Biology 1201A Lecture Notes - Lecture 1: Reverse Transcriptase, Expression Vector, Plasmid

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Cloning- generating quantities of a speciic dna sequence or gene. Extract dna from cells containing the gene of interest, cut. Dna into fragments- one of these fragments will most likely carry the desired gene. Each of the fragments is inserted into a plasmid producing a collection of recombinant dna. Recombinant plasmids are introduced to bacteria, continues to grow and divide. Resource that you can return to repeatedly. Low quantities of re will partially digest dna. Partially cut chromosomal dna with a frequent-cutter restriction enzyme to generate a sequence of overlapping fragments representing every cutting site in the original sample. Library contains complete genome- probe for any gene of interest. The important thing with re is that you don"t digest the dna at every. If you put enough re it will cut all sites, if you use less than that quantity of re there is not enough for it to cut all sites.

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