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Construction of a cellulase hyper-expression system in Trichoderma reesei by promoter and enzyme engineering

机译:利用启动子和酶工程技术构建里氏木霉纤维素酶超表达系统

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摘要

BackgroundTrichoderma reesei is the preferred organism for producing industrial cellulases. However, a more efficient heterologous expression system for enzymes from different organism is needed to further improve its cellulase mixture. The strong cbh1 promoter of T. reesei is frequently used in heterologous expression, however, the carbon catabolite repressor CREI may reduce its strength by binding to the cbh1 promoter at several binding sites. Another crucial point to enhance the production of heterologous enzymes is the stability of recombinant mRNA and the prevention of protein degradation within the endoplasmic reticulum, especially for the bacteria originated enzymes.In this study, the CREI binding sites within the cbh1 promoter were replaced with the binding sites of transcription activator ACEII and the HAP2/3/5 complex to improve the promoter efficiency. To further improve heterologous expression efficiency of bacterial genes within T. reesei, a flexible polyglycine linker and a rigid α-helix linker were tested in the construction of fusion genes between cbh1 from T. reesei and e1, encoding an endoglucanase from Acidothermus cellulolyticus.
机译:背景技术里氏木霉是用于生产工业纤维素酶的优选生物。然而,需要用于来自不同生物的酶的更有效的异源表达系统,以进一步改善其纤维素酶混合物。里氏木霉的强cbh1启动子经常用于异源表达,但是碳分解代谢物阻遏物CREI可能会通过在几个结合位点与cbh1启动子结合而降低其强度。增强异源酶产生的另一个关键点是重组mRNA的稳定性以及防止内质网中蛋白质降解的能力,特别是对于细菌起源的酶而言。在这项研究中,cbh1启动子内的CREI结合位点被Cbh1启动子取代了。转录激活剂ACEII和HAP2 / 3/5复合物的结合位点,以提高启动子效率。为了进一步提高里氏木霉细菌基因的异源表达效率,在里氏木霉cbh1与e1融合基因的构建中测试了柔性聚甘氨酸接头和刚性α-螺旋接头,该融合基因编码得自解酸嗜酸热菌的内切葡聚糖酶。

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