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Constructing a novel expression system by specific activation of amylase expression pathway in Penicillium

机译:通过特异性激活青霉素淀粉酶表达途径的特异性激活构建新的表达系统

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Filamentous fungi have long been used as hosts for the production of proteins, enzymes and valuable products in various biotechnological applications. However, recombinant proteins are expressed with highly secreted host proteins when stronger promoters are used under inducing conditions. In addition, the efficiency of target protein expression can be limited by the application of constitutive promoters in recently developed filamentous fungal expression systems. In this study, a novel expression system was constructed by using a Penicillium oxalium strain that has powerful protein secretion capability. The secretory background of the host was reduced by knocking out the Amy13A protein and utilizing the starch as a carbon source. The strong promoter amy15A(p) was further improved by overexpressing the transcription activator AmyR and deleting of putative repressor CreA. By using the native amylase Amy15A as a reporter, the efficiency of expression from the amy15A promoter was dramatically and specifically enhanced after redesigning the regulatory network of amylase expression. Our researches clearly indicated that the triple-gene recombinant strain Δ13A-OamyR-ΔCreA, with the amy15A(p) promoter could be used as a suitable expression system especially for high-level and high-purity protein production.
机译:丝状真菌长期以来一直被用作各种生物技术应用中蛋白质,酶和有价值产品的宿主。然而,当在诱导条件下使用较强的启动子时,重组蛋白质用高度分泌的宿主蛋白表达。此外,靶蛋白表达的效率可以通过在最近开发的丝状真菌表达系统中应用组成型启动子来限制。在该研究中,通过使用具有强大的蛋白质分泌能力的青氧鎓氧化菌株来构建新的表达系统。通过敲出AMY13A蛋白并利用淀粉作为碳源来降低宿主的分泌背景。通过过表达转录活化剂Amyr和缺失推定的阻遏物Crea,进一步改善了强启动子AMY15A(P)。通过使用本地淀粉酶AMY15A作为报告者,在重新设计淀粉酶表达的调节网络之后,从AMY15A启动子的表达效率显着,明确地增强。我们的研究清楚地表明,具有AMY15A(P)启动子的三基因重组菌株Δ13A-Oamyr-ΔCrea可用作适当的表达系统,特别是对于高水平和高纯度蛋白质产生。

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