Genetic Engineering and Gene Cloning Lecture Notes PDF

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BestSellingLorentz

Uploaded by BestSellingLorentz

Ibn Sina National College for Medical Studies

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genetic engineering gene cloning biotechnology molecular biology

Summary

These lecture notes cover genetic engineering and gene cloning. The topics include the human genome, biotechnology, bacteria, bacterial genomes, transformation, plasmids, and the use of plasmids for biotechnology. The notes also discuss methods for cutting DNA, cloning genes, and techniques for introducing DNA into cells.

Full Transcript

# Genetic Engineering ## Human Genome - 3.2 billion bases ## Biotechnology Today - Genetic Engineering - Manipulation of DNA - If you are going to engineer DNA & genes & organisms, then you need a set of tools to work with. - This unit is a survey of those tools. ## Bacteria - Bacter...

# Genetic Engineering ## Human Genome - 3.2 billion bases ## Biotechnology Today - Genetic Engineering - Manipulation of DNA - If you are going to engineer DNA & genes & organisms, then you need a set of tools to work with. - This unit is a survey of those tools. ## Bacteria - Bacteria review - One-celled prokaryotes - Reproduce by: - Binary fission - Rapid growth - Generation Every ~20 minutes - 10^8 (100 million) colony overnight! - Dominant form of life on Earth - Incredibly diverse ## Bacterial Genome - Single circular chromosome - Haploid - Naked DNA - No histone proteins - ~4 million base pairs - ~4300 genes - 1/1000 DNA in eukaryote ## Transformation - Bacteria are opportunists - Pick up naked foreign DNA wherever it may be - Have surface transport proteins that are specialized for the update of naked DNA - Import bits of chromosomes from other bacteria - Incorporate the DNA bits into their own chromosome ## Plasmids - Small extrachromosomal circular DNA - 5000 - 20,000 base pairs - Self-replicating - Carry extra genes - 2-30 genes - Genes for antibiotic resistance - Can be exchanged between bacteria ## How can plasmids help us? - A way to get genes into bacteria easily - Insert new gene into plasmid - Insert plasmid into Bacteria - vector - Bacteria now expresses new gene - Bacteria make new protein ## Biotechnology - Plasmids used to insert new genes into bacteria ## Engineered Plasmids - Building custom plasmids - Restriction Enzyme sites - Antibiotic resistance genes as a selectable marker ## Selectable Marker - Antibiotic resistance gene on plasmid - Ampicillin resistance - Selecting for successful transformation - Successful uptake of recombinant plasmid ## Selection for plasmid uptake - Antibiotic becomes a selecting agent - Only bacteria with the plasmid will grow on antibiotic (ampicillin) plate ## Screening for Recombinant Plasmid - Bacteria take up plasmid - Functional LacZ gene - Bacteria make blue color - Bacteria take up recombinant plasmid - Non-functional LacZ gene - Bacteria stay white color ## How Do We Cut DNA? - Restriction enzymes - Restriction endonucleases - Discovered in 1960s - Evolved in bacteria to cut up foreign DNA - Bacteria protect their own DNA by methylation & by not using the base sequences recognized by the enzymes in their own DNA ## Restriction Enzymes - Action of enzyme - Cut DNA at specific sequences - Restriction site - Symmetrical - Produces protruding ends - Sticky ends - Will bind to any complementary DNA - Many different enzymes - Named after organism they are found in - EcoRI, HindIII, BamHI, Smal ## Restriction Enzymes - Cut DNA at specific sites - Leave "sticky ends" ## Sticky Ends - Cut other DNA with same enzymes - Leave "sticky ends" on both - Can glue DNA together at "sticky ends" ## Sticky Ends Help Glue Genes Together - DNA ligase joins the strands. - Sticky ends stick together ## Why Mix Genes Together? - Gene produces protein in different organism or different individual ## Copy (& Read) DNA - Transformation - Insert recombinant plasmid into bacteria - Grow recombinant bacteria in agar cultures - Bacteria make lots of copies of plasmid - "cloning" the plasmid - Production of many copies of inserted gene - Production of "new" protein - Transformed Phenotype - DNA → RNA → protein → trait ## Grow Bacteria...Make More ## Cut, Paste, Copy - Word processing metaphor... - Cut - Restriction enzymes - Paste - Ligase - Copy - Plasmids - Bacterial transformation ## Gene Cloning ## Gene Cloning - What does the term cloning mean? - What is gene cloning? How does it differ from cloning an entire organism? - Why is gene cloning done? - How is gene cloning accomplished? ## Cloning Definition - A method of growing an individual from a single somatic cell of its parent - Clone: a collection of molecules or cells, all genetically identical to an original molecule or cell. ## What is DNA/gene cloning? - When DNA is extracted from an organism, all its genes are obtained - In gene (DNA) cloning a particular gene is copied (cloned) ## What is Gene cloning? - To "clone a gene" is to make many identical copies of it. - Gene can be an exact copy of a natural gene. - Gene can be an altered version of a natural gene. ## Why Clone DNA? - A particular gene can be isolated and its nucleotide sequence determined - Sequences of DNA can be identified & analyzed - Protein/enzyme/RNA function can be investigated - Mutations can be identified, e.g. gene defects related to specific diseases - Organisms can be 'engineered' for specific purposes, e.g. insulin production, insect resistance, etc. ## How is DNA cloned? - Cell-based DNA cloning - Cell-free DNA cloning (PCR) ## Cell Based DNA Cloning/ Clone in Dividing Cells - Double-stranded recombinant plasmid DNA introduced into bacterial cell ## Restriction Endonucleases - The Molecular Scissors - Host enzymes that prevent the invasion of foreign DNAs such as viral DNA, by cutting them up. - These enzymes cut within the foreign DNAs, rather than chewing them away from the ends. - These enzymes recognize a specific DNA sequence (4-12bp) and cut both DNA strands. ## Three Types of Restriction Enzymes - Type I, Type II, Type III - Type I and III - Cleave with less precision and are not used in manipulating DNA - Type II - Recognize specific DNA sequences - Cleave at specific site within sequence - Can lead to "sticky ends" that can be joined. ## DNA ligase covalently links two DNA strands ## DNA ligase - Joins the two fragments forming a stable DNA molecule - Catalyzes formation of a phosphodiester bond between adjacent phosphate and hydroxyl groups of DNA nucleotides. ## Cloning Vectors - The DNA Carriers - Plasmids (e.g. pBR 322, pUC 19) - Phages/Bacteriophages (viruses that infect bacterial cells e.g. lambda phage) - Artificial chromosome vectors, e.g. - YACs (yeast artificial chromosomes) - BACs (bacterial artificial chromosomes) - Phagemids (combined features of phages with plasmids e.g. pBluescript II KS) - Cosmids (plasmid vectors with COS site of phages) - Viral vectors (retiroviruses) - Retriever vectors - Shuttle vectors ## Plasmids that can be modified to carry new genes - Plasmids useful as cloning vectors must have: - Replicator (origin of replication) - Allow the vector as well as the foreign DNA to amplify in the host cell - Selectable marker (antibiotic resistance gene) - Allow the host to grow on selective media - Can selectively amplify this specific vector in the host cell - Multiple cloning site - Allow insertion of foreign DNA without disrupting replication or inactivating essential markers ## DNA can be inserted into a cell by: - Transformation - Electroporation - Protoplast fusion - Microinjection - Biolistics/Gene gun ## The first Cloning experiment done by Boyer and Cohen ## Inserting a DNA sample into a Plasmid ## Screening ## Propagation - Once colonies are identified, they are cultured in broth to increase numbers and therefore the amount of DNA. - Samples are also prepared for storage at -80 degrees. They can be kept for many years this way.

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