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DNA Science Day 2 Extracting, Ligating and Transforming Physical Biology Bootcamp October 2006 Caltech.

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Presentation on theme: "DNA Science Day 2 Extracting, Ligating and Transforming Physical Biology Bootcamp October 2006 Caltech."— Presentation transcript:

1 DNA Science Day 2 Extracting, Ligating and Transforming Physical Biology Bootcamp October 2006 Caltech

2 Today’s Plan? Extract the cut vector from an agarose gel Ligate the vector to the lacZ insert Transform cells

3 Gel Extraction Cut out the band with a razor blade –Shorter wavelengths = more damage to the DNA –Keep it small! What samples should be run next to it as a control? –Uncut plasmid –Ladder! QIAquickSpin.pdf

4 What Happened to the PCR Product? Digest it using HindIII and KpnI –The single cutter controls are not useful here because we don’t have enough resolution Purify the product using a Qiagen PCR purification kit –100 bp – 10 kbp

5 Ligation RocheRapidDNALigation.pdf Do different insert:vector molar ratios, total mass < 200ng –3:1 –1:1 –1:3 –No insert control –No vector control Perform a PCR purification afterwards Killer cut? –Get rid of any possible religation

6 Transformation by Electroporation Stress the cells by putting them in an electric field –They’ll take DNA! –Chemical transformation is also possible (heat=stress) Transform no more than 20 ng of ligation –All the ligations –The original plasmid Estimate the transformation efficiency –Our competent cells are 1:1000 concentrated from OD 600 0.7 –1:1E6 dilution and below for non-transformed cells –1:1 dilution and below for transformed cells Show the plates with colonies Create the new Plasmid with Vector NTI

7 Strains E. coli Genetic Sock: http://cgsc.biology.yale.edu/ Explain how we are going to screen. DH5aZ1 –No lacZYA –lacI, tetR and araC


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