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Improving the performance of industrial ethanol-producing yeast by expressing the aspartyl protease on the cell surface

机译:通过在细胞表面表达天冬氨酰蛋白酶来提高工业生产乙醇的酵母的性能

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摘要

The yeasts used in fuel ethanol manufacture are unable to metabolize soluble proteins. The PEP4 gene, encoding a vacuolar aspartyl protease in Saccharomyces cerevisiae, was either secretively or cell-surface anchored expressed in industrial ethanol-producing S. cerevisiae. The obtained recombinant strains APA (expressing the protease secretively) and APB (expressing the protease on the cell wall) were studied under ethanol fermentation conditions in feed barley cultures. The effects of expression of the protease on product formation, growth and cell protein content were measured. The biomass yield of the wild-type was clearly lower than that of the recombinant strains (0.578 +/- 0.12 g biomass/g glucose for APA and 0.582 +/- 0.08 g biomass/g glucose for APB). In addition, nearly 98-99% of the theoretical maximum level of ethanol yield was achieved (relative to the amount of substrate consumed) for the recombinant strains, while limiting the nitrogen source resulted in dissatisfactory fermentation for the wild-type and more than 30 g/l residual sugar was detected at the end of fermentation. In addition, higher growth rate, viability and lower yields of byproducts such as glycerol and pyruvic acid for recombinant strains were observed. Expressing acid protease can be expected to lead to a significant increase in ethanol productivity.
机译:用于燃料乙醇生产的酵母无法代谢可溶性蛋白质。在酿酒酵母中,PEP4基因在酿酒酵母中编码液泡天冬氨酰蛋白酶,被秘密分泌或在细胞表面锚定表达。在饲料大麦培养物中,在乙醇发酵条件下研究了获得的重组菌株APA(秘密表达蛋白酶)和APB(细胞壁表达蛋白酶)。测量了蛋白酶表达对产物形成,生长和细胞蛋白含量的影响。野生型的生物量产量明显低于重组菌株(对于APA为0.578 +/- 0.12 g生物量/ g葡萄糖,对于APB为0.582 +/- 0.08 g生物量/ g葡萄糖)。此外,重组菌株可达到理论最高乙醇产量的近98-99%(相对于底物消耗的量),同时限制氮源导致野生型发酵的效果不理想,超过30种在发酵结束时检测到g / l的残留糖。另外,观察到重组菌株的较高的生长速率,存活力和较低的副产物如甘油和丙酮酸的产率。表达酸性蛋白酶可望导致乙醇生产率的显着提高。

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