Abstract
Single-molecule microscopy is emerging as a powerful approach to analyze the behavior of signaling molecules, in particular concerning those aspect (e.g., kinetics, coexistence of different states and populations, transient interactions), which are typically hidden in ensemble measurements, such as those obtained with standard biochemical or microscopy methods. Thus, dynamic events, such as receptor-receptor interactions, can be followed in real time in a living cell with high spatiotemporal resolution. This protocol describes a method based on labeling with small and bright organic fluorophores and total internal reflection fluorescence (TIRF) microscopy to directly visualize single receptors on the surface of living cells. This approach allows one to precisely localize receptors, measure the size of receptor complexes, and capture dynamic events such as transient receptor-receptor interactions. The protocol provides a detailed description of how to perform a single-molecule experiment, including sample preparation, image acquisition and image analysis. As an example, the application of this method to analyze two G-protein-coupled receptors, i.e., β2-adrenergic and γ-aminobutyric acid type B (GABAB) receptor, is reported. The protocol can be adapted to other membrane proteins and different cell models, transfection methods and labeling strategies.
Original language | English |
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Article number | e51784 |
Journal | Journal of Visualized Experiments |
Issue number | 89 |
DOIs | |
Publication status | Published - 25 Jul 2014 |
Keywords
- Bioengineering
- Dimerization
- Issue 89
- Live-cell imaging
- Microscopy
- Pharmacology
- Protein-protein interactions
- Receptor
- Single-molecule
- Total internal reflection fluorescence
- Tracking
ASJC Scopus subject areas
- General Neuroscience
- General Chemical Engineering
- General Immunology and Microbiology
- General Biochemistry,Genetics and Molecular Biology