Restriction Digest Laboratory

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Restriction Digest Laboratory Restriction fragment length polymorphism

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Restriction Digest Laboratory. Restriction fragment length polymorphism. Reminder. You have transformed bacteria with plasmid DNA You have isolated plasmid DNA Today you will perform an RFLP analysis & Confirm your Plasmid Isolation. - PowerPoint PPT Presentation

Transcript of Restriction Digest Laboratory

Page 1: Restriction Digest Laboratory

Restriction Digest Laboratory

Restriction fragment length polymorphism

Page 2: Restriction Digest Laboratory

Reminder

• You have transformed bacteria with plasmid DNA

• You have isolated plasmid DNA

• Today you will perform an RFLP analysis• & Confirm your Plasmid Isolation

Page 3: Restriction Digest Laboratory

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)?

– 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

http://www.accessexcellence.org/AE/AEC/CC/re_chart.php

http://www.neb.com/nebecomm/tech_reference/restriction_enzymes/buffer_activity_restriction_enzymes.asp

Links to restriction enzymes:

http://www.neb.com/nebecomm/EnzymeFinder.asp?

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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

JUST AN EXAMPLENot your map!

Plasmid map

1500

80060

600

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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2 cutting sites2 fragments

2 cutting sites3 fragments

Plasmid DNA Linear DNA

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Today’s experiment

Restriction of Digest of plasmid DNAusing 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– NotI for AM lab– SfiI for AM lab

– Or

– AluI for PM lab– HphI for PM lab– 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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