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使用蛋白质聚集和 NMR 光谱学鉴定相互作用伙伴。

Identification of interaction partners using protein aggregation and NMR spectroscopy.

机构信息

Department of Chemistry, Sejong University, Seoul, Korea.

出版信息

PLoS One. 2022 Sep 9;17(9):e0270058. doi: 10.1371/journal.pone.0270058. eCollection 2022.

Abstract

The interaction among proteins is one of the most fundamental methods of information transfer in the living system. Many methods have been developed in order to identify the interaction pairs or groups either in vivo or in vitro. The in vitro pulldown/coprecipitation assay directly observes the protein that binds to the target. This method involves electrophoresis, which is a technique of a low resolution as well as a low throughput. As a better alternative, we wish to propose a new method that is based on the NMR spectroscopy. This method utilizes the aggregation of the target protein and the concomitant signal disappearance of the interacting partner. The aggregation is accomplished by the elastin-like polypeptide, which is fused to the target. If a protein binds to this supramolecular complex, its NMR signal then becomes too broadened in order to be observed, which is the basic phenomenon of the NMR spectroscopy. Thus, the protein that loses its signal is the one that binds to the target. A compound that interferes with these types of bindings among the proteins can be identified by observing the reappearance of the protein signals with the simultaneous disappearance of the signals of the compound. This technique will be applied in order to find an interaction pair in the information transfer pathway as well as a compound that disrupts it. This proposed method should be able to work with a mixture of proteins and provide a higher resolution in order to find the binding partner in a higher throughput fashion.

摘要

蛋白质之间的相互作用是生命系统中信息传递的最基本方法之一。为了在体内或体外识别相互作用的对或组,已经开发了许多方法。体外下拉/共沉淀测定法直接观察与靶标结合的蛋白质。该方法涉及电泳,电泳是一种分辨率低、通量低的技术。作为更好的选择,我们希望提出一种基于 NMR 光谱的新方法。该方法利用靶蛋白的聚集以及相互作用伙伴的伴随信号消失。通过与靶标融合的弹性蛋白样多肽来实现聚集。如果蛋白质与这种超分子复合物结合,其 NMR 信号会变宽而无法观察到,这是 NMR 光谱的基本现象。因此,失去信号的蛋白质就是与靶标结合的蛋白质。通过观察化合物信号的同时消失,以及蛋白质信号的重现,可以鉴定出干扰这些蛋白质之间相互作用的化合物。该技术将应用于寻找信息传递途径中的相互作用对以及破坏它的化合物。该方法应该能够与蛋白质混合物一起使用,并提供更高的分辨率,以便以更高的通量找到结合伴侣。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5d66/9462707/4a351e8827f0/pone.0270058.g001.jpg

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