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Intein mediated hyper-production of authentic human basic fibroblast growth factor in Escherichia coli

机译:内含肽介导的大肠杆菌中人源碱性成纤维细胞生长因子的过度生产

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摘要

Human basic fibroblast growth factor is a functionally versatile but very expensive polypeptide. In this communication, employing a novel amplification method for the target gene and genetic optimization of a previously engineered expression construct, pWK3R, together with a refined fed-batch fermentation protocol, we report an achievement of a phenomenal yield of 610 mg/L of the 146 aa authentic human basic fibroblast growth factor (bFGF) in Escherichia coli. Construct pWK3R was first modified to form plasmid pWK311ROmpAd, which was devoid of the ompA leader sequence and possessed two copies of a DNA segment encoding a fusion product comprising an intein, Saccharomyces cerevisiae vascular membrane ATPase (VMA), and bFGF. When E. coli transformant JM101 [pWK311ROmpAd] was cultivated using the refined fed-batch fermentation protocol, superb expression resulting in a total yield of 610 mg/L of bFGF was detected. Despite existing in high levels, the bFGF remained to be soluble and highly bioactive.
机译:人碱性成纤维细胞生长因子是一种功能多样但非常昂贵的多肽。在这次交流中,采用一种新颖的靶基因扩增方法,对先前设计的表达构建体pWK3R进行了遗传优化,再加上完善的分批补料发酵方案,我们报道了610 mg / L的惊人产量。 146 aa在大肠杆菌中的真实人碱性成纤维细胞生长因子(bFGF)。首先修饰构建体pWK3R以形成质粒pWK311ROmpAd,其没有ompA前导序列,并且具有两个DNA片段的拷贝,该DNA片段编码包含内含蛋白,酿酒酵母血管膜ATP酶(VMA)和bFGF的融合产物。当使用改良的分批补料发酵方案培养大肠杆菌转化体JM101 [pWK311ROmpAd]时,检测到高表达,导致bFGF的总产量为610μmg/ L。尽管存在高水平,但是bFGF仍然是可溶的并且具有高生物活性。

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