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首页> 外文期刊>Journal of Biotechnology >Enhanced cellobiose fermentation by engineered Saccharomyces cerevisiae expressing a mutant cellodextrin facilitator and cellobiose phosphorylase
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Enhanced cellobiose fermentation by engineered Saccharomyces cerevisiae expressing a mutant cellodextrin facilitator and cellobiose phosphorylase

机译:通过设计突变体蜂窝蛋白促进剂和纤维二糖磷酸化酶的工程化酵母菌酿酒酵母增强纤维二糖发酵

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摘要

To efficiently ferment intermediate cellodextrins released during cellulose hydrolysis, Saccharomyces cerevisiae has been engineered by introduction of a heterologous cellodextrin utilizing pathway consisting of a cellodextrin transporter and either an intracellular beta-glucosidase or a cellobiose phosphorylase. Among two types of cello dextrin transporters, the passive facilitator CDT-2 has not enabled better cellobiose fermentation than the active transporter CDT-1, which suggests that the CDT-2 might be engineered to provide energetic benefits over the active transporter in cellobiose fermentation. We attempted to improve cellobiose transporting activity of CDT-2 through laboratory evolution. Nine rounds of a serial subculture of S. cerevisiae expressing CDT-2 and cellobiose phosphorylase on cellobiose led to the isolation of an evolved strain capable of fermenting cellobiose to ethanol 10-fold faster than the original strain. After sequence analysis of the isolated CDT-2, a single point mutation on CDT-2 (N3061) was revealed to be responsible for enhanced cellobiose fermentation. Also, the engineered strain expressing the mutant CDT-2 with cellobiose phosphorylase showed a higher ethanol yield than the engineered strain expressing CDT-1 and intracellular beta-glucosidase under anaerobic conditions, suggesting that CDT-2 coupled with cellobiose phosphorylase may be better choices for efficient production of cellulosic ethanol with the engineered yeast
机译:为了在纤维素水解期间有效发酵中间体纤维素,通过引入使用由蜂窝天文素转运蛋白和细胞内β-葡糖苷酶或纤维素磷酸化酶组成的途径来设计酿酒酵母。在两种类型的细胞糊精转运蛋白中,无源促进剂CDT-2没有能够比活性转运蛋白CDT-1能够更好的纤维二糖发酵,这表明CDT-2可能被设计成在纤维二糖发酵中的活性转运蛋白上提供能量益处。我们试图通过实验室进化改善CDT-2的Cellobiose运输活性。在纤维生物糖上表达CDT-2和Cellobiose磷酸化酶的九轮串联亚培养物导致了能够将纤维糖发酵至乙醇的进化菌株,其比原始菌株快10倍。在分离的CDT-2的序列分析后,显示CDT-2(N3061)上的单点突变,以负责增强的纤维二糖发酵。此外,用纤维素糖磷酸化酶表达突变体CDT-2的工程化菌株显示出比在厌氧条件下表达CDT-1和细胞内β-葡糖苷酶的工程化菌株的乙醇产率较高,表明CDT-2与纤维生物糖磷酸化酶偶联可能是更好的选择高效生产纤维素乙醇与工程酵母

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