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通过 GDP-l-岩藻糖途径在 ATCC 6051a 中理性设计 α-1,3-岩藻糖基转移酶合成 3-岩藻乳糖

Rational Design of an α-1,3-Fucosyltransferase for the Biosynthesis of 3-Fucosyllactose in ATCC 6051a via GDP-l-Fucose Pathway.

机构信息

Shanghai Advanced Research Institute, Chinese Academy of Sciences, Shanghai 201210, China.

University of Chinese Academy of Sciences, Beijing 100049, China.

出版信息

J Agric Food Chem. 2024 Jan 17;72(2):1178-1189. doi: 10.1021/acs.jafc.3c07604. Epub 2024 Jan 6.

Abstract

3-Fucosyllactose (3-FL) is an important oligosaccharide and nutrient in breast milk that can be synthesized in microbial cells by α-1,3-fucosyltransferase (α-1,3-FucT) using guanosine 5'-diphosphate (GDP)-l-fucose and lactose as substrates. However, the catalytic efficiency of known α-1,3-FucTs from various sources was limited due to their low solubility. To enhance the microbial production of 3-FL, the efficiencies of α-1,3-FucTs were evaluated and in () chassis cells that had been endowed with a heterologous synthetic pathway for GDP-l-fucose, revealing that the activity of FucTa from () was higher than that of any of other reported homologues. To further improve the catalytic performance of FucTa, a rational design approach was employed, involving intracellular evaluation of the mutational sites of M32 obtained through directed evolution, analysis of the ligand binding site diversity, and protein structure simulation. Among the obtained variants, the FucTa-Y218 K variant exhibited the highest 3-FL yield, reaching 7.55 g/L in the shake flask growth experiment, which was 3.48-fold higher than that achieved by the wild-type enzyme. Subsequent fermentation optimization in a 5 L bioreactor resulted in a remarkable 3-FL production of 36.98 g/L, highlighting the great prospects of the designed enzyme and the strains for industrial applications.

摘要

3-岩藻糖基乳糖(3-FL)是母乳中的一种重要寡糖和营养物质,可以通过α-1,3-岩藻糖基转移酶(α-1,3-FucT)在微生物细胞中使用鸟苷 5'-二磷酸(GDP)-L-岩藻糖和乳糖作为底物合成。然而,由于其低溶解度,来自各种来源的已知α-1,3-FucT 的催化效率有限。为了提高 3-FL 的微生物产量,评估了α-1,3-FucT 的效率,并在已赋予 GDP-L-岩藻糖异源合成途径的()底盘细胞中,发现()来源的 FucTa 的活性高于任何其他报道的同源物。为了进一步提高 FucTa 的催化性能,采用了合理的设计方法,包括通过定向进化获得的 M32 突变位点的细胞内评估、配体结合位点多样性分析和蛋白质结构模拟。在获得的变体中,FucTa-Y218K 变体表现出最高的 3-FL 产量,在摇瓶生长实验中达到 7.55g/L,比野生型酶高 3.48 倍。随后在 5L 生物反应器中进行发酵优化,得到了显著的 36.98g/L 的 3-FL 产量,突出了设计酶和菌株在工业应用中的巨大前景。

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