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首页> 外文期刊>Engineering in Life Sciences >Engineering an industrial Saccharomyces cerevisiae strain with the inulinase gene for more efficient ethanol production from Jerusalem artichoke tubers
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Engineering an industrial Saccharomyces cerevisiae strain with the inulinase gene for more efficient ethanol production from Jerusalem artichoke tubers

机译:用菊粉酶基因工程改造工业酿酒酵母菌株,以从菊芋块茎中更有效地生产乙醇

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摘要

Engineering industrial microbial strains with inulinase production for developing a consolidated bioprocessing (CBP) strategy is a desirable solution to biofuel production from Jerusalem artichoke tubers. In this study, the integrative vector pFA6a-rDNA-PGK-INU was generated by fusing the 3.3-kb ribosomal DNA fragment with the phosphoglycerate kinase promoter to regulate the expression of the inulinase gene isolated from Kluyveromyces marxianus, which was then integrated into the chromosome of an industrial Saccharomyces cerevisiae strain for ethanol production from Jerusalem artichoke tubers. Compared to the host strain, no significant difference was observed in the growth of the recombinant yeast, but its inulinase production was enhanced: 22.9 versus 10.6 U/mL for aerobic seed cultures and 14.5 versus 10.0 U/mL for ethanol fermentation, which consequently facilitated the CBP process for ethanol production: 72.5 g/L ethanol produced in a fermentation time of 48 h, while only 67.0 g/L ethanol was produced by the host strain in a fermentation time of 60 h. Thus, the ethanol productivity was increased from 1.12 to 1.51 g/L/h, presenting an increase of 34.8%.
机译:用菊粉酶生产工业微生物菌株来开发综合生物处理(CBP)策略是从菊芋块茎生产生物燃料的理想解决方案。在这项研究中,整合载体pFA6a-rDNA-PGK-INU是通过将3.3 kb核糖体DNA片段与磷酸甘油酸激酶启动子融合来调节从马克斯克鲁维酵母分离出的菊粉酶基因的表达而产生的,然后整合到染色体中菊芋块茎生产乙醇的工业酿酒酵母菌株的制备与宿主菌株相比,重组酵母的生长没有显着差异,但是其菊粉酶的产量提高了:好氧种子培养物的菊糖酶产量为22.9 vs 10.6 U / mL,乙醇发酵的菊粉酶产量为14.5 vs 10.0 U / mL,因此促进了发酵CBP生产乙醇的过程​​:在48 h的发酵时间内产生了72.5 g / L的乙醇,而在60 h的发酵时间内宿主菌株仅产生了67.0 g / L的乙醇。因此,乙醇生产率从1.12增加到1.51g / L / h,增加了34.8%。

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