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Detection of the human VNTR using PCR* *A Polymerase Chain Reaction Experiment
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The experiment is divided into 2 parts Isolate human DNA from cheek cells The DNA will be amplified using PCR The DNA will be analyzed using gel electrophoresis
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Polymerase Chain Reaction: another method of DNA amplification
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Basis of PCR Create conditions “in vitro” for DNA replication.
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Requirements for replication DNA template Primers Taq DNA Polymerase** Nucleotides MgCl++
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Temperature cycles plays a key role: Unwinding DNA Annealing Extension 98C 45-60C 72C http://www.dnalc.org/Shockwave/pcranwhole.html
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Primers determine The sequence of DNA that will be amplified.
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Basis for sequence specific amplification Two primers are used to bracket the area you want to amplify. Primers are single stranded synthetic sequences of DNA normally 20-30 bp. One primer is complementary to the beginning of the target gene on one strand while the other primer is complementary to end of the target gene on the complementary strand.
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Summary: Unwinding DNA Annealing Extension 98C 45-60C 72C http://www.dnalc.org/Shockwave/pcranwhole.html
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The experiment is divided into 2 parts Isolate human DNA from cheek cells The DNA will be amplified using PCR The DNA will be analyzed using gel electrophoresis
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Highlights of Key Steps of your DNA Isolation
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Each person should obtain Cotton swabs A test tube with 2 mls of buffer A screw top microfuge tube 2 transfer pipets
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Isolation of DNA Cheek Cells Obtain cells by swabbing the inside of the mouth with a cotton tipped applicator.
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Next… Place cotton head in 2 ml of PBS (in conical tube) Swirl vigorously for 1 min. to dislodge cells Press the cotton head against the walls to squeeze out as much liquid as possible Use new applicator and repeat the above steps.
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Next… Transfer 2 ml to screw top tube. Spin at 5000 rpm for 1 min. Be sure you have pellet. If not repeat swabbing. Remove supernantant but SAVE PELLET (these are your cells!) Add 100 ul of chelating agent to sample
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Next… Re-suspend the pellet in 100 ul of chelator solution: MAKE SURE PELLET IS RESUSPENDED! Place screw top microfuge tube in boiling waterbath for 10 minutes to break (lyse) cells.
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Next: After 10 min boiling allow tube to cool (2 minutes and then spin microfuge tube for 2 minutes (5000 rpm)
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Next: Obtain a PCR tube with “PCR bead” Add primers to bead and 5 ul of your supernatant and gently mix. Label your PCR tube your assigned seat number Place in PCR!
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Summary of PCR tube To PCR tube containing “bead” add: 20.0 ul of primer solution 5.0 ul of cheek cell DNA
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VNTR : PCR reaction 32 cycles at: 94C 65C 72C 30 seconds
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The gel electrophoresis Analysis of your results will be carried and provided to you (time may not be available at the next lab for gel electrophoresis).
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After PCR Gel electrophoresis Warm samples (including ladder) 2 minutes at 50 C Load 25 ul of the sample Load 25 ul of ladder
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