Expression, purification and refolding of pro-MMP-2 from inclusion bodies of E. coli

包涵体 重组DNA 化学 生物化学 大肠杆菌 蛋白质纯化 酶谱 分馏 靶蛋白 色谱法 分子生物学 生物 基因
作者
Yu Nan Zhang,Jia Jian Liu,Wei Zhang,Han Qin,Lintao Wang,Yuan Yuan Chen,Yuan Li,Fang Yang,Rong Cao,Xue Jun Wang
出处
期刊:Protein Expression and Purification [Elsevier]
卷期号:208-209: 106278-106278 被引量:1
标识
DOI:10.1016/j.pep.2023.106278
摘要

MMP-2 has been reported as the most validated target for cancer progression and deserves further investigation. However, due to the lack of methods for obtaining large amounts of highly purified and bioactive MMP-2, identifying specific substrates and developing specific inhibitors of MMP-2 remains extremely difficult. In this study, the DNA fragment coding for pro-MMP-2 was inserted into plasmid pET28a in an oriented manner, and the resulting recombinant protein was effectively expressed and led to accumulation as inclusion bodies in E. coli. This protein was easy to purify to near homogeneity by the combination of common inclusion bodies purification procedure and cold ethanol fractionation. Then, our results of gelatin zymography and fluorometric assay revealed that pro-MMP-2 at least partially restored its natural structure and enzymatic activity after renaturation. We obtained approximately 11 mg refolded pro-MMP-2 protein from 1 L LB broth, which was higher than other strategies previously reported. In conclusion, a simple and cost-effective procedure for obtaining high amounts of functional MMP-2 was developed, which would contribute to the progress of studies on the gamut of biological action of this important proteinase. Furthermore, our protocol should be appropriate for the expression, purification, and refolding of other bacterial toxic proteins.
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