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首页> 外文期刊>Journal of Biotechnology >Homologous overexpression of xylanase in Fusarium oxysporum increases ethanol productivity during consolidated bioprocessing (CBP) of lignocellulosics
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Homologous overexpression of xylanase in Fusarium oxysporum increases ethanol productivity during consolidated bioprocessing (CBP) of lignocellulosics

机译:木霉镰刀菌中木聚糖酶的同源过量表达提高了木质纤维素综合生物加工(CBP)期间的乙醇生产率

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In an effort to increase ethanol productivity during the consolidated bioprocessing (CBP) of lignocellulosics by Fusarium oxysporum, we attempted the constitutive homologous overexpression of one of the key process enzymes, namely an endo-xylanase. The endo-beta-1,4-xylanase 2 gene was incorporated into the F. oxysporum genome under the regulation of the gpdA promoter of Aspergillus nidulans. The transformation was effected through Agrobacterium tumefaciens and resulted in 12 transformants, two of which were selected for further study due to their high extracellular xylanase activities under normally repressing conditions (glucose as sole carbon source). During natural induction conditions (growth on xylan) though, the extracellular enzyme levels of the transformants were only marginally higher (5-10%) compared to the wild type despite the significantly stronger xylanase 2 mRNA signals. SDS-PAGE verified enzyme assay results that there was no intracellular xylanase 2 accumulation in the transformants, suggesting the potential regulation in a post transcriptional or translational level. The fermentative performance of the transformants was evaluated and compared to that of the wild type in simple CBP systems using either corn cob or wheat bran as sole carbon sources. Both transformants produced approximately 60% more ethanol compared to the wild type on corn cob, while for wheat bran this picture was repeated for only one of them. This result is attributed to the high extracellular xylanase activities in the transformants' fermentation broths that were maintained 2-2.5-fold higher compared to the wild type
机译:为了在尖酸镰刀菌(Fusarium oxysporum)进行木质纤维素的整合生物处理(CBP)期间提高乙醇生产率,我们尝试了关键过程酶之一即木聚糖内切酶的组成型同源过表达。在构巢曲霉的gpdA启动子的调节下,将内-β-1,4-木聚糖酶2基因掺入到尖孢镰刀菌基因组中。该转化是通过根癌土壤杆菌进行的,并产生了12个转化子,由于在正常抑制条件下它们具有很高的细胞外木聚糖酶活性(葡萄糖是唯一的碳源),因此选择了其中两个进行进一步研究。在自然诱导条件下(木聚糖生长),尽管木聚糖酶2 mRNA信号明显增强,但与野生型相比,转化子的胞外酶水平仅略高(5-10%)。经SDS-PAGE验证的酶分析结果表明,转化体中没有细胞内木聚糖酶2的积累,表明在转录后或翻译后水平存在潜在的调节作用。在使用玉米芯或麦麸作为唯一碳源的简单CBP系统中,评估了转化体的发酵性能并与野生型进行了比较。与野生型玉米芯相比,这两种转化体产生的乙醇含量高出约60%,而对于麦麸,仅其中之一重复了此图。该结果归因于转化子的发酵液中的高细胞外木聚糖酶活性,与野生型相比,其保持高2-2.5倍

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