Protein interaction quantified in vivo by spectrally resolved fluorescence resonance energy transfer

Home
Animal Taxa
Plant Taxa
Semiochemicals
Floral Compounds
Semiochemical Detail
Semiochemicals & Taxa
Synthesis
Control
Invasive spp.
References

Abstract

Guide

Email to a Friend

« Previous AbstractOzone reaction with clothing and its initiated VOC emissions in an environmental chamber Next AbstractSlow desorption of volatile organic compounds from soil: evidence of desorption step limitations »

Biochem J

Title: Protein interaction quantified in vivo by spectrally resolved fluorescence resonance energy transfer

Author(s): Raicu V; Jansma DB; Miller RJ; Friesen JD;

Address: "Banting and Best Department of Medical Research, Charles H. Best Institute, University of Toronto, Toronto, Ontario M5G 1L6, Canada. vraicu@uwm.edu"

Journal Title: Biochem J

Year: 2005

Volume: 385

Issue: Pt 1

Page Number: 265 - 277

DOI: 10.1042/BJ20040226

ISSN/ISBN: 1470-8728 (Electronic) 0264-6021 (Print) 0264-6021 (Linking)

Abstract: "We describe a fluorescence resonance energy transfer (FRET)-based method for finding in living cells the fraction of a protein population (alpha(T)) forming complexes, and the average number (n) of those protein molecules in each complex. The method relies both on sensitized acceptor emission and on donor de-quenching (by photobleaching of the acceptor molecules), coupled with full spectral analysis of the differential fluorescence signature, in order to quantify the donor/acceptor energy transfer. The approach and sensitivity limits are well suited for in vivo microscopic investigations. This is demonstrated using a scanning laser confocal microscope to study complex formation of the sterile 2 alpha-factor receptor protein (Ste2p), labelled with green, cyan, and yellow fluorescent proteins (GFP, CFP, and YFP respectively), in budding yeast Saccharomyces cerevisiae. A theoretical model is presented that relates the efficiency of energy transfer in protein populations (the apparent FRET efficiency, E(app)) to the energy transferred in a single donor/acceptor pair (E, the true FRET efficiency). We determined E by using a new method that relies on E(app) measurements for two donor/acceptor pairs, Ste2p-CFP/Ste2p-YFP and Ste2p-GFP/Ste2p-YFP. From E(app) and E we determined alpha(T) approximately 1 and n approximately 2 for Ste2 proteins. Since the Ste2p complexes are formed in the absence of the ligand in our experiments, we conclude that the alpha-factor pheromone is not necessary for dimerization"

Keywords: Bacterial Proteins/*chemistry/genetics/*metabolism *Fluorescence Resonance Energy Transfer Green Fluorescent Proteins/*chemistry/genetics/*metabolism Luminescent Proteins/*chemistry/genetics/*metabolism Photobleaching Protein Binding Saccharomyces cerevis;

Notes: "MedlineRaicu, Valerica Jansma, David B Miller, R J Dwayne Friesen, James D eng England 2004/09/09 Biochem J. 2005 Jan 1; 385(Pt 1):265-77. doi: 10.1042/BJ20040226"

Citation: El-Sayed AM 2024. The Pherobase: Database of Pheromones and Semiochemicals. <http://www.pherobase.com>.
© 2003-2024 The Pherobase - Extensive Database of Pheromones and Semiochemicals. Ashraf M. El-Sayed.
Page created on 22-09-2024