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Enhanced Heterologous Protein Production In Aspergillus niger Fermentation Through Protease Inhibition Using Bioprocess Enigneering Strategies

机译:黑曲霉发酵中通过蛋白酶抑制生物过程工程提高异源蛋白生产。

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Filamentous fungal organisms such as A. niger are attractive hosts for the production of heterologous proteins due to their advantageous growth characteristics, their ability to perform correct posttranlational modification such as glycosylation, and to secrete high levels of protein production into the medium (van den Hombergh et al., 1997). However, heterologous protein secretion is often severely hampered by fungal proteases. Several biological strategies have been developed to increase these yields. Those employed include the introduction of a large number of gene copies (Withers et al., 1998), the use of strong promoters and efficient fungal secretion signals (Archer et al., 1997) and the developmetn of protease-deficient host strains (van den Hombergh et al., 1997). One of the most successful strategies involves the construction of gene fusion of the target gene to a highly expressed fungal gene, such as glucoamylase (Ward et al., 1990). The resulting fusion protein progresses through the fungal secretory pathway like the normal, homologous protein, before separation in the external medium. However, even with successful secretion of higher levels of heterologous proteins, the problem of proteolytic degradation by extracellular proteases still remains.
机译:由于其有利的生长特性,它们执行正确的翻译后修饰(例如糖基化)以及将高水平蛋白质生产分泌到培养基中的能力,丝状真菌生物(例如黑曲霉)是产生异源蛋白质的有吸引力的宿主。等人,1997)。但是,真菌蛋白酶常常严重地阻碍了异源蛋白的分泌。已经开发了几种生物学策略来增加这些产量。所采用的方法包括引入大量基因拷贝(Withers等,1998),使用强启动子和有效的真菌分泌信号(Archer等,1997)以及蛋白酶缺陷型宿主菌株的发展(van den Hombergh et al。,1997)。最成功的策略之一涉及构建靶基因与高度表达的真菌基因,例如葡糖淀粉酶的基因融合体(Ward等,1990)。产生的融合蛋白在正常情况下会通过真菌分泌途径(与正常的同源蛋白一样)传播,然后在外部培养基中分离。然而,即使成功分泌了更高水平的异源蛋白质,仍然存在细胞外蛋白酶引起的蛋白水解降解的问题。

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