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Erythritol production on wheat straw using Trichoderma reesei

机译:使用里氏木霉在麦草上生产赤藓糖醇

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摘要

We overexpressed the err1 gene in the Trichoderma reesei wild-type and in the cellulase hyperproducing, carbon catabolite derepressed strain Rut-C30 in order to investigate the possibility of producing erythritol with T. reesei. Two different promoters were used for err1 overexpression in both strains, a constitutive (the native pyruvat kinase (pki) promoter) and an inducible one (the native β-xylosidase (bxl1) promoter). The derived recombinant strains were precharacterized by analysis of err1 transcript formation on D-xylose and xylan. Based on this, one strain of each type was chosen for further investigation for erythritol production in shake flasks and in bioreactor experiments. For the latter, we used wheat straw pretreated by an alkaline organosolve process as lignocellulosic substrate. Shake flask experiments on D-xylose showed increased erythritol formation for both, the wild-type and the Rut-C30 overexpression strain compared to their respective parental strain. Bioreactor cultivations on wheat straw did not increase erythritol formation in the wild-type overexpression strain. However, err1 overexpression in Rut-C30 led to a clearly higher erythritol formation on wheat straw.
机译:为了研究里氏木霉产生赤藓糖醇的可能性,我们在里氏木霉野生型和纤维素酶高产,碳分解代谢物抑制菌株Rut-C30中过表达err1基因。在两个菌株中,两个不同的启动子用于err1过表达,一个是组成型的(天然丙酮酸激酶(pki)启动子),另一个是可诱导的启动子(天然β-木糖苷酶(bxl1)启动子)。通过分析D-木糖和木聚糖上的err1转录本的形成来表征衍生的重组菌株。基于此,选择每种菌株中的一种用于进一步研究摇瓶和生物反应器实验中赤藓糖醇的生产。对于后者,我们使用经过碱性有机溶解工艺预处理的麦秸作为木质纤维素基质。在D-木糖上进行的摇瓶实验表明,与野生型和Rut-C30过表达菌株相比,它们各自的亲本菌株都增加了赤藓糖醇的形成。在野生型过表达菌株中,小麦秸秆上的生物反应器培养未增加赤藓糖醇的形成。但是,Rut-C30中的err1过表达导致小麦秸秆上赤藓醇的形成明显更高。

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