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使用基质金属蛋白酶2(MMP2)的“形式不变”检测法进行基质辅助重折叠、纯化及活性评估。

Matrix-assisted refolding, purification and activity assessment using a 'form invariant' assay for matrix metalloproteinase 2 (MMP2).

作者信息

Singh Krishna Kumar, Jain Ruchi, Ramanan Harini, Saini Deepak Kumar

机构信息

Department of Molecular Reproduction, Development and Genetics, Indian Institute of Science, Bangalore, 560012, India.

出版信息

Mol Biotechnol. 2014 Dec;56(12):1121-32. doi: 10.1007/s12033-014-9792-7.

Abstract

Matrix metalloproteinases expression is used as biomarker for various cancers and associated malignancies. Since these proteinases can cleave many intracellular proteins, overexpression tends to be toxic; hence, a challenge to purify them. To overcome these limitations, we designed a protocol where full length pro-MMP2 enzyme was overexpressed in E. coli as inclusion bodies and purified using 6xHis affinity chromatography under denaturing conditions. In one step, the enzyme was purified and refolded directly on the affinity matrix under redox conditions to obtain a bioactive protein. The pro-MMP2 protein was characterized by mass spectrometry, CD spectroscopy, zymography and activity analysis using a simple in-house developed 'form invariant' assay, which reports the total MMP2 activity independent of its various forms. The methodology yielded higher yields of bioactive protein compared to other strategies reported till date, and we anticipate that using the protocol, other toxic proteins can also be overexpressed and purified from E. coli and subsequently refolded into active form using a one step renaturation protocol.

摘要

基质金属蛋白酶的表达被用作各种癌症及相关恶性肿瘤的生物标志物。由于这些蛋白酶能够切割许多细胞内蛋白质,其过表达往往具有毒性,因此纯化它们颇具挑战。为克服这些限制,我们设计了一种方案,将全长前MMP2酶在大肠杆菌中作为包涵体进行过表达,并在变性条件下使用6xHis亲和色谱法进行纯化。在一步操作中,该酶在氧化还原条件下直接在亲和基质上进行纯化和重折叠,以获得具有生物活性的蛋白质。通过质谱、圆二色光谱、酶谱分析以及使用一种简单的内部开发的“形式不变”测定法进行活性分析,对前MMP2蛋白进行了表征,该测定法可报告总MMP2活性,而不依赖于其各种形式。与迄今报道的其他策略相比,该方法产生的生物活性蛋白产量更高,我们预计使用该方案,其他有毒蛋白质也能够在大肠杆菌中过表达和纯化,并随后通过一步复性方案重折叠成活性形式。

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