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

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

Biochim Biophys Acta Biomembr

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

Published: May 2019

AI Article Synopsis

  • In situ studies of living cell membranes reveal dynamic behaviors of membrane proteins, which is crucial for understanding their function in complex environments.
  • Protein-specific labeling techniques, particularly using genetically encodable tags and synthetic probes, offer advantages over traditional fluorescent protein fusions, including smaller size and better control over labeling ratios.
  • This review highlights the use of heterodimeric peptide pairs that form coiled-coil structures for tagging and analyzing membrane proteins, demonstrating their effectiveness in studying protein behaviors like receptor internalization and oligomeric states in live cells.

Article 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.

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Source
http://dx.doi.org/10.1016/j.bbamem.2019.02.009DOI Listing

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