Difference between revisions of "Team:Warwick/Protocols"

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Line 73:

transfer to -80 freezer.

</p>

+

<h3> Chemical transformation </h3>

+

<p> 1. Take chemically competent cells (-80C freezer) and thaw on ice/water mix.

+

<br> 2. Add plasmid DNA to 50uL of competent cells: for minipreps 0.5-1 uL of DNA is enough, for ligations, use 5-10 uL. Mix thoroughly.

+

<br> 3. Leave on ice for 30-45 minutes. Turn on the waterbath set to 42C, so it reaches the target temperature over this time.

+

<br> 4. Heat shock the cells at 42C for 30 seconds. This will create pores in the competent cells through which the plasmid can enter into the cell.

+

<br> 5. Put back on ice for 2 minutes. This allows the cell to recover and begin repairing the pores, preventing cell death.

+

<br> 6. Add 950uL of growth media (e.g. SOC, LB, etc.) bringing the volume up to ~1000uL

+

<br> 7. Incubate with shaking at 37C for 45-60 minutes.

+

<br> 8. Plate 200uL on appropriate antibiotic: If using a ligation (or anything likely to have low efficiency) centrifuge the cells first at 8000rpm for 2 minutes and resuspend in 200uL of media then plate everything. If there are still some cells left after plating, the rest can be kept up to 3 weeks in a 4 degree fridge.

+

<br> 9. Incubate overnight at 37C.

+

</p>

+

<p>

Line 99:

Line 112:

<br>

−

~~<h3> Chemical transformation </h3>~~

−

~~<p> - Take chemically competent cells (-80C freezer) and thaw on ice/water mix.~~

−

~~<br> - Add plasmid DNA to 50uL of competent cells: for minipreps 0.5-1 uL of DNA is enough, for ligations, use 5-10 uL. Mix thoroughly.~~

−

~~<br> - Leave on ice for 30-45 minutes. Turn on the waterbath set to 42C, so it reaches the target temperature over this time.~~

−

~~<br> - Heat shock the cells at 42C for 30 seconds. This will create pores in the competent cells through which the plasmid can enter into the cell.~~

−

~~<br> - Put back on ice for 2 minutes. This allows the cell to recover and begin repairing the pores, preventing cell death.~~

−

~~<br> - Add 950uL of growth media (e.g. SOC, LB, etc.) bringing the volume up to ~1000uL~~

−

~~<br> - Incubate with shaking at 37C for 45-60 minutes.~~

−

<br> - Plate 200uL on appropriate antibiotic: If using a ligation (or anything likely to have low efficiency) centrifuge the cells first at 8000rpm for 2 minutes and resuspend in 200uL of media then plate everything. If there are still some cells left after plating, the rest can be kept up to 3 weeks in a 4 degree fridge.

−

~~<br> - Incubate overnight at 37C.~~

−

~~</p>~~

</div>

Difference between revisions of "Team:Warwick/Protocols"

Revision as of 12:52, 17 September 2015

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Protocols

Competent Cell Protocol

Produced chemically competent cells

Chemical transformation

Ethanol Precipitation Protocol

Ethanol Precipitation of DNA Reagents Needed:

Protocol

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@@ Line 73: / Line 73: @@
 transfer to -80 freezer.
 </p>
+<h3> Chemical transformation </h3>
+<p> 1. Take chemically competent cells (-80C freezer) and thaw on ice/water mix.
+<br> 2. Add plasmid DNA to 50uL of competent cells: for minipreps 0.5-1 uL of DNA is enough, for ligations, use 5-10 uL. Mix thoroughly.
+<br> 3. Leave on ice for 30-45 minutes. Turn on the waterbath set to 42C, so it reaches the target temperature over this time.
+<br> 4. Heat shock the cells at 42C for 30 seconds. This will create pores in the competent cells through which the plasmid can enter into the cell.
+<br> 5. Put back on ice for 2 minutes. This allows the cell to recover and begin repairing the pores, preventing cell death.
+<br> 6. Add 950uL of growth media (e.g. SOC, LB, etc.) bringing the volume up to ~1000uL
+<br> 7. Incubate with shaking at 37C for 45-60 minutes.
+<br> 8. Plate 200uL on appropriate antibiotic: If using a ligation (or anything likely to have low efficiency) centrifuge the cells first at 8000rpm for 2 minutes and resuspend in 200uL of media then plate everything. If there are still some cells left after plating, the rest can be kept up to 3 weeks in a 4 degree fridge.
+<br> 9. Incubate overnight at 37C.
+</p>
 <p>
@@ Line 99: / Line 112: @@
 <br>
-<h3> Chemical transformation </h3>
-<p> - Take chemically competent cells (-80C freezer) and thaw on ice/water mix.
-<br> - Add plasmid DNA to 50uL of competent cells: for minipreps 0.5-1 uL of DNA is enough, for ligations, use 5-10 uL. Mix thoroughly.
-<br> - Leave on ice for 30-45 minutes. Turn on the waterbath set to 42C, so it reaches the target temperature over this time.
-<br> - Heat shock the cells at 42C for 30 seconds. This will create pores in the competent cells through which the plasmid can enter into the cell.
-<br> - Put back on ice for 2 minutes. This allows the cell to recover and begin repairing the pores, preventing cell death.
-<br> - Add 950uL of growth media (e.g. SOC, LB, etc.) bringing the volume up to ~1000uL
-<br> - Incubate with shaking at 37C for 45-60 minutes.
-<br> - Plate 200uL on appropriate antibiotic: If using a ligation (or anything likely to have low efficiency) centrifuge the cells first at 8000rpm for 2 minutes and resuspend in 200uL of media then plate everything. If there are still some cells left after plating, the rest can be kept up to 3 weeks in a 4 degree fridge.
-<br> - Incubate overnight at 37C.
-</p>
 </div>