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Purification of a Multidrug Resistance Transporter for Crystallization Studies

机译:纯化用于结晶研究的多药耐药转运蛋白

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Crystallization of integral membrane proteins is a challenging field and much effort has been invested in optimizing the overexpression and purification steps needed to obtain milligram amounts of pure, stable, monodisperse protein sample for crystallography studies. Our current work involves the structural and functional characterization of the Escherichia coli multidrug resistance transporter MdtM, a member of the major facilitator superfamily (MFS). Here we present a protocol for isolation of MdtM to increase yields of recombinant protein to the milligram quantities necessary for pursuit of structural studies using X-ray crystallography. Purification of MdtM was enhanced by introduction of an elongated His-tag, followed by identification and subsequent removal of chaperonin contamination. For crystallization trials of MdtM, detergent screening using size exclusion chromatography determined that decylmaltoside (DM) was the shortest-chain detergent that maintained the protein in a stable, monodispersed state. Crystallization trials of MdtM performed using the hanging-drop diffusion method with commercially available crystallization screens yielded 3D protein crystals under several different conditions. We contend that the purification protocol described here may be employed for production of high-quality protein of other multidrug efflux members of the MFS, a ubiquitous, physiologically and clinically important class of membrane transporters.
机译:整合膜蛋白的结晶是一个充满挑战的领域,并且已经投入大量精力来优化过表达和纯化步骤,以获取毫克量的用于晶体学研究的纯净,稳定,单分散的蛋白质样品。我们目前的工作涉及大肠杆菌多药抗性转运蛋白MdtM(主要促进子超家族(MFS)的成员)的结构和功能表征。在这里,我们提出了一种分离MdtM的方案,以将重组蛋白的产量提高到使用X射线晶体学进行结构研究所需的毫克量。 MdtM的纯化通过引入细长的His标签,随后鉴定和随后去除伴侣蛋白污染而得到增强。对于MdtM的结晶试验,使用尺寸排阻色谱法进行去污剂筛选确定癸基麦芽糖苷(DM)是最短链的去污剂,可将蛋白质保持在稳定的单分散状态。 MdtM的结晶试验使用吊滴扩散法和可商购的结晶屏幕进行,在几种不同条件下产生了3D蛋白晶体。我们认为此处描述的纯化方案可用于生产MFS的其他多药外排成员的高质量蛋白质,MFS是普遍存在的,生理上和临床上重要的一类膜转运蛋白。

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