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Bioengineering

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Nanyang Technological University

High-resolution Spatiotemporal Analysis of Receptor Dynamics by Single-molecule Fluorescence Microscopy

11.3K Views

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15:13 min

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July 25th, 2014

DOI :

10.3791/51784-v

July 25th, 2014

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Titiwat Sungkaworn¹, Finn Rieken¹, Martin J. Lohse¹, Davide Calebiro¹

¹Institute of Pharmacology and Toxicology and Bio-Imaging Center/Rudolf Virchow Center, DFG-Research Center for Experimental Biomedicine, University of Würzburg, Germany

Summary

This protocol describes how to use total internal reflection fluorescence microscopy to visualize and track single receptors on the surface of living cells and thereby analyze receptor lateral mobility, size of receptor complexes as well as to visualize transient receptor-receptor interactions. This protocol can be extended to other membrane proteins.

Explore More Videos

Single molecule Microscopy

Receptor Dynamics

TIRF Microscopy

Receptor receptor Interactions

Membrane Proteins

G protein coupled Receptors

2 adrenergic Receptor

Spatiotemporal Analysis

Fluorescence Labeling

Real time Imaging

Ensemble Measurements

Chapters in this video

0:05

Title

2:00

Coverslip Cleaning

3:33

Preparation of Calibration Samples

4:41

Transfection

7:35

Protein Labeling

8:58

Image Acquisition

10:49

Image Analysis

12:35

Results: TIRF Microscopy Detects and Tracks Single Receptors on the Surface of Living Cells

14:31

Conclusion

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