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Engineering of Cyclodextrin Glucanotransferase on the Cell Surface of Saccharomyces cerevisiae for Improved Cyclodextrin Production

机译:酿酒酵母细胞表面上环糊精葡糖基转移酶的工程改造以提高环糊精的生产

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摘要

The cyclodextrin glucanotransferase (CGTase) gene (cgt) from Bacillus circulans 251 was cloned into plasmid pYD1, which allowed regulated expression, secretion, and detection. The expression of CGTase with a-agglutinin at the N-terminal end on the extracellular surface of Saccharomyces cerevisiae was confirmed by immunofluorescence microscopy. This surface-anchored CGTase gave the yeast the ability to directly utilize starch as a sole carbon source and the ability to produce the anticipated products, cyclodextrins, as well as glucose and maltose. The resulting glucose and maltose, which are efficient acceptors in the CGTase coupling reaction, could be consumed by yeast fermentation and thus facilitated cyclodextrin production. On the other hand, ethanol produced by the yeast may form a complex with cyclodextrin and shift the equilibrium in favor of cyclodextrin production. The yeast with immobilized CGTase produced 24.07 mg/ml cyclodextrins when it was incubated in yeast medium supplemented with 4% starch.
机译:将来自圆形芽孢杆菌251的环糊精葡糖基转移酶(CGTase)基因(cgt)克隆到质粒pYD1中,该质粒可以调节表达,分泌和检测。通过免疫荧光显微镜检查证实了酿酒酵母细胞外表面N末端带有α-凝集素的CGTase的表达。这种表面锚定的CGTase使酵母能够直接利用淀粉作为唯一的碳源,并具有产生预期产物,环糊精以及葡萄糖和麦芽糖的能力。产生的葡萄糖和麦芽糖是CGTase偶联反应的有效受体,可被酵母发酵消耗,从而促进环糊精的生产。另一方面,由酵母产生的乙醇可与环糊精形成复合物,并转移平衡以利于环糊精的产生。当在添加了4%淀粉的酵母培养基中孵育时,带有固定化CGTase的酵母产生24.07 mg / ml环糊精。

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