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利用顺磁扰动快速探索螺旋膜蛋白的折叠拓扑结构。

Rapid exploration of the folding topology of helical membrane proteins using paramagnetic perturbation.

机构信息

Division of Magnetic Resonance, Korea Basic Science Institute (KBSI), Yangcheong-Ri, Ochang, Chungbuk 363-883, Korea.

出版信息

Protein Sci. 2010 Dec;19(12):2409-17. doi: 10.1002/pro.521. Epub 2010 Nov 11.

Abstract

An understanding of the folding states of α-helical membrane proteins in detergent systems is important for functional and structural studies of these proteins. Here, we present a rapid and simple method for identification of the folding topology and assembly of transmembrane helices using paramagnetic perturbation in nuclear magnetic resonance spectroscopy. By monitoring the perturbation of signals from glycine residues located at specific sites, the folding topology and the assembly of transmembrane helices of membrane proteins were easily identified without time-consuming backbone assignment. This method is validated with Mistic (membrane-integrating sequence for translation of integral membrane protein constructs) of known structure as a reference protein. The folding topologies of two bacterial histidine kinase membrane proteins (SCO3062 and YbdK) were investigated by this method in dodecyl phosphocholine (DPC) micelles. Combing with analytical ultracentrifugation, we identified that the transmembrane domain of YbdK is present as a parallel dimer in DPC micelle. In contrast, the interaction of transmembrane domain of SCO3062 is not maintained in DPC micelle due to disruption of native structure of the periplasmic domain by DPC micelle.

摘要

了解 α-螺旋膜蛋白在去污剂系统中的折叠状态对于这些蛋白质的功能和结构研究非常重要。在这里,我们提出了一种使用核磁共振波谱中的顺磁扰动快速简便地鉴定跨膜螺旋折叠拓扑结构和组装的方法。通过监测位于特定位置的甘氨酸残基信号的扰动,可以轻松识别膜蛋白的折叠拓扑结构和跨膜螺旋的组装,而无需耗时的骨架分配。该方法以已知结构的 Mistic(整合膜蛋白构建体翻译的膜整合序列)作为参考蛋白进行了验证。通过该方法在十二烷基磷酸胆碱(DPC)胶束中研究了两种细菌组氨酸激酶膜蛋白(SCO3062 和 YbdK)的折叠拓扑结构。结合分析超速离心,我们确定 YbdK 的跨膜结构域在 DPC 胶束中呈平行二聚体存在。相比之下,由于 DPC 胶束破坏了周质域的天然结构,SCO3062 的跨膜结构域在 DPC 胶束中不再相互作用。

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