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首页> 外文期刊>Process Biochemistry >Soluble overexpression, high-level production and purification of receptor binding domain of human VEGF_(8-109) in E. coli
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Soluble overexpression, high-level production and purification of receptor binding domain of human VEGF_(8-109) in E. coli

机译:在大肠杆菌中,可溶性过度表达,高级别的人VEGF_(8-109)的受体结合结构域的纯化

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摘要

The high-yield production of vascular endothelial growth factor (VEGF), as a major therapeutic target in pathological angiogenesis and diabetic wound healing, provides critical advantages for in vitro studies. In the present study, to improve the soluble production of human VEGF(8-109) (receptor-binding domain (RBD) of VEGF or VEGF RBD), at first VEGF(8-109) encoded gene was expressed in SHuffle T7 E. coli. Moreover, in two steps, the protein production was optimized based on Taguchi design, by evaluating optimal levels of various induction parameters, such as cell density in induction time, temperature, inducer concentration, and media components. The results indicated that the highest amount of the protein was achieved in TB medium containing glycerol 6 g L-1, peptone to yeast extract ratio 1:1, ethanol 3% and MgSO4 4 g L-1, under inducing with 0.05 mM IPTG in OD600 of 0.7 at 24 degrees C for 22 h. The bioactivity of the purified protein was confirmed by cell proliferation assay. Finally, bench-scale production of VEGF(8-109) was performed under the optimum conditions and resulted in 182 mg of soluble VEGF(8-109) expressed per liter. Totally, our results can be considered as a basis for economical production of the recombinant VEGF in future.
机译:血管内皮生长因子(VEGF)的高产量产生,作为病理血管生成和糖尿病伤口愈合的主要治疗靶标,为体外研究提供了关键优势。在本研究中,为了改善人VEGF(8-109)的可溶性产生(VEGF或VEGF RBD的受体结合结构域(RBD)),在第一个VEGF(8-109)中,在洗涤T7 E中表达编码基因。大肠杆菌。此外,在两个步骤中,通过评估诱导时间,温度,诱导剂浓度和介质组分等各种诱导参数的最佳水平,基于Taguchi设计进行了优化了蛋白质产生。结果表明,在含有甘油6g L-1的Tb培养基中达到最高量,蛋白胨至酵母提取物比例1:1,乙醇3%和MgSO 4 4g L-1,诱导0.05mm IPTG OD600在24℃下为0.7℃。通过细胞增殖测定证实纯化蛋白的生物活性。最后,在最佳条件下进行VEGF(8-109)的长度制作,并产生每升182毫克可溶性VEGF(8-109)。完全,我们的结果可被视为未来重组VEGF经济生产的基础。

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