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通过携带马克斯克鲁维酵母菊粉酶的重组酿酒酵母从菊粉生产乙醇来优化启动子和分泌信号序列。

Optimizing promoters and secretory signal sequences for producing ethanol from inulin by recombinant Saccharomyces cerevisiae carrying Kluyveromyces marxianus inulinase.

作者信息

Hong Soo-Jeong, Kim Hyo Jin, Kim Jin-Woo, Lee Dae-Hee, Seo Jin-Ho

机构信息

Department of Agricultural Biotechnology and Center for Food and Bioconvergence, Seoul National University, 599 Gwanak-Ro, Gwanak-Gu, Seoul, 151-921, South Korea.

出版信息

Bioprocess Biosyst Eng. 2015 Feb;38(2):263-72. doi: 10.1007/s00449-014-1265-7. Epub 2014 Aug 21.

DOI:10.1007/s00449-014-1265-7
PMID:25142154
Abstract

Inulin is a polyfructan that is abundant in plants such as Jerusalem artichoke, chicory and dahlia. Inulinase can easily hydrolyze inulin to fructose, which is consumed by microorganisms. Generally, Saccharomyces cerevisiae, an industrial workhorse strain for bioethanol production, is known for not having inulinase activity. The inulinase gene from Kluyveromyces marxianus (KmINU), with the ability of converting inulin to fructose, was introduced into S. cerevisiae D452-2. The inulinase gene was fused to three different types of promoter (GPD, PGK1, truncated HXT7) and secretory signal sequence (KmINU, MFα1, SUC2) to generate nine expression cassettes. The inulin fermentation performance of the nine transformants containing different promoter and signal sequence combinations for inulinase production were compared to select an optimized expression system for efficient inulin fermentation. Among the nine inulinase-producing transformants, the S. cerevisiae carrying the PGK1 promoter and MFα1 signal sequence (S. cerevisiae D452-2/p426PM) showed not only the highest specific KmINU activity, but also the best inulin fermentation capability. Finally, a batch fermentation of the selected S. cerevisiae D452-2/p426PM in a bioreactor with 188.2 g/L inulin was performed to produce 80.2 g/L ethanol with 0.43 g ethanol/g inulin of ethanol yield and 1.22 g/L h of ethanol productivity.

摘要

菊粉是一种多聚果糖,在菊芋、菊苣和大丽花等植物中含量丰富。菊粉酶能够轻易地将菊粉水解成果糖,而果糖会被微生物消耗。一般来说,酿酒酵母作为生物乙醇生产的工业主力菌株,以不具有菊粉酶活性而闻名。将来自马克斯克鲁维酵母的菊粉酶基因(KmINU)导入酿酒酵母D452-2中,该基因具有将菊粉转化为果糖的能力。菊粉酶基因与三种不同类型的启动子(GPD、PGK1、截短的HXT7)和分泌信号序列(KmINU、MFα1、SUC2)融合,以产生九个表达盒。比较了含有不同启动子和信号序列组合用于菊粉酶生产的九个转化体的菊粉发酵性能,以选择一个优化的表达系统用于高效菊粉发酵。在九个产生菊粉酶的转化体中,携带PGK1启动子和MFα1信号序列的酿酒酵母(酿酒酵母D452-2/p426PM)不仅显示出最高的比KmINU活性,而且具有最佳的菊粉发酵能力。最后,在生物反应器中对选定的酿酒酵母D452-2/p426PM进行了分批发酵,以188.2 g/L菊粉为原料,生产出80.2 g/L乙醇,乙醇产率为0.43 g乙醇/g菊粉,乙醇生产率为1.22 g/L·h。

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