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Comparative Production Analysis of Three Phlebovirus Nucleoproteins under Denaturing or Non-Denaturing Conditions for Crystallographic Studies

机译:在变性或非变性条件下三种噬菌体病毒核蛋白的比较生产分析,用于晶体学研究

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摘要

Nucleoproteins (NPs) encapsidate the Phlebovirus genomic (-)RNA. Upon recombinant expression, NPs tend to form heterogeneous oligomers impeding characterization of the encapsidation process through crystallographic studies. To overcome this problem, we set up a standard protocol in which production under both non-denaturing and denaturing/refolding conditions can be investigated and compared. The protocol was applied for three phlebovirus NPs, allowing an optimized production strategy for each of them. Remarkably, the Rift Valley fever virus NP was purified as a trimer under native conditions and yielded protein crystals whereas the refolded version could be purified as a dimer. Yields of trimeric Toscana virus NP were higher from denaturing than from native condition and lead to crystals. The production of Sandfly Fever Sicilian virus NP failed in both protocols. The comparative protocols described here should help in rationally choosing between denaturing or non-denaturing conditions, which would finally result in the most appropriate and relevant oligomerized protein species. The structure of the Rift Valley fever virus NP has been recently published using a refolded monomeric protein and we believe that the process we devised will contribute to shed light in the genome encapsidation process, a key stage in the viral life cycle.
机译:核蛋白(NPs)包裹了噬菌病毒基因组(-)RNA。重组表达后,NPs倾向于形成异质寡聚体,阻碍通过结晶学研究表征衣壳化过程。为了克服这个问题,我们建立了一个标准协议,其中可以研究和比较在非变性和变性/复性条件下的生产。该协议已应用于三个静脉病毒NP,从而为每个NP优化了生产策略。值得注意的是,裂谷热病毒NP在天然条件下被纯化为三聚体,并产生蛋白质晶体,而重折叠的版本可被纯化为二聚体。变性的三聚体托斯卡纳病毒NP的产量高于天然条件,并导致结晶。在两种方案中,桑德弗热西西里病毒NP的生产均失败。本文所述的比较方案应有助于合理选择变性或非变性条件,这将最终导致最合适和最相关的寡聚蛋白质种类。裂谷热病毒NP的结构最近已经使用一种折叠的单体蛋白发表,我们相信我们设计的过程将有助于阐明基因组衣壳化过程,这是病毒生命周期的关键阶段。

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