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Chapter 20: Biotechnology
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Essential Knowledge u 3.a.1 – DNA, and in some cases RNA, is the primary source of heritable information (20.1 & 20.2)
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Focus of Chapter u An introduction to the methods and developments in: u Recombinant DNA u Genetic Engineering u Biotechnology
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Recombinant DNA u DNA in which genes from different sources are linked u Ex: the “green” mice
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Genetic Engineering u The direct manipulation of genes for practical purposes u Ex: Using E. coli to produce human insulin
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Biotechnology u The use of living organisms or their components to perform practical tasks u Ex: the use of bacteria to digest oil spills
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Plasmids u Small circular piece of DNA u Carry many important traits u Used extensively in biotechnology and recombinant DNA u Serve as a “vehicle” for transporting genes
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Steps for Plasmid Use 1. Get the DNA for the trait 2. Insert DNA into the plasmid 3. Bacterial transformation 4. Identification of the new trait *Fig 20.4, page 399
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Restrictive Enzymes u Cut DNA at specific nucleotide sequences called “restriction sites” u Used to "cut and splice" DNA u Obtained from bacteria u Ex. EcoRI and Hind III
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Insertion u Placing foreign DNA into a plasmid u Open plasmid with enzymes to create “sticky ends” u Splice the new DNA and plasmid together.
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Transformation u Placing the plasmid into a bacterial cell
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Methods u Temperature shock & salt treatment u Electric current u Injection
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Identification u Screening the altered cells for the desired gene u Ex: Antibiotic sensitivity or the expression of a “new” trait (color, glowing etc.)
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Example Applications 1. Insulin 2. Human Growth Hormone 3. Other Proteins
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DNA Sources 1. Organism - use a section of their chromosome 2. cDNA - created copy of DNA (to avoid introns)
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Organism DNA u Isolated by restrictive enzyme cuts u Separation by gel electrophoresis u Pieces stored in a genomic library
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cDNA u CDNA u Complementary DNA u Artificial gene with no introns u Made from the mRNA for that specific protein using Reverse Transcriptase
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DNA Sequencing: Sanger Method u Uses dideoxynucleotides u Build new DNA from single strand DNA u Used to separate out nucleotides
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PCR Method u Polymerase Chain Reaction u Used to make many copies of a small segment of DNA u Quicker than Sanger method
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RFLP Method u Restriction Fragment Length Polymorphism u Used for detecting minor differences in DNA u Uses: u DNA fingerprinting (crimes) u Pedigree studies (DNA markers)
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Southern Blotting method u Developed by EM Southern in 1975 u Used to compare fragments from different genomes u Looks like a photograph u More permanent results
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DNA Technology: Applications 1. Basic Research 2. Medical 3. Forensics 4. Agricultural
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Basic Research 1. DNA and protein studies 2. Evolution 3. Gene structure and control mechanisms
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Human Genome Project (HGP) u 15 year project which started in 1990 u Project was basically completed in February 2000
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HGP Goals 1. Linkage mapping of the human genome. 2. Physical mapping of the human genome. 3. Human genome sequence. 4. Genomes of other species.
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Medical Uses 1. Diagnosis of Diseases 2. Gene Therapy 3. Vaccines 4. Pharmaceutical Products
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Forensic Uses u DNA fingerprints for crime solving u DNA identification records
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Agricultural Uses 1. Animals u Increased milk production u Increased feed utilization u Increased meat production
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Injecting DNA into egg
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PharmAnimals
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Agricultural Uses 2. Plants u Herbicide resistance u Retard spoilage of fruits u Insect resistance u Nitrogen-Fixation ability
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Future Of DNA Technology u Cloning of higher animals u Growth of replacement tissues and organs u Gene therapy to correct DNA defects u?u?
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Gene Therapy
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Summary u Recognize some of the basic strategies and methods of gene manipulation and analysis. u Identify representative examples of the applications of DNA technology. u Be prepared to discuss the implications of genetically modified organisms (GMO’s) on science, technology and society.
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