Minnesota/4 July 2008
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Revision as of 17:08, 7 July 2008 by Emartin9808 (Talk | contribs)
1. PCR (Polymerase Chain Reaction): PCR used to modify Lambda_cI by copying a section of the gene, adding RBS, and using RS (restriction site enzyme) to cut copied gene section at the appropriate restriction site. |
Components | Volume |
---|---|
Phusion HF Buffer | 10.0uL |
10 mM dNTP's | 1.0uL |
Primer mix | 2.5uL |
Template DNA | 1.0uL |
Phusion DNA Polymerase | 0.5uL |
H20 | 35.0uL |
2. Run PCR in Gel Electrophoresis: |
a. Used 0.8% agarose gel, TAE buffer, and ethidium bromide (interculating agent) |
b. Gel proved have correct Lambda_cI gene with 750 base pairs. Can now perform PCR purification (add buffers). |
3. Miniprep MCherry gene |
4. Spectrophotometry: |