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An optimized Npro-based method for the expression and purification of intrinsically disordered proteins for an NMR study

机译:一种基于Npro的优化方法用于表达和纯化内在无序的蛋白质用于NMR研究

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摘要

Intrinsically disordered proteins (IDPs) are an emerging concept. IDPs have high flexibility in their polypeptide chains, lacking a stable 3-dimensional structure. Because of the difficulty in performing X-ray crystallography for IDPs, nuclear magnetic resonance (NMR) spectroscopy is the first choice for atomic-level investigation of their nature. Given that isotopically labeled IDP samples are necessary for NMR study, a robust and cost-effective protocol for bacterial expression and purification of IDP is also needed. We employed the Npro (EDDIE)-autoprotease fusion protein system. Although IDPs are believed to be readily degraded by endogenous proteases when expressed in Escherichia coli, Npro-fused IDPs showed excellent resistance to degradation. Seven IDPs of uncharacterized function sampled from the human genome as well as 3 constructs from IDP regions derived from human FancM and Thermococcus kodakarensis Hef were prepared. We improved the protocol of refolding of Npro (EDDIE) to use dialysis, which is convenient for subsequent purification using reversed-phase (RP) HPLC. The method is robust and widely applicable to any IDP sample, promoting the acquisition of experimental data for IDPs in a high-throughput manner.
机译:本质上无序的蛋白质(IDP)是一个新兴的概念。 IDP在其多肽链中具有高度的灵活性,缺乏稳定的3维结构。由于对IDP进行X射线晶体学分析很困难,因此核磁共振(NMR)光谱学是对其性质进行原子级研究的首选。鉴于同位素标记的IDP样品对于NMR研究是必需的,因此还需要一种健壮且经济高效的方案来进行细菌表达和IDP的纯化。我们使用了N pro (EDDIE)-自动蛋白酶融合蛋白系统。尽管IDP被认为在大肠杆菌中表达时很容易被内源蛋白酶降解,但是N ro> sup>融合的IDP显示出极好的抗降解性。制备了从人类基因组中取样的七个未鉴定功能的IDP,以及来自人FancM和kodkarensis Hefcoccus kodakarensis Hef的IDP区域的3个构建体。我们改进了N pro (EDDIE)的重折叠方案以使用透析,这便于后续使用反相(RP)HPLC进行纯化。该方法是鲁棒的,并且广泛适用于任何IDP样品,从而以高通量方式促进了IDP实验数据的获取。

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