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痤疮丙酸杆菌亚油酸异构酶的酵母细胞表面展示及其在反式-10,顺式-12共轭亚油酸生产中的应用。

Yeast cell surface display of linoleic acid isomerase from Propionibacterium acnes and its application for the production of trans-10, cis-12 conjugated linoleic acid.

作者信息

He Xihong, Shang Jiling, Li Fan, Liu Hao

机构信息

Key Laboratory of Industrial Fermentation Microbiology, Ministry of Education, College of Biotechnology, Tianjin University of Science and Technology, Tianjin, People's Republic of China.

出版信息

Biotechnol Appl Biochem. 2015 Jan-Feb;62(1):1-8. doi: 10.1002/bab.1249. Epub 2014 Nov 17.

Abstract

Conjugated linoleic acid (CLA), a family of geometric and positional isomers of linoleic acid, has many health-promoting properties. Different isomers of CLA may have very different physiological effects. In the current work, we explore the possibility to produce single isomer of CLA by using biocatalysis based on displayed biocatalysts on the yeast cell surfaces. A reporter system used to assess gene expression and protein distribution was established by combining the egfp gene to the N-terminus of Propionibacterium acnes pai gene encoding the linoleic isomerase onto vector pYD1. After induction of the yeast strains containing pYD1::egfp::pai with galactose, strong green fluorescence was observed on the surface of cells, demonstrating that the fusion protein was successfully displayed. Using the engineered strains as whole-cell biocatalyst, trans-10, cis-12 CLA was detected in the reaction mixture. To improve the biocatalytic potential of this system, the first 20 amino codons of pai were modified, and the catalytic reaction conditions were optimized. Optimization of the codon usage resulted in 35% increase of CLA production, and the maximum yield of CLA was observed within 20 H in the optimal conditions: pH 7.0, 4 mg/mL linoleic acid, 37 °C. The system established in the present work can guide the development of biocatalytic strategies to produce trans-10, cis-12 CLA single isomer.

摘要

共轭亚油酸(CLA)是亚油酸的一系列几何异构体和位置异构体,具有许多促进健康的特性。CLA的不同异构体可能具有非常不同的生理效应。在当前的工作中,我们探索了基于酵母细胞表面展示的生物催化剂利用生物催化生产CLA单一异构体的可能性。通过将egfp基因与编码亚油酸异构酶的痤疮丙酸杆菌pai基因的N端连接到载体pYD1上,建立了一个用于评估基因表达和蛋白质分布的报告系统。用半乳糖诱导含有pYD1::egfp::pai的酵母菌株后,在细胞表面观察到强烈的绿色荧光,表明融合蛋白成功展示。使用工程菌株作为全细胞生物催化剂,在反应混合物中检测到反式-10,顺式-12 CLA。为了提高该系统的生物催化潜力,对pai的前20个氨基酸密码子进行了修饰,并优化了催化反应条件。密码子使用的优化使CLA产量提高了35%,在最佳条件下(pH 7.0、4 mg/mL亚油酸、37°C),在20小时内观察到CLA的最大产量。本工作中建立的系统可以指导生产反式-10,顺式-12 CLA单一异构体的生物催化策略的开发。

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