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用于生产与SUMO融合的EAK(16)肽的发酵培养基富集及表达条件优化。

Enrichment of fermentation media and optimization of expression conditions for the production of EAK(16) peptide as fusions with SUMO.

作者信息

Satakarni Makkapati, Koutinas Apostolis A, Webb Colin, Curtis Robin

机构信息

School of Chemical Engineering and Analytical Science, The University of Manchester, PO Box 88, Manchester M601QD, United Kingdom.

出版信息

Biotechnol Bioeng. 2009 Feb 15;102(3):725-35. doi: 10.1002/bit.22114.

Abstract

EAK(16) (AEAEAKAKAEAKAEAK) belongs to a novel class of self-assembling peptides, which is being investigated in research and industry. SUMO belongs to the ubiquitin class of proteins and is a promising fusion partner currently in use. In this study, EAK(16) peptide fusions with hexa-histidine tagged SUMO have been constructed using Escherichia coli based pET expression vector. Intracellular expression of the SUMO-EAK(16) fusion using LB media has been optimized. Low-cost complex media (fungal autolysates, wheat and gluten hydrolysates) produced via a novel wheat-based biorefinery have been used as alternative fermentation media to LB. Shake flask cultures using either enriched LB or complex wheat-derived media containing 2 g/L of glucose resulted in intracellular SUMO-EAK(16) fusion protein production of approximately 250 mg/L fermentation volume which corresponded to 30-35% of the total bacterial protein expressed being the fusion protein. Fusion protein productivities up to five times higher were achieved when using a bioreactor.

摘要

EAK(16)(AEAEAKAKAEAKAEAK)属于一类新型的自组装肽,目前正在科研和工业领域进行研究。SUMO属于泛素类蛋白质,是目前正在使用的一种有前景的融合伴侣。在本研究中,使用基于大肠杆菌的pET表达载体构建了与六组氨酸标签SUMO融合的EAK(16)肽。利用LB培养基对SUMO-EAK(16)融合蛋白的胞内表达进行了优化。通过新型小麦生物精炼工艺生产的低成本复合培养基(真菌自溶产物、小麦和麸质水解产物)已被用作LB的替代发酵培养基。使用富含LB或含有2 g/L葡萄糖的复合小麦衍生培养基进行摇瓶培养,胞内SUMO-EAK(16)融合蛋白产量约为每升发酵体积250 mg,相当于表达的总细菌蛋白中30%-35%为融合蛋白。使用生物反应器时,融合蛋白生产率提高了五倍。

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