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使用 SpyTag/SpyCatcher 蛋白连接系统进行依赖于可及性的膜蛋白拓扑结构研究。

Accessibility-dependent topology studies of membrane proteins using a SpyTag/SpyCatcher protein-ligation system.

机构信息

Department of Biological Sciences, Ulsan National Institute of Science and Technology (UNIST), Ulsan 44919, Republic of Korea.

Department of Biological Sciences, Ulsan National Institute of Science and Technology (UNIST), Ulsan 44919, Republic of Korea.

出版信息

Int J Biol Macromol. 2021 Apr 1;175:171-178. doi: 10.1016/j.ijbiomac.2021.02.015. Epub 2021 Feb 4.

DOI:10.1016/j.ijbiomac.2021.02.015
PMID:33549659
Abstract

Covalent protein-ligation methods were used not only to visualize the localization of proteins of interest in cells, but also to study the topology of plasma and subcellular organelle membrane proteins using fluorescent cell imaging. A 13-amino-acid SpyTag (ST) peptide was genetically introduced either into a variety of subcellular proteins of interest or into different positions of plasma or subcellular organelle membrane proteins individually. Conversely, a 15 kDa SpyCatcher (SC) protein was chemically conjugated with either fluorescent dyes or horseradish peroxidase (HRP) via a thiol-maleimide reaction. The extracellular ST-fused plasma membrane proteins were efficiently labeled with the fluorescent-dye-conjugated SC in both live and permeabilized cells, whereas the intracellularly localized ST-fused subcellular proteins were only labeled in permeabilized cells because of the limited accessibility of the fluorescent-dye-conjugated SC to the membrane. The fluorescent-dye-labeled SC together with selective membrane-permeabilizing agents successfully labeled the plasma or the subcellular organelle membrane proteins in a topology-dependent manner. Moreover, the HRP-conjugated SC not only successfully labeled the ST-fused plasma membrane proteins, thus significantly enhancing fluorescent signals in combination with the tyramide signal amplification agents, but also ligated with an external ST-fused target ligand, thus selectively binding to the endogenously expressed cellular receptors of the target cancer cells.

摘要

共价蛋白连接方法不仅用于可视化细胞中感兴趣的蛋白质的定位,还用于使用荧光细胞成像研究质膜和亚细胞器膜蛋白的拓扑结构。将 13 个氨基酸的 SpyTag (ST) 肽基因引入各种感兴趣的亚细胞蛋白中,或单独引入质膜或亚细胞器膜蛋白的不同位置。相反,通过硫醇-马来酰亚胺反应,将 15 kDa 的 SpyCatcher (SC) 蛋白与荧光染料或辣根过氧化物酶 (HRP) 化学偶联。在活细胞和透化细胞中,荧光染料偶联的 SC 可有效地标记细胞外融合了 ST 的质膜蛋白,而在透化细胞中仅可标记细胞内定位的融合了 ST 的亚细胞蛋白,因为荧光染料偶联的 SC 对膜的可及性有限。荧光染料标记的 SC 与选择性的膜通透剂一起,以依赖拓扑的方式成功标记质膜或亚细胞器膜蛋白。此外,HRP 偶联的 SC 不仅成功标记了融合了 ST 的质膜蛋白,从而与辣根过氧化物酶信号放大试剂结合显著增强了荧光信号,而且还与外部融合了 ST 的靶标配体连接,从而选择性地结合到靶癌细胞的内源性表达的细胞受体。

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