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Green Fluorescent Protein: Research Tool: Difference between revisions

New page: ==Use in the Laboratory== Green fluorescent protein has had great success as a marker protein in a variety of biological systems due to its inherent stability, which only adds to its many...
 
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===Use of GFP in FRET===
===Use of GFP in FRET===
[http://en.wikipedia.org/wiki/Förster_resonance_energy_transfer Förster resonance energy transfer] (FRET) is a laboratory technique used to detect the proximity of two biological molecules by the fusion of fluorescent proteins with each of the proteins of interest.  When the two fluorophores come within a certain proximity (typcially <100Å) in the proper orientation, the excited fluorophore (donor) emits energy that excites the second longer-wavelength fluorophore (acceptor) suc that it also fluoresces.  Results can then be seen by the ratio of the donor and acceptor emission intensities.  FRET is noninvasive and is therefore safe for using within live cells<ref name="Pollock" />.
Förster resonance energy transfer (FRET) is a laboratory technique used to detect the proximity of two biological molecules by the fusion of fluorescent proteins with each of the proteins of interest.  When the two fluorophores come within a certain proximity (typcially <100Å) in the proper orientation, the excited fluorophore (donor) emits energy that excites the second longer-wavelength fluorophore (acceptor) suc that it also fluoresces.  Results can then be seen by the ratio of the donor and acceptor emission intensities.<ref>For a more extensive description and development of this topic, go to [http://en.wikipedia.org/wiki/F%C3%B6rster_resonance_energy_transfer Wikipedia]</ref> FRET is noninvasive and is therefore safe for using within live cells<ref name="Pollock" />.


While the wild-type GFP protein has not been particularly useful as a sensor in FRET, several mutants of GFP have been manufactured to create proteins with distinct fluorescence spectra.  FRET has been done between two GFP molecules or a single GFP molecule and a secondary fluorophore <ref name="Pollock" />.
While the wild-type GFP protein has not been particularly useful as a sensor in FRET, several mutants of GFP have been manufactured to create proteins with distinct fluorescence spectra.  FRET has been done between two GFP molecules or a single GFP molecule and a secondary fluorophore <ref name="Pollock" />.
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*[[1huy]] Crystal structure of citrine, an improved yellow variant of green fluorescent protein
*[[1huy]] Crystal structure of citrine, an improved yellow variant of green fluorescent protein
*[[1oxd]] ''Aequorea victoria'' Cyan Variant of Green Fluorescent Protein
*[[1oxd]] ''Aequorea victoria'' Cyan Variant of Green Fluorescent Protein
==List of 3D structures of green fluorescent protein==
[[Green Fluorescent Protein]]


==Reference for this Structure==
==Reference for this Structure==

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