Team:Imperial College London/Protocol
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|'''Listed below are the protocols we used for the project. We hope you find them useful!''' | |'''Listed below are the protocols we used for the project. We hope you find them useful!''' | ||
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+ | |style="font-family: helvetica, arial, sans-serif;font-size:2em;color:#ea8828;"|Lab Safety | ||
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+ | |We have only worked with Category 1 organisms during the course of our project, and have not used toxic chemicals except when they are in appropriate solutions and therefore safe. | ||
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{| style="width:900px;background:#f5f5f5;text-align:justify;font-family: helvetica, arial, sans-serif;color:#555555;margin-top:5px;" cellspacing="20" | {| style="width:900px;background:#f5f5f5;text-align:justify;font-family: helvetica, arial, sans-serif;color:#555555;margin-top:5px;" cellspacing="20" |
Revision as of 21:09, 23 October 2010
Lab protocols |
Listed below are the protocols we used for the project. We hope you find them useful! |
Lab Safety |
We have only worked with Category 1 organisms during the course of our project, and have not used toxic chemicals except when they are in appropriate solutions and therefore safe. |
Restriction Digests | ||||||||||||||||||||||||||||||||||
Method:
Reaction mixtures:
Or you can use this as a guide:
The buffer depends on the restriction enzymes used. Prefix Insertion:
SpeI doesn’t cut particularly at the end of PCR products particularly well as there are few flanking bases. Can leave overnight and add the second enzyme as a second 90 minute cutting step. |
Ligations |
A typical ligation reaction mixture is around 10 μl and contains
Insert mass (ng) = 6 x (Insert length (bp)/vector length (bp) x Vector mass (ng) Once the solution is made up, the tubes are vortexed and then spun down for around 10 seconds in a microcentrifuge. The ligation is done at 14°C in a water bath in the cold cabinet, and is left overnight. |
E. coli Transformations |
N.B. During pipetting the sides of the tube should not be touched to avoid contamination. Bubbles should be avoided because they can cause the cells stress.
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PCR |
PCR Reaction Mix
PCR programme
(-t°C optimal: 72°C for Taq // time optimal: 2-3kb/60 sec) (-t°C optimal:68°C for Pfu // time optimal: 1kb/15 sec)
We also used a positive control (other DNA to which the primers will definitely anneal) and a negative control (ddH20). The temperature cycle was as follows:
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Overnight Cultures |
Tubes containing 5ml of LB medium are inoculated with cells from one colony and then 5μl of antibiotic (for example chloramphenicol) is added. They are then left at 37°C overnight. |
SDS-PAGE |
Short for: Sodium Dodecyl Sulfate Polyacrylamide Gel Electrophoresis
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Catechol Assay |
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Other Useful Information |
PCR purification
Used to purify DNA to remove primers, salts and enzymes. It can also be used to purify away small fragments from restriction digests, for example when cutting a vector open. We used the E.Z.N.A.® Cycle Pure Kit and protocol (Omega bio-tek) (ddH2O instead of Elusion Buffer used in last step). Gel purification We used the QIAquick® Gel Extraction Kit (250) and protocol (ddH2O instead of Elusion Buffer used in last step).
The [http://www.omegabiotek.com/product_detail.php?ID=21# E.Z.N.A.® Kit] and protocol was used. Midipreps The [http://www.qiagen.com/products/plasmid/qiagenplasmidpurificationsystem/hispeedplasmidmaxikit.aspx#Tabs=t0 QIAGEN HiSpeed Plasmid Midi Kit] and protocol was used. Agarose gels
Diluting Primers
Oligo annealing
Sequencing reaction mix
DpnI Digests DpnI digests methylated DNA, such as template DNA extracted from cells (colony PCR/Mini/Midi-prep), while leaving non-methylated PCR products uncut.
Rapid Alkaline Phosphotase Dephosphorylation useful to prevent vector self re-ligation.
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