Biotechnology

1. Biotechnology Chapter 17

2. How did it all start? • Recombinant DNA

3. How is Recombinant DNA made? • Restriction Enzymes • Restriction sites • Type 1 • Type 2 • Dna Ligase

4. Gel Electrophoresis • Separates fragmented DNA • Takes advantage of DNA’s negative charge • Separates by size

5. Transformation • So what is it? • In E.coli • Transgenenic Organisms

6. Molecular Cloning • Host-Vector Systems • Commonly used host? • Commonly used vectors? • How to clone a gene!

7. Plasmid Vector • Must have • 1. Origin of replication • 2. Selectable marker

9. Phage Vectors • Can hold more inserted DNA up to 40 kb • Lambda phages kill cells, and are linear

11. DNA Libraries • DNA Library vs Genomic Library • Reverse Transcriptase • Making cDNA • Hybridization

12. Steps to Hybridization • 1. Colonies of plasmid w/ bacteria each containing a singe DNA from the library are grown on agar. • 2. A replica of the plate is made using filter paper • 3. Filter paper is washed in a solution that breaks cells open and denatures DNA- the filter is incubated with radioactively labeled probe that will from hybrids with complimentary DNA gene of interest. • 4. Colonies of interest will retain the radioactive probe. • 5. A comparison between the original plate and the filter paper is made. • FIGURE 17.6

13. DNA ANALYSIS • Restriction Maps • Southern Blots • RFLP Analysis • DNA fingerprinting • PCR

15. DNA Sequencing • Enzymatic Sequencing • PCR • Applications

16. Genetic Engineering • ASSIGNMENT!!!!!!!!!!! • Read and Outline IN DEPTH Pages 339-346. • Develop two arguments one for and one against the use of genetic engineering. • Write a 2 page paper outlining both the pro’s and con’s of Genetic Engineering • Be prepared to present your findings in class!!!!!!