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A systematic assessment of mature MBP in membrane protein production: Overexpression, membrane targeting and purification

机译:对膜蛋白生产中成熟MBP的系统评估:过表达,膜靶向和纯化

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摘要

Obtaining enough membrane protein in native or native-like status is still a challenge in membrane protein structure biology. Maltose binding protein (MBP) has been widely used as a fusion partner in improving membrane protein production. In the present work, a systematic assessment on the application of mature MBP (mMBP) for membrane protein overexpression and purification was performed on 42 membrane proteins, most of which showed no or poor expression level in membrane fraction fused with an N-terminal Histag. It was found that most of the small membrane proteins were overexpressed in the native membrane of Escherichia coli when using mMBP. In addition, the proteolysis of the fusions were performed on the membrane without solubilization with detergents, leading to the development of an efficient protocol to directly purify the target membrane proteins from the membrane fraction through a one-step affinity chromatography. Our results indicated that mMBP is an excellent fusion partner for overexpression, membrane targeting and purification of small membrane proteins. The present expression and purification method may be a good solution for the large scale preparation of small membrane proteins in structural and functional studies.
机译:以天然或类似天然的状态获得足够的膜蛋白仍然是膜蛋白结构生物学的挑战。麦芽糖结合蛋白(MBP)已被广泛用作提高膜蛋白产量的融合伴侣。在目前的工作中,对42种膜蛋白进行了关于成熟MBP(mMBP)在膜蛋白过表达和纯化中的应用的系统评估,其中大多数膜蛋白在与N端Histag融合的膜级分中没有表达或表达水平很低。发现使用mMBP时,大多数小膜蛋白在大肠杆菌的天然膜中过表达。另外,融合物的蛋白水解在膜上进行而无需用去污剂溶解,从而导致开发了一种有效的方案,可通过一步亲和色谱法直接从膜级分中纯化目标膜蛋白。我们的结果表明,mMBP是超表达,膜靶向和小膜蛋白纯化的出色融合伙伴。目前的表达和纯化方法可能是在结构和功能研究中大规模制备小膜蛋白的良好解决方案。

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