Team:Imperial College London/Protocol
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{{:Team:Imperial_College_London/Templates/Header}} | {{:Team:Imperial_College_London/Templates/Header}} | ||
{| style="width:900px;background:#f5f5f5;text-align:justify;font-family: helvetica, arial, sans-serif;color:#555555;margin-top:25px;" cellspacing="20" | {| style="width:900px;background:#f5f5f5;text-align:justify;font-family: helvetica, arial, sans-serif;color:#555555;margin-top:25px;" cellspacing="20" | ||
+ | |style="font-family: helvetica, arial, sans-serif;font-size:2em;color:#ea8828;"|Lab protocols | ||
+ | |- | ||
+ | |'''Listed below are the protocols we used for the project. We hope you find them useful!''' | ||
+ | |} | ||
+ | {| style="width:900px;background:#f5f5f5;text-align:justify;font-family: helvetica, arial, sans-serif;color:#555555;margin-top:5px;" cellspacing="20" | ||
|style="font-family: helvetica, arial, sans-serif;font-size:2em;color:#ea8828;"|Restriction Digests | |style="font-family: helvetica, arial, sans-serif;font-size:2em;color:#ea8828;"|Restriction Digests | ||
|- | |- | ||
|'''Method:''' | |'''Method:''' | ||
- | #Determine the concentration of the DNA sample by running both the vector and insert | + | #Determine the concentration of the DNA sample by running both the vector and insert on a 1% agarose gel and comparing the bands intensity with the ladder (concentration known). |
#Calculate how much solution is needed to obtain desired total amount of DNA for digestion. | #Calculate how much solution is needed to obtain desired total amount of DNA for digestion. | ||
#The volume of DNA solution can be no more than 70% of the total solution. Therefore calculate the total volume of digestion (probably around 20µl or 30µl). | #The volume of DNA solution can be no more than 70% of the total solution. Therefore calculate the total volume of digestion (probably around 20µl or 30µl). | ||
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'''Reaction mixtures:''' | '''Reaction mixtures:''' | ||
- | + | <html> | |
+ | <table width="300px" border="0"> | ||
+ | <tr> | ||
+ | <td style="background-color:#FFCC66;height:30px;width:150;text-align:center"><b>Required components</b></td> | ||
+ | <td style="background-color:#FFCC66;height:30px;width:150;text-align:center"><b>Example</b></td> | ||
+ | </tr> | ||
+ | |||
+ | <tr> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">1/20 Enzyme 1</td> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">1.5µl EcoRI</td> | ||
+ | </tr> | ||
- | + | <tr> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">1/20 Enzyme 2</td> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">1.5µl PstI</td> | |
- | + | </tr> | |
- | + | ||
- | + | <tr> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">1/10 BSA</td> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">3µl BSA</td> | |
- | + | </tr> | |
- | + | ||
- | + | <tr> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">1/10 Buffer* (x 10)</td> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">3µl Buffer 4 (x 10)</td> | |
- | + | </tr> | |
- | + | ||
- | + | <tr> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">X/10 DNA solution</td> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">20µl DNA (pSB1C3)</td> | |
- | + | </tr> | |
+ | <tr> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">7-X/10 ddH2O</td> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">1µl ddH2O</td> | ||
+ | </tr> | ||
+ | |||
+ | <tr> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Total: 10/10</td> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Total: 30µl</td> | ||
+ | </tr> | ||
+ | </table> | ||
+ | </html> | ||
+ | Or you can use this as a guide: | ||
# 20µl reaction volume unless digesting large amounts of DNA (use 30µl) | # 20µl reaction volume unless digesting large amounts of DNA (use 30µl) | ||
# 4µl DNA (if from Midi-preps, use 8µl Mini-Prep DNA) | # 4µl DNA (if from Midi-preps, use 8µl Mini-Prep DNA) | ||
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'''Prefix Insertion:''' | '''Prefix Insertion:''' | ||
- | + | <html> | |
+ | <table width="450px" border="0"> | ||
+ | <tr> | ||
+ | <td style="background-color:#FFCC66;height:30px;width:150;text-align:center"><b></b></td> | ||
+ | <td style="background-color:#FFCC66;height:30px;width:150;text-align:center"><b>Enzymes used:</b></td> | ||
+ | <td style="background-color:#FFCC66;height:30px;width:150;text-align:center"><b>Required buffer:</b></td> | ||
+ | </tr> | ||
+ | |||
+ | <tr> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Prefix (insert)</td> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">EcoRI & SpeI</td> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Buffer 2</td> | ||
+ | </tr> | ||
- | + | <tr> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Suffix (vector)</td> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">EcoRI & XbaI</td> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">EcoRI buffer</td> | |
- | + | </tr> | |
- | + | ||
+ | </table> | ||
+ | </html> | ||
- | |||
+ | '''Suffix insertion:''' | ||
+ | <html> | ||
+ | <table width="450px" border="0"> | ||
+ | <tr> | ||
+ | <td style="background-color:#FFCC66;height:30px;width:150;text-align:center"><b></b></td> | ||
+ | <td style="background-color:#FFCC66;height:30px;width:150;text-align:center"><b>Enzymes used:</b></td> | ||
+ | <td style="background-color:#FFCC66;height:30px;width:150;text-align:center"><b>Required buffer:</b></td> | ||
+ | </tr> | ||
+ | |||
+ | <tr> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Prefix (vector)</td> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">SpeI & PstI</td> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Buffer 2</td> | ||
+ | </tr> | ||
- | + | <tr> | |
- | + | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Suffix (insert)</td> | |
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">XbaI & PstI</td> | ||
+ | <td style="background-color:#eeeeee;height:30px;width:150 px;text-align:center;">Buffer 3</td> | ||
+ | </tr> | ||
+ | |||
+ | </table> | ||
+ | </html> | ||
- | + | 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. | |
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
- | + | ||
|} | |} | ||
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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" | ||
- | |style="font-family: helvetica, arial, sans-serif;font-size:2em;color:#ea8828;"|E. coli Transformations | + | |style="font-family: helvetica, arial, sans-serif;font-size:2em;color:#ea8828;"|''E. coli'' Transformations |
|- | |- | ||
| | | | ||
*One 15ml tube for each sample, in addition to one for a negative control, is put on ice. | *One 15ml tube for each sample, in addition to one for a negative control, is put on ice. | ||
- | *Tubes containing 1ml LB were incubated in a | + | *Tubes containing 1ml LB were incubated in a water bath is set to 42°C . |
*Between 25µl and 40µl of competent cells is transferred to each tube. | *Between 25µl and 40µl of competent cells is transferred to each tube. | ||
*The cells are left on ice for 10min. | *The cells are left on ice for 10min. | ||
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The temperature cycle was as follows: | The temperature cycle was as follows: | ||
# 95°C for 30 seconds | # 95°C for 30 seconds | ||
- | # 30 cycles of: | + | # 30 cycles of: 95°C for 30 seconds, 62°C for 90 seconds, 68 °C for 30 seconds |
- | 95°C for 30 seconds | + | |
- | + | ||
- | 62°C for 90 seconds | + | |
- | + | ||
- | 68 °C for 30 seconds | + | |
- | + | ||
# 68°C for 10 minutes | # 68°C for 10 minutes | ||
# Hold at 4°C | # Hold at 4°C | ||
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|''Short for:'' Sodium Dodecyl Sulfate Polyacrylamide Gel Electrophoresis | |''Short for:'' Sodium Dodecyl Sulfate Polyacrylamide Gel Electrophoresis | ||
- | # '''Prepare gel''' : Two glass plates are cleaned with ethanol and are fitted into a holder. The separation layer of the gel is prepared first, following the recipe but before and after addition of the last two substances the solution should be inverted. The mixture, that now starts to polymerize, in now pipetted between the glass plates until it reaches the green bar. Around 700µl of ethanol are than added | + | # '''Prepare gel''' : Two glass plates are cleaned with ethanol and are fitted into a holder. The separation layer of the gel is prepared first, following the recipe but before and after addition of the last two substances the solution should be inverted. The mixture, that now starts to polymerize, in now pipetted between the glass plates until it reaches the green bar. Around 700µl of ethanol are than added on top of the gel, which is left to solidify. The separating gel contains 10% acrylamide '''(toxic!)''' that has been polymerized by TEMED. Stacking gel contains less acrylamide for wide pores. After the gel has solidified take out the comb. Once solidified the stacking gel can be prepared using a different recipe but same method. Once the ethanol has been removes the solution is poured onto of the gel and the comb inserted. The gel is now left to solidify. |
# '''Load samples''' : The proteins, which have been denatured by SDS, are loaded into the wells. | # '''Load samples''' : The proteins, which have been denatured by SDS, are loaded into the wells. | ||
# '''Run gels''' : The gel is run at 100V for around 2-3 hours until dye front has reached the bottom of the gel. | # '''Run gels''' : The gel is run at 100V for around 2-3 hours until dye front has reached the bottom of the gel. | ||
- | # '''Analysis of results''' : The gel can be analyzed by staining with Coomassie blue | + | # '''Analysis of results''' : The gel can be analyzed by staining with Coomassie blue or Western Blot. |
|} | |} | ||
{| 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" | ||
|style="font-family: helvetica, arial, sans-serif;font-size:2em;color:#ea8828;"|Catechol Assay | |style="font-family: helvetica, arial, sans-serif;font-size:2em;color:#ea8828;"|Catechol Assay | ||
|- | |- | ||
- | |* Catechol assay is performed in the plate reader on a 96 well plate | + | | |
+ | * Catechol assay is performed in the plate reader on a 96 well plate | ||
* Each well must be filled with 100um of solution | * Each well must be filled with 100um of solution | ||
* Usually use 90ul of cell culture and 10um of catechol solution | * Usually use 90ul of cell culture and 10um of catechol solution | ||
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'''Minipreps''' | '''Minipreps''' | ||
- | E.Z.N.A.® | + | |
+ | The [http://www.omegabiotek.com/product_detail.php?ID=21# E.Z.N.A.® Kit] and protocol was used. | ||
'''Midipreps''' | '''Midipreps''' | ||
- | The QIAGEN HiSpeed Plasmid Midi Kit and protocol was used. | + | |
+ | The [http://www.qiagen.com/products/plasmid/qiagenplasmidpurificationsystem/hispeedplasmidmaxikit.aspx#Tabs=t0 QIAGEN HiSpeed Plasmid Midi Kit] and protocol was used. | ||
'''Agarose gels''' | '''Agarose gels''' | ||
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# 50-100ηg of DNA | # 50-100ηg of DNA | ||
# Label with sequencing labels and make sure that the codes from these are entered on MWG website. | # Label with sequencing labels and make sure that the codes from these are entered on MWG website. | ||
+ | |||
+ | '''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. | ||
+ | |||
+ | # Can use 1µl of DpnI straight in the 25µl PCR product (PCR buffer is sufficient) | ||
+ | # Alternatively use Buffer 4 – does not require BSA. | ||
+ | # Incubate for 1 hr at 37°C | ||
+ | |||
+ | '''Rapid Alkaline Phosphatase''' | ||
+ | |||
+ | Dephosphorylation useful to prevent vector self re-ligation. | ||
+ | # 10µl Total Reaction Volume | ||
+ | # --µl DNA vector ( concentration depends on relative concentrations of the parts to be ligated) | ||
+ | # 1µl Phosphatase buffer | ||
+ | # 1µl Alkaline Phosphatase | ||
+ | # -µl make up 10 µl with ddH2O | ||
+ | |||
|} | |} |
Latest revision as of 23:35, 27 October 2010
Lab protocols |
Listed below are the protocols we used for the project. We hope you find them useful! |
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.
|
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:
|
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
|
Catechol Assay |
|
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 Phosphatase Dephosphorylation useful to prevent vector self re-ligation.
|