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Co-production of ethanol and squalene using a Saccharomyces cerevisiae ERG1 (squalene epoxidase) mutant and agro-industrial feedstock

机译:使用酿酒酵母ERG1(角鲨烯环氧酶)突变体和农用工业原料共同生产乙醇和角鲨烯

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Background Genetically customised Saccharomyces cerevisiae that can produce ethanol and additional bio-based chemicals from sustainable agro-industrial feedstocks (for example, residual plant biomass) are of major interest to the biofuel industry. We investigated the microbial biorefinery concept of ethanol and squalene co-production using S. cerevisiae (strain YUG37-ERG1) wherein ERG1 (squalene epoxidase) transcription is under the control of a doxycycline-repressible tet07-CYC1 promoter. The production of ethanol and squalene by YUG37-ERG1 grown using agriculturally sourced grass juice supplemented with doxycycline was assessed. Results Use of the tet07-CYC1 promoter permitted regulation of ERG1 expression and squalene accumulation in YUG37-ERG1, allowing us to circumvent the lethal growth phenotype seen when ERG1 is disrupted completely. In experiments using grass juice feedstock supplemented with 0 to 50 ?g doxycycline mL?1, YUG37-ERG1 fermented ethanol (22.5 [±0.5] mg mL?1) and accumulated the highest squalene content (7.89?±?0.25 mg g?1 dry biomass) and yield (18.0?±?4.18 mg squalene L?1) with supplements of 5.0 and 0.025 ?g doxycycline mL?1, respectively. Grass juice was found to be rich in water-soluble carbohydrates (61.1 [±3.6] mg sugars mL?1) and provided excellent feedstock for growth and fermentation studies using YUG37-ERG1. Conclusion Residual plant biomass components from crop production and rotation systems represent possible substrates for microbial fermentation of biofuels and bio-based compounds. This study is the first to utilise S. cerevisiae for the co-production of ethanol and squalene from grass juice. Our findings underscore the value of the biorefinery approach and demonstrate the potential to integrate microbial bioprocess engineering with existing agriculture.
机译:背景技术可以从可持续的农业工业原料(例如,残留的植物生物质)生产乙醇和其他生物基化学物质的基因定制酿酒酵母对生物燃料产业具有重大意义。我们调查了使用酿酒酵母(菌株YUG37-ERG1)联合生产乙醇和角鲨烯的微生物生物精炼概念,其中ERG1(角鲨烯环氧酶)的转录受强力霉素抑制的tet07-CYC1启动子的控制。评估了YUG37-ERG1的乙醇和角鲨烯的生产,该YUG37-ERG1是使用农业生产的草汁加多西环素补充生长而成的。结果使用tet07-CYC1启动子可以调节YUG37-ERG1中ERG1的表达和角鲨烯的积累,从而使我们能够规避当ERG1被完全破坏时看到的致死性生长表型。在使用添加了0至50微克多西环素mL?1的草汁原料进行的实验中,YUG37-ERG1发酵了乙醇(22.5 [±0.5] mg mL?1),并积累了最高的角鲨烯含量(7.89±±0.25 mg g?1)。干物质)和产量(18.0±±4.18 mg角鲨烯L±1),分别补充5.0和0.025μg多西环素mL-1。草汁被发现富含水溶性碳水化合物(61.1 [±3.6] mg糖mL?1),并为使用YUG37-ERG1进行生长和发酵研究提供了极好的原料。结论作物生产和轮作系统中残留的植物生物量成分是微生物发酵生物燃料和生物基化合物的可能底物。这项研究是首次利用酿酒酵母从草汁中联合生产乙醇和角鲨烯。我们的发现强调了生物精炼方法的价值,并证明了将微生物生物工艺工程与现有农业相结合的潜力。

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