Team:Alberta/Notebook/protocols/pcr
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- | {{Team:Alberta/navbar| | + | {{Team:Alberta/navbar|notebook=selected}} |
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+ | {{Team:Alberta/beginLeftSideBar|toc=NO}} | ||
+ | |||
+ | |||
+ | ==General Protocols== | ||
+ | ----------------------------- | ||
+ | *[[Team:Alberta/Notebook/protocols/invitro_biobyte_assembly | In Vitro BioByte Assembly]] | ||
+ | ----------------------------- | ||
+ | *[[Team:Alberta/Notebook/protocols/LB | LB Plates and Broth]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/transformations |Transformations]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/overnight |5mL Overnight ]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/glycerol | Glycerol Stock ]] | ||
+ | ----------------------------- | ||
+ | *[[Team:Alberta/Notebook/protocols/miniprep | Plasmid Miniprep ]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/digest | Restriction Digest ]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/vector_dephos | Vector Dephosphorylation]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/ligation | Ligation ]] | ||
+ | ----------------------------- | ||
+ | *[[Team:Alberta/Notebook/protocols/agarose_gel | Agarose Gel Electrophoresis ]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/gel_extraction | Gel Extraction ]] | ||
+ | ----------------------------- | ||
+ | *[[Team:Alberta/Notebook/protocols/pcr | PCR]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/colony_pcr | Colony PCR ]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/pcr_purification | PCR Purification ]] | ||
+ | ----------------------------- | ||
+ | *[[Team:Alberta/Notebook/protocols/labelling | Sample Labelling Conventions]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/sequencing | Fluorescent Sequencing Reaction]] | ||
+ | |||
+ | *[[Team:Alberta/Notebook/protocols/primer_design | Primer Design]] | ||
+ | ----------------------------- | ||
+ | |||
+ | |||
+ | {{Team:Alberta/endMainContent}} | ||
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- | + | ==PCR== | |
- | Procedure: | + | ===Procedure:=== |
* Before you start: | * Before you start: | ||
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Latest revision as of 02:30, 27 October 2010
PCR
Procedure:
- Before you start:
- KEEP EVERYTHING ON ICE. Put Taq back into freezer as soon as you`re done with it. DON`T put back dNTP tubes.
- Reserve a thermocycler and check what size of tubes it takes.
- Making a master mix conserves expensive reagents, so try to always use one.
- You may have to do dilutions of your reagents in order to make them usable for PCR (ex: primers, plasmid DNA...)
- DON'T PUT PRIMERS OR TEMPLATE INTO THE MASTER MIX. ADD POLYMERASE TO THE MASTER MIX LAST (after your other tubes already have template DNA and primers in them)!
- To add into a tube:
PCR buffer | 5ul |
10uM dNTPs | 1ul |
50uM MgCl2 | 2ul |
Forward primer | 2.5ul |
Reverse primer | 2.5ul |
1ng Template | 1ul |
Taq polymerase | 0.5ul |
MilliQ water | 35.5ul |
TOTAL | 50ul |
- Program to run:
1. 94oC | 3 minutes |
2. 94oC | 45 seconds |
3. 62oC | 30 seconds |
4. 72oC | 90 seconds |
5. Cycle steps 1 to 4 "30" times | |
6. 72oC | 10 minutes |