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首页> 外文期刊>Applied biochemistry and biotechnology, Part A. enzyme engineering and biotechnology >Expression and secretion of the human erythropoietin using an optimized cbh1 promoter and the native CBH i signal sequence in the industrial fungus Trichoderma reesei
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Expression and secretion of the human erythropoietin using an optimized cbh1 promoter and the native CBH i signal sequence in the industrial fungus Trichoderma reesei

机译:使用优化的cbh1启动子和天然CBH i信号序列在工业真菌里氏木霉中表达和分泌人类促红细胞生成素

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摘要

The human erythropoietin (HuEPO) structural gene was fused with the secretion signal of the Trichoderma reesei cellobiohydrolase I and controlled by a newly optimized cbh1 promoter in an integrated expression vector pTrCBH-EPO. The recombinant HuEPO construct was transformed into two different T. reesei strains, a protease-deficient strain RutC-30 M3, and a glycosylation-modified strain T108. After lactose induction, the heterologous rHuEPO was found to be stably expressed in the selected transformants T47 (derived from RutC-30 M3) and T112 (derived from T108), which were shown to have high genetic stability. Secretion of erythropoietin in these transformants was further confirmed by SDS-PAGE and western blot analysis. Moreover, the secreted rHuEPO from T112 had an apparent molecular weight of 32 kDa, which was higher than from T47 (28 kDa) and similar to that of mammals (more than 30 kDa). These results demonstrate the potential of using industrial filamentous fungi for the production of human-derived erythropoietin.
机译:人促红细胞生成素(HuEPO)结构基因与里氏木霉纤维二糖水解酶I的分泌信号融合,并在整合表达载体pTrCBH-EPO中由新优化的cbh1启动子控制。重组的HuEPO构建体被转化为两个不同的里氏木霉菌株,蛋白酶缺陷菌株RutC-30 M3和糖基化修饰的菌株T108。乳糖诱导后,发现异源rHuEPO在选定的转化体T47(衍生自RutC-30M3)和T112(衍生自T108)中稳定表达,显示具有高的遗传稳定性。通过SDS-PAGE和蛋白质印迹分析进一步证实了这些转化体中促红细胞生成素的分泌。此外,T112分泌的rHuEPO的表观分子量为32 kDa,高于T47的分子量(28 kDa),与哺乳动物的相似(超过30 kDa)。这些结果证明了使用工业丝状真菌生产人源促红细胞生成素的潜力。

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