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在巴斯德毕赤酵母中通过密码子优化、启动子和菌株选择对长枝木霉 ATCC 20611 的 β-呋喃果糖苷酶的异源生产的影响。

Influence of codon optimization, promoter, and strain selection on the heterologous production of a β-fructofuranosidase from Aspergillus fijiensis ATCC 20611 in Pichia pastoris.

机构信息

Department of Process Engineering, Stellenbosch University, Private Bag X1, Matieland, 7602, South Africa.

出版信息

Folia Microbiol (Praha). 2022 Apr;67(2):339-350. doi: 10.1007/s12223-022-00947-8. Epub 2022 Feb 8.

DOI:10.1007/s12223-022-00947-8
PMID:35133569
Abstract

Fructooligosaccharides (FOS) are compounds possessing various health properties and are added to functional foods as prebiotics. The commercial production of FOS is done through the enzymatic transfructolysation of sucrose by β-fructofuranosidases which is found in various organisms of which Aureobasidium pullulans and Aspergillus niger are the most well known. This study overexpressed two differently codon-optimized variations of the Aspergillus fijiensis β-fructofuranosidase-encoding gene (fopA) under the transcriptional control of either the alcohol oxidase (AOX1) or glyceraldehyde-3-phosphate dehydrogenase (GAP) promoters. When cultivated in shake flasks, the two codon-optimized variants displayed similar volumetric enzyme activities when expressed under control of the same promoter with the GAP strains producing 11.7 U/ml and 12.7 U/ml, respectively, and the AOX1 strains 95.8 U/ml and 98.6 U/ml, respectively. However, the highest production levels were achieved for both codon-optimized genes when expressed under control of the AOX1 promoter. The AOX1 promoter was superior to the GAP promoter in bioreactor cultivations for both codon-optimized genes with 13,702 U/ml and 2718 U/ml for the AOX1 promoter for ATUM and GeneArt, respectively, and 6057 U/ml and 1790 U/ml for the GAP promoter for ATUM and GeneArt, respectively. The ATUM-optimized gene produced higher enzyme activities when compared to the one from GeneArt, under the control of both promoters.

摘要

果寡糖(FOS)是具有多种健康特性的化合物,被添加到功能性食品中作为益生元。FOS 的商业生产是通过β-呋喃果糖苷酶对蔗糖进行转果糖作用来完成的,β-呋喃果糖苷酶存在于各种生物体中,其中最著名的是出芽短梗霉和黑曲霉。本研究在转录水平上分别受醇氧化酶(AOX1)和 3-磷酸甘油醛脱氢酶(GAP)启动子的控制下,过表达了两种不同密码子优化的aspergillus fijiensis β-呋喃果糖苷酶编码基因(fopA)的变体。在摇瓶培养中,当在相同的启动子控制下表达时,两种密码子优化的变体显示出相似的比酶活,其中 GAP 菌株分别产生 11.7 U/ml 和 12.7 U/ml,AOX1 菌株分别产生 95.8 U/ml 和 98.6 U/ml。然而,当在 AOX1 启动子的控制下表达时,两种密码子优化基因都达到了最高的表达水平。对于两种密码子优化基因,在生物反应器培养中,AOX1 启动子优于 GAP 启动子,对于 ATUM 和 GeneArt,AOX1 启动子分别产生 13702 U/ml 和 2718 U/ml,GAP 启动子分别产生 6057 U/ml 和 1790 U/ml。与 GeneArt 相比,在两种启动子的控制下,ATUM 优化基因产生的酶活更高。

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