Template:SBB-SOEing: Difference between revisions
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='''Full SOEing Run'''= | ='''Full SOEing Run'''= | ||
Here is the complete SOEing reaction guide. | Here is the complete SOEing reaction guide. | ||
== | ==Normal PCR== | ||
'''Cloning by PCR'''<br> | '''Cloning by PCR'''<br> | ||
'''This is the basic PCR method to amplify your DNA from a plasmid or genomic DNA sample using the Expand polymerase. You also use this protocol for an EIPCR reaction.''' | '''This is the basic PCR method to amplify your DNA from a plasmid or genomic DNA sample using the Expand polymerase. You also use this protocol for an EIPCR reaction.''' | ||
Revision as of 16:11, 25 June 2009
Full SOEing Run
Here is the complete SOEing reaction guide.
Normal PCR
Cloning by PCR
This is the basic PCR method to amplify your DNA from a plasmid or genomic DNA sample using the Expand polymerase. You also use this protocol for an EIPCR reaction.
The oligo concentrations in your stocks should be 100uM. You use them at 10uM in this protocol. So, you first need to make an oligo dilution of:
9uL Water 1uL 100uM oligo
You can throw away the remainder of the diluted oligo when you are done, but hold onto your stock tube!
Set up the following reaction in a PCR tube:
24uL ddH2O 3.3uL 10x Expand Buffer "2" 3.3uL dNTPs (2mM in each) 1uL Oligo 1, 10uM 1uL Oligo 2, 10uM 0.5uL Expand polymerase "1" 0.5uL Template DNA
The Expand temperature programs are a little complicated, so I won’t write them out here. They all involve 2 distinct cycling phases—the first 10 cycles have shorter extensions than the latter 20 cycles. You choose which one you want based on the length of your predicted product. If it is under 2kb, use 2K55. If it is between 2kb and 4kb, use 4K55. If it is over 4kb, use 8K55. In each case, start with the "55" version of the program. If you get no product or poor yield of product, repeat the same PCR reaction as two different variants, both with the “45” program. The first reaction will be the same composition as the first. For the second one, don’t add 3.3 uL of the water and instead use the volume for 3.3 uL of DMSO (dimethylsulfoxide). If these PCRs fail as well, well you'd either redesign, use a different template source, or give up.
Run Gel then Zymo Gel Purification
- All spins until the drying step are 15 second full speed spins.
- cut out bands minimizing extra gel matter.
- put in ependorf tube and add 600uL of Zymo ADB buffer (brown bottle).
- heat at 55, shake and/or vortex until the gel has dissolved.
- If the DNA is <300bp add 250uL of isopropanol
- transfer into the Zymo column inside a collection tube (small clear guys)
- spin through, discard waste.
- Add 200 uL of PE buffer (which is basically 70% ethanol)
- spin through, discard waste.
- Add 200 uL of PE buffer
- spin through, discard waste.
- spin for 90 seconds, full speed to dry.
- elute with 8.5 uL of water into a fresh Eppendorf tube
