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利用卷曲螺旋标记法对膜蛋白进行活细胞成像——原理与应用。

Live-cell imaging of membrane proteins by a coiled-coil labeling method-Principles and applications.

机构信息

Graduate School of Pharmaceutical Sciences, Kyoto University, 46-29 Yoshida-Shimoadachi-cho, Sakyo-ku, Kyoto 606-8501, Japan.

Graduate School of Pharmaceutical Sciences, Kyoto University, 46-29 Yoshida-Shimoadachi-cho, Sakyo-ku, Kyoto 606-8501, Japan.

出版信息

Biochim Biophys Acta Biomembr. 2019 May 1;1861(5):1011-1017. doi: 10.1016/j.bbamem.2019.02.009. Epub 2019 Mar 1.

DOI:10.1016/j.bbamem.2019.02.009
PMID:30831076
Abstract

In situ investigations in living cell membranes are important to elucidate the dynamic behaviors of membrane proteins in complex biomembrane environments. Protein-specific labeling is a key technique for the detection of a target protein by fluorescence imaging. The use of post-translational labeling methods using a genetically encodable tag and synthetic probes targeting the tag offer a smaller label size, labeling with synthetic fluorophores, and precise control of the labeling ratio in multicolor labeling compared with conventional genetic fusions with fluorescent proteins. This review focuses on tag-probe labeling studies for live-cell analysis of membrane proteins based on heterodimeric peptide pairs that form coiled-coil structures. The robust and simple peptide-peptide interaction enables not only labeling of membrane proteins by noncovalent interactions, but also covalent crosslinking and acyl transfer reactions guided by coiled-coil assembly. A number of studies have demonstrated that membrane protein behaviors in live cells, such as internalization of receptors and the oligomeric states of various membrane proteins (G-protein-coupled receptors, epidermal growth factor receptors, influenza A M2 channel, and glycopholin A), can be precisely analyzed using coiled-coil labeling, indicating the potential of this labeling method in membrane protein research.

摘要

在活细胞膜中进行原位研究对于阐明复杂生物膜环境中膜蛋白的动态行为非常重要。蛋白质特异性标记是通过荧光成像检测靶蛋白的关键技术。与传统的荧光蛋白基因融合相比,使用带有遗传编码标签的翻译后标记方法和针对该标签的合成探针提供了更小的标记大小、用合成荧光团进行标记以及在多色标记中精确控制标记比。本文综述了基于形成卷曲螺旋结构的异二聚体肽对的膜蛋白活细胞分析的标签-探针标记研究。这种稳定而简单的肽-肽相互作用不仅可以通过非共价相互作用对膜蛋白进行标记,还可以通过卷曲螺旋组装引导共价交联和酰基转移反应。许多研究表明,使用卷曲螺旋标记可以精确分析活细胞中膜蛋白的行为,如受体的内化和各种膜蛋白(G 蛋白偶联受体、表皮生长因子受体、流感 A M2 通道和糖蛋白 A)的寡聚状态,这表明该标记方法在膜蛋白研究中的潜力。

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