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Green Fluorescent Protein

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Title: Green Fluorescent Protein


1
Green Fluorescent Protein
  • a B/MB senior seminar
  • brought to you by Colm OCarroll

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This presentation will cover
  • The structural aspects of GFP which make
    fluorescence possible
  • The advantages of using GFP and GFP mutants over
    other fluorescent markers
  • The use of GFP to monitor viral movement in
    plants

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The Green Fluorescent Protein
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GFPs unique structure
  • Composed of 238 amino acids
  • Paint in a can
  • Each monomer composed of a central ?-helix
    surrounded by an eleven stranded cylinder of
    anti-parallel ?-sheets
  • Cylinder has a diameter of about 30A and is about
    40A long
  • Fluorophore located on central helix

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The Active Site
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The Fluoropore Active Site
  • Ser65-Tyr66-Gly67
  • Deprotonated phenolate of Tyr66 is cause of
    fluorescence
  • Forster Cycle (1949-Theodor Forster)
  • Proton transfer to His148

10
Fluorophore formation
  • One limitation of wtGFP is its slow rate of
    fluorescence acquisition in vivo
  • Renaturation most likely by a parallel pathway
  • Oxidation of Fluoropore (2-4 hours)
  • Two step process

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Useful GFP mutants
  • Re-engineered GFP with preferred human codon
    usage
  • 20 fold enhancement consistent with 20 fold
    increase of GFP protein levels
  • GFP mutants can fluoresce different colors and be
    used simultaneously to monitor independent events
    in cells
  • Some GFP mutants exhibit more rapid formation of
    fluorophore

15
Improved mutant GFPuv
  • Excitation (dashed lines) and emission (solid
    lines) spectra of wt GFP (black lines) GFPuv
    (purple lines). The emission data were obtained
    with excitation at 385 nm.
  • Exhibiting lower toxicity in bacteria, GFPuv
    grows 2-3 times faster than wt GFP.

16
Advantages of GFP mutants in plants
  • High levels of GFP do not interfere with
    transformation, regeneration, or growth
  • Early nondestructive identification of
    transformed cells
  • Developing and optimizing transformation methods
  • Spatial and temporal gene expression at
    subcellular, cellular and plant levels

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Studying virus invasion and spread in plant tissue
  • Replaces marker protein ?-glucuronidase (GUS)
  • Procedure safe for cells
  • Requires only molecular oxygen for flourophore
    formation

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Procedure
  • Plants infected with PVX (Potato virus x-based
    vector)
  • Containing various GFP inserts
  • PVX expressing free GFP gene
  • PVX expressing GFP PC (protein coat) fusion
  • PVX with PC deletion/GFP replacement
  • PVX with GFP fusion to movement proteins

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Results indicated
  • Free GFP expression-radial expansion
  • GFP CP fusion cells possess a GFP overcoat
  • PC Deletion/GFP replacement- fluorescence
    restricted to single inoculated cells
  • GFP/MP fusion localized to plasmodesmata

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Bibliography
  • Nina, Haruki, et al. "Chemical nature of light
    emitter of Aequorea green fluorescent protein"
    (1996) Proceedings Natl. Acad. Sci. USA vol. 93
    p.13671-13622
  • Oparka, Karl, et al. "Using GFP to study virus
    invasion and spread in plant tissues"(1997)
    Nature vol. 388 p. 401-402
  • Reid, Brian, Gregory Flynn. "Chromophore
    formation in Green Fluorescent Protein" (1997)
    Biochemistry vol. 36 p. 6786-6791
  • Yang, F., L. Moss, G. Phillips. "The Molecular
    Structure of GFP" (1996) Nature Biotechnology
    vol. 14 p. 1219-1220
  • Youvan, Douglas., Gregory Flynn. "Chromophore
    formation in Green Fluorescent Protein" (1997)
    Biochemistry vol. 36 6786-6791

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Sources on the World Wide Web
  • Medical College of Wisconsin (www.biochem.mcw.edu/
    science_ed/Pages/gfp/index.html
  • Clonetech (www.gfp.clontech.com)
  • www.biorad.com/889168.html
  • www.bio.cmu.edu/Courses/03740/GFPTest/GFP.html
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