BIO370Y5 Lecture Notes - Lecture 2: Restriction Enzyme, Calcium Chloride, Antimicrobial Resistance

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26 Apr 2016
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Part a- transformation of e. coli with recombinant dna. Competent cells are transformed with ligated products (antibiotic resistance genes) We"ll basically be incubating e. coli with the recombinant plasmid and purified pkan and pamp: a heat shock is applied so that the plasmid goes in. Plate them in amp, kan and amp+kan plates. The goal is determining the colonies that have the recombinant plasmid: we need one with 3755 (amp resistance and ori) and 1875 bp (kan resistance) The ones that have them grow on amp+kan plates. Part b- classic procedures for preparing competent cells. The classic proceudres make transformation efficiencies from 5 x 104-106 colonies/ug plasmid: relaxed circular and linear dna make 5-100 times fewer transformants compared with super-coiled dna. The tube with pamp and pkan (ligated) is heated to 85 c because it will inhibit restriction enzyme activity and prevent competition with ligation.

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