BIOL 200 Lecture Notes - Lecture 39: Calcium Chloride, Autoradiograph, Ecori

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22 Jun 2016
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O cell tissue extract rna reverse transcription mixture of cdna pcr using specific primers specific pcr product quantitation/sequencing (ie separate on gel and compare patterns) Lecture 22: molecular genetic techniques i: cloning, libraries. Dna cloning to prepare large quantities of identical dna: vector + dna fragment = recombinant dna replication within host cells isolation, sequencing, manipulation of purified dna fragment. Vectors: plasmids are the most common technique in dna cloning, as it is simple and practical for small sized dna; ie bacteria and yeast plasmids. Agar plate: soft solid support with nutrients; spread bacteria in a diluted solution where a single bacteria can replicate into clones (better than tube) Cloning involves cutting with restriction enzymes and pasting with dna ligases. Principle: open the circular vector and introduce the insert (gene of interest); paste insert into the vector; vector + insert = new recombinant dna restriction enzyme: cuts at specific sequence; generic name for dna cutting enzyme is nuclease.

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