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利用表达植物乳杆菌L-阿拉伯糖异构酶的工程化大肠杆菌菌株从乳清粉中两步生物合成D-塔格糖。

Two-stage biosynthesis of D-tagatose from milk whey powder by an engineered Escherichia coli strain expressing L-arabinose isomerase from Lactobacillus plantarum.

作者信息

Zhang Guoyan, Zabed Hossain M, Yun Junhua, Yuan Jiao, Zhang Yufei, Wang Yang, Qi Xianghui

机构信息

School of Food and Biological Engineering, Jiangsu University, 301 Xuefu Road, Zhenjiang 212013, Jiangsu, China.

School of Food and Biological Engineering, Jiangsu University, 301 Xuefu Road, Zhenjiang 212013, Jiangsu, China.

出版信息

Bioresour Technol. 2020 Jun;305:123010. doi: 10.1016/j.biortech.2020.123010. Epub 2020 Feb 11.

Abstract

In this study, a new strain of Lactobacillus plantarum (CY.6) was identified and its L-arabinose isomerase (L-AI) encoding gene (araA) was overexpressed in Escherichia coli BL21 for the biosynthesis of D-tagatose from milk whey powders (WP). Whole-cell biotransformation of lactose in WP into D-tagatose was done by three technological approaches, including 100%, 50% and 0% hydrolysis of lactose in WP before biotransformation, where simultaneous saccharification and biotransformation (SSB, 0% prior hydrolysis of lactose) produced maximum amounts of D-tagatose. Two-stage SSB provided 73.6% conversion efficiency (based on D-galactose) and 36.8% (in term of lactose), with 51.5 g/L of D-tagatose after 96 h, while concentration of D-tagatose produced after first stage was 34.4 g/L. Yield and volumetric productivity of D-tagatose after two-stage SSB were found to be 0.26 g/g of WP (0.37 g/g of lactose, 0.74 g/g of D-galactose produced from lactose) and 0.54 g/L/h, respectively.

摘要

在本研究中,鉴定出了一种新的植物乳杆菌菌株(CY.6),并在大肠杆菌BL21中过表达其编码L-阿拉伯糖异构酶(L-AI)的基因(araA),用于从乳清粉(WP)生物合成D-塔格糖。通过三种技术方法将WP中的乳糖全细胞生物转化为D-塔格糖,包括在生物转化前对WP中的乳糖进行100%、50%和0%的水解,其中同时糖化和生物转化(SSB,乳糖预水解0%)产生的D-塔格糖量最大。两阶段SSB提供了73.6%的转化效率(基于D-半乳糖)和36.8%(基于乳糖),96小时后产生51.5 g/L的D-塔格糖,而第一阶段产生的D-塔格糖浓度为34.4 g/L。两阶段SSB后D-塔格糖的产率和体积生产率分别为0.26 g/g WP(0.37 g/g乳糖,由乳糖产生的0.74 g/g D-半乳糖)和0.54 g/L/h。

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