SBB12Ntbk-Mike Hwang: Difference between revisions
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Mike Hwang (talk | contribs) (New page: ~~~~ <pre> Day 1 - Preparation of PCR and PCA PCA Preparation for Leucine Zipper RLER Protocol 1. Added 38uL ddH2O to small PCR tube using p100 micropipette 2. Added 5 uL of 10X expand bu...) |
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<pre> | <pre> | ||
Day 1 - Preparation of PCR and PCA | Day 1 - Preparation of PCR and PCA | ||
PCA Preparation for Leucine Zipper RLER | PCA Preparation for Leucine Zipper RLER | ||
Protocol | Protocol: | ||
1. Added 38uL ddH2O to small PCR tube using p100 micropipette | 1. Added 38uL ddH2O to small PCR tube using p100 micropipette | ||
2. Added 5 uL of 10X expand buffer (labeled with red) using p10 | 2. Added 5 uL of 10X expand buffer (labeled with red) using p10 | ||
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PCR Preparation of cI and oBP constructs | PCR Preparation of cI and oBP constructs | ||
Protocol: | |||
1. Labeled 2 different PCR tubes cI as A and oBP as B. | 1. Labeled 2 different PCR tubes cI as A and oBP as B. | ||
2. Added 24uL of ddH2O into both tubes | 2. Added 24uL of ddH2O into both tubes |
Revision as of 12:50, 16 February 2012
Mike Hwang 14:49, 16 February 2012 (EST)
Day 1 - Preparation of PCR and PCA PCA Preparation for Leucine Zipper RLER Protocol: 1. Added 38uL ddH2O to small PCR tube using p100 micropipette 2. Added 5 uL of 10X expand buffer (labeled with red) using p10 3. Added 5 uL of 2mM dNTPs (labeled with blue) using p10 4. Prepared separate 6uL oligo mixture of 100uM concentration by adding 2 uL each of o1, o2 and o7 oligos and mixed well. To make 100uM solutions of o1 and o2, 922 uL and 961 uL of ddH2O added to stock o1 and o2, respectively. 5. From above solution, 1 uL was removed and added to the PCR tube 6. Added .75 uL expand polymerase 7. Labeled PCR tube with A, MH and designated as PCA reaction 8. Placed PCR tube on small rack labeled PCA and put on ice PCR Preparation of cI and oBP constructs Protocol: 1. Labeled 2 different PCR tubes cI as A and oBP as B. 2. Added 24uL of ddH2O into both tubes 3. Added 3.3 uL of 10X expand buffer and 3.3 uL of 2mM dNTPs into both tubes 4. Added 1 uL of 10uM Ca998 to tube A 5. Added 1 uL of 10uM ca1333R to tube A 6. Added 1 uL of 10uM 1333F to tube B 7. Added 1 uL of 10 uM g00101 to tube B 8. Added 0.5 uL of jtk2768 to tube A 9. Added 0.5 uL of 9525-1835 to tube B 10. Added 0.5 uL of expand polymerase to both tubes 11. Placed in '500-1000bp' labeled rack on ice