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金黄色葡萄球菌截短 AgrC 组氨酸激酶在模型膜系统中的功能重建。

Functional reconstitution of Staphylococcus aureus truncated AgrC histidine kinase in a model membrane system.

机构信息

Dalian Institute of Chemical Physics, Chinese Academy of Sciences, Dalian, China.

出版信息

PLoS One. 2013 Nov 26;8(11):e80400. doi: 10.1371/journal.pone.0080400. eCollection 2013.

Abstract

The integral membrane protein AgrC is a histidine kinase whose sensor domains interact with an autoinducing peptide, resulting in a series of downstream responses. In this study, truncated AgrCTM5-6C and AgrCTM5-6C-GFP with GFP as a reporter gene were produced using a bacterial system. Purified AgrCTM5-6C and AgrCTM5-6C-GFP were reconstituted into liposomes by a detergent-mediated method. To achieve high-yield protein incorporation, we investigated the effect of different detergents on protein reconstitution efficiency. The highest incorporation was found with N,N-dimethyldode-cylamine N-oxide during complete liposome solubilization, which resulted in a yield of 85±5%. The COOH-terminus of the protein AgrCTM5-6C was almost exclusively oriented towards the inside of the vesicles. AgrCTM5-6C in proteoliposomes exhibited approximately a 6-fold increase in constitutive activity compared with AgrCTM5-6C in detergent micelles. The reconstitution of AgrCTM5-6C or AgrCTM5-6C-GFP was characterized using dynamic light scattering, fluorescence microscopy, and transmission electron microscopy. Based on the results, the optimal conditions for protein incorporation were defined. These findings contribute to the study of membrane protein structure and function in vitro using a reconstitution system.

摘要

整合膜蛋白 AgrC 是一种组氨酸激酶,其传感器结构域与自动诱导肽相互作用,导致一系列下游反应。在本研究中,使用细菌系统产生了带有 GFP 作为报告基因的截断 AgrCTM5-6C 和 AgrCTM5-6C-GFP。通过去污剂介导的方法将纯化的 AgrCTM5-6C 和 AgrCTM5-6C-GFP 重构成脂质体。为了实现高产量的蛋白质掺入,我们研究了不同去污剂对蛋白质重组成效率的影响。在完全脂质体溶解过程中,使用 N,N-二甲基十二烷基氧化胺(N,N-dimethyldodecylamine N-oxide)可获得最高的掺入率,达到 85±5%。该蛋白 AgrCTM5-6C 的 COOH 末端几乎完全朝向囊泡内部。与去污剂胶束中的 AgrCTM5-6C 相比,在质体脂质体中的 AgrCTM5-6C 表现出约 6 倍的组成型活性增加。使用动态光散射、荧光显微镜和透射电子显微镜对 AgrCTM5-6C 或 AgrCTM5-6C-GFP 的重组成分进行了表征。基于这些结果,确定了蛋白质掺入的最佳条件。这些发现为使用重组系统研究膜蛋白的结构和功能提供了参考。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e8d9/3841183/963c6c02a654/pone.0080400.g001.jpg

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