Understanding FRET as a research tool for cellular studies

Communication of molecular species through dynamic association and/or dissociation at various cellular sites governs biological functions. Understanding these physiological processes require delineation of molecular events occurring at the level of individual complexes in a living cell. Among the fe...

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Bibliographic Details
Published inInternational Journal of Molecular Sciences Vol. 16; no. 4; pp. 6718 - 6756
Main Authors Shrestha, Dilip, Jenei, Attila, Nagy, Péter, Vereb, György, Szöllősi, János
Format Journal Article Book Review
LanguageEnglish
Published Switzerland MDPI AG 25.03.2015
MDPI
Subjects
Anisotropy
Biophysics
CD1d
ErbB
Flow Cytometry
Fluorescence intensity
Fluorescence lifetime
Fluorescence Resonance Energy Transfer - methods
FRET
Green Fluorescent Proteins - chemistry
IL15
IL2
Immune synapse
Major Histocompatibility Complex (MHC)
Methods for measuring FRET
Microscopy, Fluorescence - methods
Molecular biology
Proteomics - methods
Review
Signal Transduction
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Summary:Communication of molecular species through dynamic association and/or dissociation at various cellular sites governs biological functions. Understanding these physiological processes require delineation of molecular events occurring at the level of individual complexes in a living cell. Among the few non-invasive approaches with nanometer resolution are methods based on Förster Resonance Energy Transfer (FRET). FRET is effective at a distance of 1-10 nm which is equivalent to the size of macromolecules, thus providing an unprecedented level of detail on molecular interactions. The emergence of fluorescent proteins and SNAP- and CLIP- tag proteins provided FRET with the capability to monitor changes in a molecular complex in real-time making it possible to establish the functional significance of the studied molecules in a native environment. Now, FRET is widely used in biological sciences, including the field of proteomics, signal transduction, diagnostics and drug development to address questions almost unimaginable with biochemical methods and conventional microscopies. However, the underlying physics of FRET often scares biologists. Therefore, in this review, our goal is to introduce FRET to non-physicists in a lucid manner. We will also discuss our contributions to various FRET methodologies based on microscopy and flow cytometry, while describing its application for determining the molecular heterogeneity of the plasma membrane in various cell types.
ISSN:1422-0067
1661-6596
1422-0067
DOI:10.3390/ijms16046718