GFP Purification Procedures - CERHB Purification Procedures Day 2 Day 3 Day 1 ... ©UF
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Transcript of GFP Purification Procedures - CERHB Purification Procedures Day 2 Day 3 Day 1 ... ©UF
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Purification
The art of chromatography
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Purify a single recombinant protein of interest from over 4,000 naturally occurring
E. coli gene products.
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Column Chromatography
• A separation method in which different components of a mixture travel through the resin of a column differently.
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Protein purification is based on chemical properties
• Proteins can be separated based on: – Size – Charge (ion exchange)
• Cation Exchanger (anions on resin bind positively charged protein)
• Anion Exchanger (Cations on resin bind negatively charged protein)
– Specific binding affinity (resin coupled w/antibody specific to protein of interest)
– Hydrophobicity (Hydrophobic Interaction Column).
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Hydrophobic Interaction
• Hydrophobic (water hating) substances do not mix well with water
• Some amino acids of proteins are very hydrophobic
• In salt water, these parts of the protein stick tightly to other hydrophobic substances (causes conformational change so hydrophilic regions are protected).
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HIC Column
• Hydrophobic amino acids of protein bind to a support (gel matrix) in the column, which contains immobilized hydrophobic groups (phenyl).
Hydrophobic bead
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Step 1:Hydrophobic Interaction
Chromatography
• Add bacterial lysate to column matrix in high salt buffer– Hydrophobic
proteins interact with column
http://www.bio-rad.com/LifeScience/docs/Official_pGLO_GFP_powerpoint_Spring_2005.ppt
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Step 2:Hydrophobic Interaction
Chromatography• Wash less
hydrophobic from column with low salt buffer– Less
hydrophobic E. coli proteins fall from column
– GFP remains bound to the column
http://www.bio-rad.com/LifeScience/docs/Official_pGLO_GFP_powerpoint_Spring_2005.ppt
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Step 3:Hydrophobic Interaction
Chromatography
• Elute GFP from column by adding no salt buffer
GFP– Released
from column matrix
– Flows through the column
http://www.bio-rad.com/LifeScience/docs/Official_pGLO_GFP_powerpoint_Spring_2005.ppt
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Biopharmaceutical Manufacturing
• Controlled Process– Reproducible– Consistent– Robust– Aseptic
• Product– Safe– Pure– Potent– Stable
Center of Excellence for Regenerative Health Biotechnology
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Protein Purification
http://www4.amershambiosciences.com18102229AD.pdf
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http://www.pharmaceutical-technology.com/contractors/contract/neo/
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© UFCenter of Excellence for Regenerative Health Biotechnology
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Chromatogram
http://www4.amershambiosciences.com18102229AD.pdf
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Purity
http://www.genedetect.com/rave.htm
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Process Development
1. Identification of target protein w/therapeutic value
2. Identification of target gene3. Isolation of the target gene4. Insertion of the target gene into a host
cell (such as E.coli) & express protein5. Purification: Separation of the target
protein from the host cell protein
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Process Development cont.
6. Large scale production of the target protein (under controlled manufacturing conditions)
7. Formulate8. Testing for safety and efficacy9. Marketing of a new medicine
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GFP Purification Procedures
Day 3Day 2
Day 1
http://www.bio-rad.com/LifeScience/docs/Official_pGLO_GFP_powerpoint_Spring_2005.ppt
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Hydrophobic Interaction Chromatography:
Steps 1–31.Add bacterial lysate to column matrix in
high salt buffer
2.Wash less hydrophobic proteins from column in low salt buffer
3.Elute GFP from column with no salt buffer
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© UFhttp://www.bio-rad.com/LifeScience/docs/Official_pGLO_GFP_powerpoint_Spring_2005.ppt
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Helpful Hints:Hydrophobic Interaction
Chromatography• Add a small piece of
paper to collection tube where column seats to insure column flow
• Rest pipette tip on side of column to avoid column bed disturbance when adding solutions
• Drain until the meniscus is just above the matrix for best separation
http://www.bio-rad.com/LifeScience/docs/Official_pGLO_GFP_powerpoint_Spring_2005.ppt
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This material is based upon work supported by the National Science Foundation under Grant No. 0438229.
Any opinions, findings, and conclusions or recommendations expressed in this material are those of the author(s) and do not necessarily reflect the views of the National Science Foundation.