Lidstrom:PCR: Difference between revisions
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==General Guidelines== | ==General Guidelines== | ||
*Use the extension temperature stated on the kit -- being even 2 degrees to high or too low is detrimental! | *Use the extension temperature stated on the kit -- being even 2 degrees to high or too low is detrimental! | ||
*If a PCR isn't working there are more variables than you can | *Try T_annealing = 55oC first, then try other conditions if that fails. | ||
*If a PCR isn't working: | |||
**there are more variables (annealing temperature, annealing time, concentration of several reagents, reaction additives) than you can play with, especially because they all have combinatorial effects on the result. When [[User:Janet B. Matsen|Janet]] gets stuck, she does what Justin Siegel proposed: 55oC, 60oC, 65oC, and 70oC ish and do each of these temperatures with 0%, 5%, and 10% DMSO. That makes 12 rxns; do on a gradient PCR block. | |||
**Also consider including positive and negative controls in repeat attempts. | |||
==Taq== | ==Taq== | ||
Revision as of 21:15, 7 March 2012
General Guidelines
- Use the extension temperature stated on the kit -- being even 2 degrees to high or too low is detrimental!
- Try T_annealing = 55oC first, then try other conditions if that fails.
- If a PCR isn't working:
- there are more variables (annealing temperature, annealing time, concentration of several reagents, reaction additives) than you can play with, especially because they all have combinatorial effects on the result. When Janet gets stuck, she does what Justin Siegel proposed: 55oC, 60oC, 65oC, and 70oC ish and do each of these temperatures with 0%, 5%, and 10% DMSO. That makes 12 rxns; do on a gradient PCR block.
- Also consider including positive and negative controls in repeat attempts.
Taq
- Cheap
- Use for colony PCR (you don't keep the DNA so higher error rattes are ok)
Phusion
- faster, more accurate, & higher processiviy
- use for DNA modifications (e.g. things that will be put in vivo)
- more details & instructions: Phusion
- more stable (DNA/polymerase or tRNA/DNA?) interactions at high annealing temps (said Justin Siegal)
- Amanda heard that the Finnzymes version is better than NEB's. I couldn't find supporting information. (Janet)
General Notes
- When finishing a PCR cycle please cancel or stop all running programs before turning the thermocycler off. Turning certain thermocyclers off with a running program can cause machine errors or erratic behavior when turning the machine back on again. -Andrew Lamb 2/22/12
Buying Reagents
- Phusion
- You can buy from NEB or finnzymes; Janet uses NEB. You can buy the pure enzyme or a 2X master mix solution wherein they added the nucleotides for you. You pay ~50% more per rxn when you use the 2X version put there are pros: (a) it does save some time (b) it prevents the possibility of forgetting to add dNTPs and (c) saves you the cost/hassle of buying a set of dNTPs separately. User:Janet B. Matsen I called customer support on 3/6/2012 to ask whether I can make my own 2X mix from the less expensive pure enzymes. They do add a stabilizer to the 2X version (probably for the nucleotides) and they can't tell me what it is. They plan to get back to me when they ask experts whether I can make my own 2X anyway.
- You can also buy 2X mix that is a hot-start version of the enzyme, allowing you to set up your reactions at room temp. You pay even more for this.
