Transformation of E. coli with Green Fluorescent Protein (GFP)

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Transformation of E. coli with Green Fluorescent Protein (GFP)

Transcript of Transformation of E. coli with Green Fluorescent Protein (GFP)

Page 1: Transformation of E. coli with Green Fluorescent Protein (GFP)

Transformation of E. coli withGreen Fluorescent Protein (GFP)

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Central Framework of Molecular Biology

DNA RNA Protein Trait

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Links 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

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Using GFP as a biological tracer

http://www.conncoll.edu/ccacad/zimmer/GFP-ww/prasher.htmlWith permission from Marc Zimmer

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Transformation Procedure Overview

Day 1

Day 2

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What is Transformation?

• Uptake of foreign DNA, often a circular plasmid

GFP

Beta-lactamase

Ampicillin

Resistance

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What is a plasmid?

• A circular piece of autonomously replicating DNA

• Originally evolved by bacteria

• May express antibiotic resistance gene

or be modified to express proteins of interest

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Bacterial DNA

Plasmid DNA

Bacterial cell

Genomic DNA

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The Many Faces of Plasmids

Scanning electron micrograph of supercoiled plasmid

Graphic representation

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GeneExpression

• Beta Lactamase– Ampicillin resistance

• Green Fluorescent Protein (GFP)– Aequorea victoria

jellyfish gene

• araC regulator protein– Regulates GFP

transcription

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Bacterial Transformation

Beta lactamase(ampicillin resistance)

pGLO plasmids

Bacterial chromosomal DNA

Cell wall

GFP

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Transcriptional Regulation

• Lactose operon

• Arabinose operon

• pGLO plasmid

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Transcriptional Regulation

B A DaraC

B A DaraC

RNA Polymerase

Effector (Arabinose)

araC B A D

ara Operon

RNA Polymerase

Z Y A

Z Y ALacI

Effector (Lactose)

Z Y ALacI

lac Operon

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Gene Regulation

RNA Polymerase

araC

ara GFP Operon

GFP Gene

araC GFP Gene

araC GFP Gene

Effector (Arabinose)

B A DaraC

B A DaraC

RNA Polymerase

Effector (Arabinose)

araC B A D

ara Operon

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Methods of Transformation

• Electroporation– Electrical shock makes cell membranes

permeable to DNA

• Calcium Chloride/Heat-Shock– Chemically-competent cells uptake DNA after

heat shock

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Transformation Procedure

• Suspend bacterial colonies in Transformation solution

• Add pGLO plasmid DNA

• Place tubes on ice

• Heat-shock at 42°C and place on ice

• Incubate with nutrient broth

• Streak plates

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Reasons for Performing Each Transformation Step?

1. Transformation solution = CaCI2

Positive charge of Ca++ ions shields negative charge of DNA phosphates

Ca++

Ca++

OCH2

O

P O

O

OBase

CH2

O

P

O

O

O

Base

OH

Sugar

Sugar

OCa++

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Why Perform Each Transformation Step?

2. Incubate on iceslows fluid cell membrane

3. Heat-shockIncreases permeability of membranes

4. Nutrient broth incubationAllows beta-lactamase expression

Beta-lactamase(ampicillin resistance)

Cell wall

GFP

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What is Nutrient Broth? • Luria-Bertani (LB) broth

• Medium that contains nutrients for bacterial growth and gene expression– Carbohydrates– Amino acids– Nucleotides– Salts– Vitamins

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Grow? Glow?

• Follow protocol

• On which plates will colonies grow?

• Which colonies will glow?

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LaboratoryQuick Guide

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Volume Measurement