Berkeley Protocols
From 2006.igem.org
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<h1>Protocols</h1> | <h1>Protocols</h1> | ||
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Vector: EcoRI, Xba I, Buffer 2<br> | Vector: EcoRI, Xba I, Buffer 2<br> | ||
| - | ==Gel Purification | + | ==Gel Purification== |
| - | Pouring the gel: | + | Pouring the gel:<br> |
| - | 25mL of 1X TAE | + | 25mL of 1X TAE<br> |
| - | About 180mg of agarose powder | + | About 180mg of agarose powder<br> |
| - | Swirl and cover with kimwipe before microwaving for about 45 seconds | + | Swirl and cover with kimwipe before microwaving for about 45 seconds<br> |
| - | Make sure all the agarose is dissolved before pouring into mold | + | Make sure all the agarose is dissolved before pouring into mold<br> |
| - | Use taped off comb and longer mold | + | Use taped off comb and longer mold<br> |
| - | Once the surface of the mold is covered it should be enough volume | + | Once the surface of the mold is covered it should be enough volume<br> |
| - | + | <br> | |
| - | Loading and running the gel: | + | Loading and running the gel:<br> |
| - | Write down the order of samples in the lab notebook | + | Write down the order of samples in the lab notebook<br> |
| - | Spin down tubes briefly in the little centrifuge | + | Spin down tubes briefly in the little centrifuge<br> |
| - | Add 5microliters of loading dye to each tube. | + | Add 5microliters of loading dye to each tube.<br> |
| - | Mix and load slowly into well should be 50-55microliters | + | Mix and load slowly into well should be 50-55microliters<br> |
| - | Use one of the normal lanes for the ladder | + | Use one of the normal lanes for the ladder<br> |
| - | Run at 90-110V for about 40 minutes | + | Run at 90-110V for about 40 minutes<br> |
| - | + | <br> | |
| - | Excising the bands: | + | Excising the bands:<br> |
| - | Get a new razor blade | + | Get a new razor blade<br> |
| - | Before putting the gel on the uv box make sure you have an idea of which lane is vector and which is insert as well as relative sizes. | + | Before putting the gel on the uv box make sure you have an idea of which lane is vector and which is insert as well as relative sizes.<br> |
| - | Prepare 1.5ml tubes for each sample | + | Prepare 1.5ml tubes for each sample<br> |
| - | Once you turn on the uv light be as quick as possible cutting the gel, do not take a picture first. | + | Once you turn on the uv light be as quick as possible cutting the gel, do not take a picture first.<br> |
| - | Put each gel slice in a 1.5ml tube | + | Put each gel slice in a 1.5ml tube<br> |
| - | If you’re not sure if the fragments were the right size then take a picture afterwards, you can compare where you cut to the ladder | + | If you’re not sure if the fragments were the right size then take a picture afterwards, you can compare where you cut to the ladder<br> |
| - | Blank the scale with an empty tube then weigh each sample. | + | Blank the scale with an empty tube then weigh each sample.<br> |
| - | Add 2x volume of buffer QG to each tube. 100mg gets 200microliters of QG | + | Add 2x volume of buffer QG to each tube. 100mg gets 200microliters of QG<br> |
| - | Dissolve in 55C water bath for 10minutes | + | Dissolve in 55C water bath for 10minutes<br> |
| - | Proceed with gel purification protocol | + | Proceed with gel purification protocol<br> |
| - | Elute in 30ml of EB and nanodrop | + | Elute in 30ml of EB and nanodrop<br> |
| - | + | <br> | |
| - | Ligations | + | ==Ligations== |
| - | I usually use 50-100ng of vector which hopefully is about 2-3 microliters. | + | I usually use 50-100ng of vector which hopefully is about 2-3 microliters.<br> |
| - | Then I add insert to a total of 8 microliters so if I used 2 of vector I use 6 of insert | + | Then I add insert to a total of 8 microliters so if I used 2 of vector I use 6 of insert<br> |
| - | Another tube is for vector only so use the same amount of vector as in the normal tube and add to 8microliters of H20 | + | Another tube is for vector only so use the same amount of vector as in the normal tube and add to 8microliters of H20<br> |
| - | Add 1 microliter of ligase buffer | + | Add 1 microliter of ligase buffer<br> |
| - | Add 1 microliter of DNA ligase | + | Add 1 microliter of DNA ligase<br> |
| - | Can put in fridge overnight or move on to transformation immediately | + | Can put in fridge overnight or move on to transformation immediately<br> |
| - | Transformation (chemical) | + | ==Transformation (chemical)== |
| - | Make sure water level in 42 degree incubator is not too low otherwise add some | + | Make sure water level in 42 degree incubator is not too low otherwise add some<br> |
| - | Get appropriate plates and put them in 37C incubator | + | Get appropriate plates and put them in 37C incubator<br> |
| - | Get ice bucket and take out the 5X KCM buffer and sterile water 50ml Falcon tubes from the fridge | + | Get ice bucket and take out the 5X KCM buffer and sterile water 50ml Falcon tubes from the fridge<br> |
| - | Get enough tubes of chemically competent cells (hopefully we will have our own stock) | + | Get enough tubes of chemically competent cells (hopefully we will have our own stock)<br> |
| - | Each tube is enough for two ligations | + | Each tube is enough for two ligations<br> |
| - | Spin the tube down very briefly after thawing on ice and leave it on the ice | + | Spin the tube down very briefly after thawing on ice and leave it on the ice<br> |
| - | Add 70microliters of H20 to each ligation tube | + | Add 70microliters of H20 to each ligation tube<br> |
| - | Add 20microliters of 5X KCM | + | Add 20microliters of 5X KCM<br> |
| - | Finally add 100microliters of cells and put on ice for 20minutes (use timer) | + | Finally add 100microliters of cells and put on ice for 20minutes (use timer)<br> |
| - | After 20 minutes place in 42C water bath for 1.5 minutes | + | After 20 minutes place in 42C water bath for 1.5 minutes<br> |
| - | Remove and place back on ice | + | Remove and place back on ice<br> |
Plate the whole tube’s volume immediately | Plate the whole tube’s volume immediately | ||
Revision as of 09:29, 13 November 2005
Contents |
Protocols
Innoculations
10mL of LB
5microliters of 2000X Amp
10 microliters of 1000X Chloramphenicol
50 microliters of 200X Kan
Half everything if only growing for sequencing
Plasmid Prep
For sequencing elute in 30microliters of H20
For restriction elute in 40microliters of EB
Nanodrop and write concentration on tube with date
Restriction Digest
In PCR tube if running overnight 8hr at 37C
Can add everything to plasmid prep tube if digesting in 37degree water bath (6hr)
5ml 10X BSA
5ml NEB Buffer
37ml of purified plasmid (should be this much after eluting and nanodropping)
1.5mL of Enzyme 1
1.5mL of Enzyme 2
Suffix insertion:
Insert: Spe I, Xba I,Buffer 3
Vector: Spe I, Pst I, Buffer 2
Prefix insertion:
Insert: EcoRI, Spe I, Buffer EcoRI
Vector: EcoRI, Xba I, Buffer 2
Gel Purification
Pouring the gel:
25mL of 1X TAE
About 180mg of agarose powder
Swirl and cover with kimwipe before microwaving for about 45 seconds
Make sure all the agarose is dissolved before pouring into mold
Use taped off comb and longer mold
Once the surface of the mold is covered it should be enough volume
Loading and running the gel:
Write down the order of samples in the lab notebook
Spin down tubes briefly in the little centrifuge
Add 5microliters of loading dye to each tube.
Mix and load slowly into well should be 50-55microliters
Use one of the normal lanes for the ladder
Run at 90-110V for about 40 minutes
Excising the bands:
Get a new razor blade
Before putting the gel on the uv box make sure you have an idea of which lane is vector and which is insert as well as relative sizes.
Prepare 1.5ml tubes for each sample
Once you turn on the uv light be as quick as possible cutting the gel, do not take a picture first.
Put each gel slice in a 1.5ml tube
If you’re not sure if the fragments were the right size then take a picture afterwards, you can compare where you cut to the ladder
Blank the scale with an empty tube then weigh each sample.
Add 2x volume of buffer QG to each tube. 100mg gets 200microliters of QG
Dissolve in 55C water bath for 10minutes
Proceed with gel purification protocol
Elute in 30ml of EB and nanodrop
Ligations
I usually use 50-100ng of vector which hopefully is about 2-3 microliters.
Then I add insert to a total of 8 microliters so if I used 2 of vector I use 6 of insert
Another tube is for vector only so use the same amount of vector as in the normal tube and add to 8microliters of H20
Add 1 microliter of ligase buffer
Add 1 microliter of DNA ligase
Can put in fridge overnight or move on to transformation immediately
Transformation (chemical)
Make sure water level in 42 degree incubator is not too low otherwise add some
Get appropriate plates and put them in 37C incubator
Get ice bucket and take out the 5X KCM buffer and sterile water 50ml Falcon tubes from the fridge
Get enough tubes of chemically competent cells (hopefully we will have our own stock)
Each tube is enough for two ligations
Spin the tube down very briefly after thawing on ice and leave it on the ice
Add 70microliters of H20 to each ligation tube
Add 20microliters of 5X KCM
Finally add 100microliters of cells and put on ice for 20minutes (use timer)
After 20 minutes place in 42C water bath for 1.5 minutes
Remove and place back on ice
Plate the whole tube’s volume immediately
