"
Team:Paris Saclay/Protocols/PCR clean-up
From 2014.igem.org
(Difference between revisions)
(→PCR clean-up) |
(→PCR clean-up) |
||
| (6 intermediate revisions not shown) | |||
| Line 1: | Line 1: | ||
| - | = | + | {{Team:Paris_Saclay/protocols_header}} |
| + | =PCR clean-up= | ||
| - | After the PCR, pool your PCR result in an eppendorf 1,5ml. | + | # After the PCR, pool your PCR result in an eppendorf 1,5ml. |
| - | Add | + | # Add double the amount of PCR result in NTI. |
| - | + | # Centrifuge at 11000g, 30 seconds RT. | |
| - | Centrifuge at 11000g, 30 | + | # Discard the supernatant, wash a first time with 700µl NT3. |
| - | Discard the supernatant, wash first time with 700µl NT3. | + | # Centrifuge at 11000g, 30 secondes RT. |
| - | Centrifuge at 11000g, 30 secondes RT. | + | # Discard the supernatant, wash a second time with 700µl NT3. |
| - | Discard the supernatant, wash a second time with 700µl NT3. | + | # Centrifuge at 11000g, 30 seconds RT. |
| - | Centrifuge at 11000g, 30 | + | # Centrifuge the column empty. |
| - | + | # Add 15-30µl elution buffer and centrifuge at 11000g, 1 min RT. | |
| - | Centrifuge the column empty. | + | # Collect your DNA in an eppendorf 1,5ml. |
| - | + | {{Team:Paris_Saclay/protocols_footer}} | |
| - | Add | + | |
| - | Collect your DNA in an eppendorf 1,5ml. | + | |
Latest revision as of 11:53, 11 August 2014
PCR clean-up
- After the PCR, pool your PCR result in an eppendorf 1,5ml.
- Add double the amount of PCR result in NTI.
- Centrifuge at 11000g, 30 seconds RT.
- Discard the supernatant, wash a first time with 700µl NT3.
- Centrifuge at 11000g, 30 secondes RT.
- Discard the supernatant, wash a second time with 700µl NT3.
- Centrifuge at 11000g, 30 seconds RT.
- Centrifuge the column empty.
- Add 15-30µl elution buffer and centrifuge at 11000g, 1 min RT.
- Collect your DNA in an eppendorf 1,5ml.
