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Restriction Digest Laboratory
Restriction fragment length polymorphism
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Reminder You have transformed bacteria with plasmid DNA
You have isolated plasmid DNA Today you will perform an RFLP analysis & Confirm your Plasmid Isolation
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This is the third and final section of your lab report.
Digest plasmid DNA Determine number of cutting sites Determine location of cutting sites Determine size of fragments Present the “map” of the plasmid in your report The steps in BLUE you will complete outside of class as part of your data analysis.
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What is: A restriction enzyme(s)? A restriction digest?
An endonuclease We will focus on type II. A restriction digest?
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Restriction Enzyme Digest
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Examples of Restriction Enzymes
Links to restriction enzymes:
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Gel Electrophoresis Following Digest
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Analysis of Data Allows you to identify sizes of plasmid
By comparing migration of digested plasmid To KNOWN SIZES of DNA.
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Example of known sizes of DNA DNA Ladder or Markers
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A map gives the size of fragments
A map gives the number and position of cutting sites 60 800 600 JUST AN EXAMPLE Not your map! 1500 Plasmid map 1400
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Remember Plasmid is Circular
Circular DNA: the number of fragments=number (N) of cutting sites versus Linear DNA: number of fragments=N+1
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Linear DNA Plasmid DNA 2 cutting sites 2 fragments 2 cutting sites 3 fragments
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Today’s experiment Restriction of Digest of plasmid DNA
using two restriction enzymes.
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Please refer to page 10 of the handout (6 groups)
Each Group set up a rack with: Reaction buffer water Plasmid DNA PVU I SacII Loading Dye Standard (marker or ladder) DNA Label four microfuge tubes 1→4 Must keep on ice
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Pipette the samples as shown on page in handout—not lab manual.
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After you are finished pipetting your samples
Place samples at 37C for 1 hour After 1 hour you will be ready to load your gel
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Restriction Digest AFTER 1 hour DIGESTION: You must add 5 ul 10X loading dye to your samples (not to the ladder (L)). Pre-heat all samples including ladder for 3-5 min. at 65C
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Gel Electrophoresis Load 25 ul per well
Run gel at 75 volts until the dye front is approximately half-way down gel. Take photograph
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