Lecture 42. Techniques 2: Cloning Flashcards
How can you express a eukaryotic gene in E. coli?
By converting the mRNA of the subject into cDNA (complementary DNA)
How can a gene with a known sequence be cloned?
By performing PCR with primers with engineered restriction sites
Synthesis of the first strand of cDNA
- Hybridise a poly(dT) primer to the polyA tail in the mRNA
- Use an RNA-dependent DNA polymerase called reverse transcriptase to make a single strand DNA copy of the mRNA
- Remove mRNA strand by alkaline digestion
Synthesis of the second strand of cDNA
- Add oligo(dG) to 3’ end of cDNA using Terminal Transferase
- Hybridise oligo (dC)
- Use DNA polymerase to make a second DNA strand
What is special about Type II restriction enzymes?
They are used extensively for DNA manipulations
How many types of restriction enzymes are there?
4
What do Type II restriction enzymes recognise?
A 4, 6 or 8 bp sequence known as a restriction site
After recognition of a restriction site, what does the Type II restriction enzyme do?
It hydrolyses a phosphodiester bond in each strand of the DNA
What are most Type II restriction sites?
Palindromic
What are plasmids used for in coding?
Vectors for inserting our genes
What does an origin of replication (ori) do?
This allows the plasmid to be maintained in the host cell
Different vectors have different ‘copy numbers’
What does a selectable marker (e.g an antibiotic resistant gene) do?
When plated in the presence of an antibiotic, only those bacteria containing the plasmid will grow
What does a disruptable marker (e.g lacZ’) do?
This allows selection of recombinant plasmids with DNA cloned into the disruptable marker
What does a no conjugation ability do?
The plasmid vector cannot easily be spread from cell to cell – it can only be transmitted by cell division, forming a clone
How does pUC cloning work?
Cut plasmid with enzymes and insert correct plasmid using DNA ligase (recombinant plasmid with disrupted lacZ’)
Rapidly growing E. coli treated with CaCl₂ will take up plasmids
