A covalently linked probe to monitor local membrane properties surrounding plasma membrane proteins

Author:

Umebayashi Miwa12ORCID,Takemoto Satoko3ORCID,Reymond Luc4ORCID,Sundukova Mayya567ORCID,Hovius Ruud4ORCID,Bucci Annalisa5ORCID,Heppenstall Paul A.5ORCID,Yokota Hideo3ORCID,Johnsson Kai8ORCID,Riezman Howard1ORCID

Affiliation:

1. Department of Biochemistry and National Centre for Competence in Research in Chemical Biology, Sciences II, University of Geneva, Geneva, Switzerland 1

2. Myoridge Co. Ltd., Kyoto, Japan 2

3. Image Processing Research Team, RIKEN Centre for Advanced Photonics, Wako, Japan 3

4. Ecole Polytechnique Fédérale de Lausanne, Institute of Chemical Sciences and Engineering (ISIC), Institute of Bioengineering, National Centre of Competence in Research (NCCR) in Chemical Biology, Lausanne, Switzerland 4

5. Epigenetics and Neurobiology Unit, European Molecular Biology Laboratory Rome, Monterotondo, Italy 5

6. Instituto Biofisika (UPV/EHU, CSIC), University of the Basque Country, Leioa, Spain 6

7. Fundación Biofísica Bizkaia/Biofisika Bizkaia Fundazioa (FBB), Leioa, Spain 7

8. Department of Chemical Biology, Max Planck Institute for Medical Research, Heidelberg, Germany 8

Abstract

Functional membrane proteins in the plasma membrane are suggested to have specific membrane environments that play important roles to maintain and regulate their function. However, the local membrane environments of membrane proteins remain largely unexplored due to the lack of available techniques. We have developed a method to probe the local membrane environment surrounding membrane proteins in the plasma membrane by covalently tethering a solvatochromic, environment-sensitive dye, Nile Red, to a GPI-anchored protein and the insulin receptor through a flexible linker. The fluidity of the membrane environment of the GPI-anchored protein depended upon the saturation of the acyl chains of the lipid anchor. The local environment of the insulin receptor was distinct from the average plasma membrane fluidity and was quite dynamic and heterogeneous. Upon addition of insulin, the local membrane environment surrounding the receptor specifically increased in fluidity in an insulin receptor-kinase dependent manner and on the distance between the dye and the receptor.

Funder

Swiss National Centre for Competence in Research in Chemical Biology

Swiss National Science Foundation

Leducq Foundation

Publisher

Rockefeller University Press

Subject

Cell Biology

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