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Published byPaul Shaw Modified over 9 years ago
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Dheeraj K. Jalluri Gene Team 2015
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CCATGG GGTACC Restriction Enzymes are “ Scissors” that cut at Restriction Sites 5’ 3’ 5’ Racecar Level Civic Kayak Madam Reviver RESTRICTION SITE
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REs create Sticky Ends ATCGCCATGGTGCA TAGCGGTACCACGT 5’ 3’ STICKY ENDS CATGGTGCA CACGT 5’ 3’ ATCGC TAGCGGTAC 5’ 3’
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Genes can be inserted into plasmids using REs Insulin gene Bacterial Plasmid Insulin gene = CCATGG GGTACC C GGTAC C CATGG INSULIN GENE C GGTAC C CATGG Ligase
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REs Sites can be used to Identify Plasmids p1 p2p3
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Restriction (Check) Digests check Plasmid’s Identity ReagentStart Conc.Final Conc.Volume3x Buffer10X1X DNA mini-prep100 ng / µL500 ng (total) Water-- Enzyme10 U / µL- TOTAL20 µL 2 µL 5 µL 1 µL 12 µL 6 µL 36 µL 3 µL
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Restriction Digest Review Restriction Enzymes cut at DNA palindromes called Restriction Sites REs form DNA overhangs called Sticky Ends REs can be used to insert a gene into a plasmid The number and locations of restriction sites are unique to a plasmid Check Digest tables show specific amounts of reagents needed to cut plasmids with a RE …now we need to look at the separated fragments…
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Gel Electrophoresis separates DNA segments
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DNA is Negatively Charged + - DNA
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Gel is made from Agarose
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Ethidium Bromide helps visualize the bands
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Gel Electrophoresis Review - + LARGER smaller
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Enzyme(s)Expected Bands 1. BglII 3350, 1142 2. BglII + BsiWI 2891, 1142, 459 1. 2. 1. 2.
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Images http://genetics.thetech.org/sites/default/files/DNAscissors.gif http://cyberbridge.mcb.harvard.edu/images/dna1_4.png https://www.mun.ca/biology/scarr/gel_electrophoresis.gif http://genetics.thetech.org/sites/default/files/AgaroseUpClose.gif http://www.cf.ac.uk/chemy/staffinfo/platts/ethid.png http://2008.igem.org/wiki/images/thumb/0/07/Ethidium2.jpg/231px- Ethidium2.jpg http://2008.igem.org/wiki/images/thumb/0/07/Ethidium2.jpg/231px- Ethidium2.jpg
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