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pGLO ™ & GFP

pGLO ™ & GFP. DNA. RNA. Protein. Trait. Central Framework of Molecular Biology The Central Dogma as proposed by Francis Crick. Links of this Lab to Real-world. GFP is a visual marker Study of biological processes (example: synthesis of proteins)

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pGLO ™ & GFP

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  1. pGLO™& GFP

  2. DNA RNA Protein Trait Central Framework of Molecular BiologyThe Central Dogma as proposed by Francis Crick

  3. Links of this Lab to Real-world • GFP is a visual marker • Study of biological processes (example: synthesis of proteins) • Localization and regulation of gene expression • Cell movement • Cell fate during development • Formation of different organs • Screenable marker to identify transgenic organisms

  4. Transformation Procedure Day 2 Day 1

  5. Bacterial DNAImages Bacterial cell Plasmid DNA Genomic DNA

  6. GFP Beta-lactamase Ampicillin Resistance What is Transformation? • Uptake of foreign DNA, often a circular plasmid • The plasmid that we want the bacteria to uptake in this lab is calledpGLO. • There are two important genes found on this operon: • One called AMP that codes for the enzyme beta-lactamase (the enzyme that allows the bacteria to be resistant to amoxicillin – an antibiotic. • One called GFP that codes for the green flourescent protein (allows the bacteria to glow under certain conditions.)

  7. Bacterial Transformation Cell wall GFP Bacterial chromosomal DNA Beta lactamase (ampicillin resistance) pGLO plasmids

  8. Volume Measurement

  9. What is Nutrient Broth? • Luria-Bertani (LB) broth • Medium (Food) that contains nutrients for bacterial growth and gene expression • Carbohydrates • Amino acids • Nucleotides • Salts • Vitamins • The petri dishes are made using LB broth. For this lab you will be using three different dishes: • Some of the dishes will just have the LB • Some will have arabinose added to the broth, and • Some dishes will have both arabinose and ampicillin added.

  10. Transcriptional Regulation: Modification of the normal Arabinose Operon • Lactose operon • Arabinose operon • pGLO plasmid

  11. ara Operon lac Operon araC B A D LacI Z Y A Effector (Arabinose) Effector(Lactose) araC B A D LacI Z Y A RNA Polymerase RNA Polymerase B A D araC Z Y A Transcriptional Regulation: The lac and ara (Arabinose Operon) are both inducible. The effector is another name for the INDUCER.

  12. ara GFP Operon ara Operon araC GFP Gene araC B A D Effector(Arabinose) Effector (Arabinose) araC B A D araC GFP Gene RNA Polymerase RNA Polymerase B A D araC araC GFP Gene Gene Regulation: How the ara Operon has been modified. The B-A-D structural genes have been enzymatically removed from the operon and have been replaced by the GFP Gene.

  13. Methods of Transformation • Electroporation • Electrical shock makes cell membranes permeable to DNA • Calcium Chloride/Heat-Shock • Chemically-competent cells uptake DNA after heat shock

  14. Transformation Procedure • Suspend bacterial colonies in Transformation solution • Add pGLO plasmid DNA • Place tubes in ice • Heat-shock at 42°C and place on ice • Incubate with nutrient broth • Streak plates

  15. Reasons for Performing Each Transformation Step? Ca++ O Ca++ O P O Base • Transformation solution = CaCI2 Positive charge of Ca++ ions shields negative charge of DNA phosphates O O CH2 Sugar O Ca++ O O P Base O O CH2 Sugar OH

  16. Why Perform Each Transformation Step? Cell wall GFP 2. Incubate on ice slows fluid cell membrane 3. Heat-shock Increases permeability of membranes to allow for plasmid uptake 4. Nutrient broth incubation Allows beta-lactamase expression (transcription/transl. of the gene will occur) Beta-lactamase (ampicillin resistance)

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