| Literature DB >> 25690655 |
Orestis Faklaris1, Martin Cottet1, Amandine Falco1, Brice Villier1, Michel Laget1, Jurriaan M Zwier1, Eric Trinquet1, Bernard Mouillac1, Jean-Philippe Pin1, Thierry Durroux2.
Abstract
Identifying the interacting partners and the dynamics of the molecular networks constitutes the key point in understanding cellular processes. Different methods often based on energy transfer strategies have been developed to examine the molecular dynamics of protein complexes. However, these methods suffer a couple of drawbacks: a single complex can be studied at a time, and its localization and tracking cannot generally be investigated. Here, we report a multicolor time-resolved Förster resonance energy transfer microscopy method that allows the identification of up to 3 different complexes simultaneously, their localization in cells, and their tracking after activation. Using this technique, we studied GPCR oligomerization and internalization in human embryonic kidney 293 cells. We definitively show that receptors can internalize as oligomers and that receptor coexpression deeply impacts oligomer internalization processes. © FASEB.Entities:
Keywords: lanthanide; multigate mode; oligomers; quantum dot; vasopressin V1a/V2 receptor
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Year: 2015 PMID: 25690655 DOI: 10.1096/fj.14-260059
Source DB: PubMed Journal: FASEB J ISSN: 0892-6638 Impact factor: 5.191