BSC 219 Lecture Notes - Lecture 22: Multiple Cloning Site, Plasmid, Restriction Digest

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A mixing of dna to result in a new genetic combination. Usually involves inserting a gene or fragment of dna (like a promoter) into a circular piece of dna called a plasmid (vector) The dna can be inserted, either naturally or by lab manipulation. Dna can be from same or different species. Recom dna was a major advancement that allowed for the study of specific dna sequences. Cloning is used to: generate multiple copies of the same gene o piece of dna, generate transgenic organisms, to generate an expression system for dna of interest in cell culture. Cloning involves the transfer of a dna fragment of interest from one organism to a self-replicating genetic element such as a bacterial plasmid. Isolate dna of interest (pcr: prepare dna (restriction digest, move dna into plasmid (ligation and transformation) Once you have dna of interest you need to prepare. There is a bacterial protein that cuts viral dna at a specific nucleotide sequence.

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