BIOL 142 Lecture Notes - Lecture 15: Cloning, Ampicillin, Dwarfism

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7 May 2018
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Biology 142- Lecture 15- Recombinant DNA Technology Continued
Restriction Enzyme Restriction Sites
How often does a specific restriction site occur in random DNA?
o 4number base of pairs in the restriction site sequence
Cloning Vectors
Different cloning vectors
o plasmid (10 kilobases [kb] or less)
o bacteriophage (20 kb or less)
o Cosmid vector (approximately 40 kb)
o Bacterial Artificial chromosome (BAC) (approximately 150 kb)
o Yeast Artificial chromosome (YAC) (approximately 1000 kb)
Different size vectors are used based on the host organism
A cloning vector/insert can be derived from many things:
o Another plasmid
o Genomic DNA
o PCR product
o cDNA (DNA can be made from mRNA)
cDNA are DNA/genes that are only being expressed in a specific cell type
Amplification in Recombinant DNA Technology
One of the first steps of recombinant DNA technology is to amplify the DNA
Amplification can occur one of two ways
o By inserting the DNA fragment containing gene into a plasmid in bacterial cells
and allowing the cells to grow
o By polymerase chain reactions (PCR)
How amplification works:
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Image from: PowerPoint, slide 19
Plasmid Vector
Components of a plasmid: origin of replication, screenable marker, and a selectable
marker
o Screenable marker
Can be used to select for specific plasmids without killing them
o Selectable marker
Used to kill plasmids that don’t meet the selected criteria
Empty vectors: plasmids that don’t get the fragment of interest transferred into the
genetic code
Screenable and selectable markers are used to select for empty vectors
Plasmid vector example: PUC18
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