BIOC 3021 Lecture Notes - Lecture 21: Southern Blot, Recombinant Dna, Dna Ligase

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27 Apr 2018
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GCCA
CGGT
CGGT
ACCG
- Recombinant DNA technology:
- Requirements:
- DNA source
- Cloning vector
- Restriction endonucleases
- DNA ligase
- Host organism
- Restriction Endonucleases:
- Hydrolytic enzymes that make cuts at distinct sites in DNA
- 2-fold axis of symmetry
- DNA is complementary and has inverted symmetry
- Also called palindromes
- Sequence can be read forward and backwards
- Only true if DNA sequences are read by crossing over at central axis of
symmetry
Gel Electrophoresis:
- Digestion of DNA with different endonucleases produces characteristic fragments
- Fragments are separated on a gel run with an electric current
- Smaller fragments travel faster and further on gel
Southern Blotting:
- Uses a DNA probe with a sequence of interest
- Hybridizes sample with a complementary sequence
- Sample cleaved with endonucleases subjected to electrophoresis
- Separated pieces are transferred to nitrocellulose paper
- Visualized by autoradiography
Restriction-Fragment-Length Polymorphism (RFLP):
- Southern blotting can be used to follow inheritance of selected genes
- Mutations within restriction sites change the size of restriction fragments/positions of
bands
- Polymorphism: genetic diversity in a population
DNA SEQUENCING:
GCCA
CGGT
CGGT
ACCG
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Document Summary

Hydrolytic enzymes that make cuts at distinct sites in dna. Dna is complementary and has inverted symmetry. Sequence can be read forward and backwards. Only true if dna sequences are read by crossing over at central axis of. Digestion of dna with different endonucleases produces characteristic fragments. Fragments are separated on a gel run with an electric current. Smaller fragments travel faster and further on gel. Uses a dna probe with a sequence of interest. Sample cleaved with endonucleases subjected to electrophoresis. Separated pieces are transferred to nitrocellulose paper. Southern blotting can be used to follow inheritance of selected genes. Mutations within restriction sites change the size of restriction fragments/positions of bands. Template dna strand to be sequenced. Usually 4 reaction mixtures each with one specific dideoxy-ntp. Elongation of primer strands stops when dideoxynucleotide is incorporated. Elongation of primer strand stops when dideoxynucleotide is incorporated. Cohesive sticky ends will naturally adhere to each other by base pairings.

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