological activities. Glycosyltransferases catalyze the production of PhGs from phenylethanols via a transglycosylation reaction. The low activity and stability of glycosyltransferase limit its industrial application. An ancestral glycosyltransferase, UGTAn85, with heat resistance, alkali resistance, and high stability was resurrected using ancestral sequence reconstruction technology. This enzyme can efficiently convert phenylethanols to PhGs. The optimal reaction temperature and pH for UGTAn85 were found to be 70 °C and pH 10.0, respectively. This study employed a combination of structure-guided rational design and co-evolution analysis to enhance its catalytic activity. Potential mutation sites were identified through computer-aided design, including homology modeling, molecular docking, Rosetta dock design, molecular dynamics simulation, and co-evolution analysis. By targeted mutagenesis, the UGTAn85 mutant Q23E/N65D exhibited a 2.2-fold increase in enzyme activity (11.85 U/mg) and elevated affinity ( = 0.11 mM) for 2-phenylethanol compared to UGTAn85. Following a fed-batch reaction, 36.16 g/L 2-phenylethyl-β-d-glucopyranoside and 51.49 g/L salidroside could be produced within 24 h, respectively. The findings in this study provide a new perspective on enhancing the stability and activity of glycosyltransferases, as well as a potential biocatalyst for the industrial production of PhGs.

摘要

苯乙醇苷类(PhGs)是一类天然存在的糖苷,来源于具有多种生物活性的植物。糖基转移酶通过转糖苷反应催化苯乙醇生成 PhGs。糖基转移酶活性和稳定性低,限制了其工业应用。利用祖先序列重建技术,复活了一种具有耐热、耐碱和高稳定性的祖先糖基转移酶 UGTAn85。该酶能高效地将苯乙醇转化为 PhGs。发现 UGTAn85 的最适反应温度和 pH 分别为 70°C 和 pH 10.0。本研究采用结构导向的理性设计和共进化分析相结合的方法来提高其催化活性。通过计算机辅助设计,确定了潜在的突变位点,包括同源建模、分子对接、Rosetta 对接设计、分子动力学模拟和共进化分析。通过定点突变,UGTAn85 的突变体 Q23E/N65D 的酶活性(11.85 U/mg)提高了 2.2 倍,对 2-苯乙醇的亲和力( = 0.11 mM)也有所提高。经过分批补料反应,24 h 内可分别生产 36.16 g/L 2-苯乙基-β-d-吡喃葡萄糖苷和 51.49 g/L 红景天苷。本研究为提高糖基转移酶的稳定性和活性提供了新的视角,为 PhGs 的工业生产提供了一种潜在的生物催化剂。

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