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Development of a multipurpose scaffold for the display of peptide loops

机译:开发用于展示肽环的多功能支架

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摘要

Protein–protein interactions (PPIs) determine a wide range of biological processes and analysis of these dynamic networks is increasingly becoming a mandatory tool for studying protein function. Using the globular ATPase domain of recombinase RadA as a scaffold, we have developed a peptide display system (RAD display), which allows for the presentation of target peptides, protein domains or full-length proteins and their rapid recombinant production in bacteria. The design of the RAD display system includes differently tagged versions of the scaffold, which allows for flexibility in the protein purification method, and chemical coupling for small molecule labeling or surface immobilization. When combined with the significant thermal stability of the RadA protein, these features create a versatile multipurpose scaffold system. Using various orthogonal biophysical techniques, we show that peptides displayed on the scaffold bind to their natural targets in a fashion similar to linear parent peptides. We use the examples of CK2β/CK2α kinase and TPX2/Aurora A kinase protein complexes to demonstrate that the peptide displayed by the RAD scaffold can be used in PPI studies with the same binding efficacy but at lower costs compared with their linear synthetic counterparts.
机译:蛋白质间相互作用(PPI)决定了广泛的生物学过程,对这些动态网络的分析正日益成为研究蛋白质功能的必不可少的工具。使用重组酶RadA的球状ATPase域作为支架,我们开发了一种肽展示系统(RAD展示),该系统可用于呈递目标肽,蛋白结构域或全长蛋白,并在细菌中快速重组生产。 RAD展示系统的设计包括支架的不同标记版本,从而允许灵活的蛋白质纯化方法以及用于小分子标记或表面固定的化学偶联。当与RadA蛋白的显着热稳定性相结合时,这些功能将创建一个通用的多功能支架系统。使用各种正交生物物理技术,我们显示了在支架上显示的肽以类似于线性亲本肽的方式与它们的天然靶标结合。我们以CK2β/CK2α激酶和TPX2 / Aurora A激酶蛋白复合物为例,证明RAD支架展示的肽可用于PPI研究,具有相同的结合功效,但与线性合成类似物相比,成本较低。

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