Measuring ligand-cell surface receptor affinities with axial line-scanning fluorescence correlation spectroscopy

被引:23
|
作者
Eckert, Antonia Franziska [1 ]
Gao, Peng [1 ,2 ,5 ]
Wesslowski, Janine [3 ]
Wang, Xianxian [3 ]
Rath, Jasmijn [1 ]
Nienhaus, Karin [1 ]
Davidson, Gary [3 ]
Nienhaus, Gerd Ulrich [1 ,2 ,3 ,4 ]
机构
[1] Karlsruhe Inst Technol, Inst Appl Phys, Karlsruhe, Germany
[2] Karlsruhe Inst Technol, Inst Nanotechnol, Karlsruhe, Germany
[3] Karlsruhe Inst Technol, Inst Biol & Chem Syst, Karlsruhe, Germany
[4] Univ Illinois, Dept Phys, Urbana, IL 61801 USA
[5] Xidian Univ, Sch Phys & Optoelect Engn, Xian, Peoples R China
来源
ELIFE | 2020年 / 9卷
关键词
KREMEN PROTEINS; WNT; ACTIVATION; MECHANISM; COMPLEX; BINDING; MICROSCOPY; DICKKOPF-1; REVEALS; DOMAINS;
D O I
10.7554/eLife.55286
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Development and homeostasis of multicellular organisms is largely controlled by complex cell-cell signaling networks that rely on specific binding of secreted ligands to cell surface receptors. The Wnt signaling network, as an example, involves multiple ligands and receptors to elicit specific cellular responses. To understand the mechanisms of such a network, ligand-receptor interactions should be characterized quantitatively, ideally in live cells or tissues. Such measurements are possible using fluorescence microscopy yet challenging due to sample movement, low signal-to-background ratio and photobleaching. Here, we present a robust approach based on fluorescence correlation spectroscopy with ultra-high speed axial line scanning, yielding precise equilibrium dissociation coefficients of interactions in the Wnt signaling pathway. Using CRISPR/Cas9 editing to endogenously tag receptors with fluorescent proteins, we demonstrate that the method delivers precise results even with low, near-native amounts of receptors.
引用
收藏
页码:1 / 92
页数:29
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