Sandbox 12

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<scene name='Sandbox_12/Green_flourescent_66ligand/1'>Detail view of the green flourescent chromophore.</scene> <ref>PMID:8790375</ref>
<scene name='Sandbox_12/Green_flourescent_66ligand/1'>Detail view of the green flourescent chromophore.</scene> <ref>PMID:8790375</ref>
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==This is a placeholder==
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<references/>
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This is a placeholder text to help you get started in
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placing a Jmol applet on your page. At any time, click
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Replace the PDB id (use lowercase!) after the STRUCTURE_ and after PDB= to load
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and display another structure.
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{{STRUCTURE_3cin | PDB=3cin | SCENE= }}
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Revision as of 13:28, 1 September 2009

Green fluorescent protein (GFP), originally isolated from the jellyfish Aequorea victoria (PDB entry 1ema), fluorsceses green (509nm) when exposed to blue light (395nm and 475nm). It is one of the most important proteins used in biological research because it can be used to tag otherwise invisible gene products of interest and thus observe their existence, location and movement.

Exploring the Structure

Green fluorescent protein

Drag the structure with the mouse to rotate

GFP is a beta barrel protein with 11 beta sheets. It is a 26.9kDa protein made up of 238 amino acids. The chromophore, responsible for the fluorescent properties of the protein, is buried inside the beta barrel as part of the central alpha helix passing through the barrel. The chromophore forms via spontaneous cyclization and oxidation of three residues in the central alpha helix: -Thr65 (or Ser65)-Tyr66-Gly67. This cyclization and oxidation creates the chromophore's five-membered ring via a new bond between the threonine and the glycine residues. [1]

  1. Korfhagen TR, Bruno MD, Ross GF, Huelsman KM, Ikegami M, Jobe AH, Wert SE, Stripp BR, Morris RE, Glasser SW, Bachurski CJ, Iwamoto HS, Whitsett JA. Altered surfactant function and structure in SP-A gene targeted mice. Proc Natl Acad Sci U S A. 1996 Sep 3;93(18):9594-9. PMID:8790375
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