Simple Protein Crosslinking: Difference between revisions
From Powers Wiki
(LearningSorting) |
No edit summary |
||
| (One intermediate revision by the same user not shown) | |||
| Line 20: | Line 20: | ||
*Heat @70C for 1 hour or until paraformaldehyde is dissolved | *Heat @70C for 1 hour or until paraformaldehyde is dissolved | ||
[[category: | [[category:Protein_Preparation]] | ||
[[category:Cell_Culturing]] | [[category:Cell_Culturing]] | ||
Latest revision as of 06:39, 20 January 2022
Simple Protein Crosslinking
- Have tagged, purified protein ready before starting the rest of this procedure.
- Grow up a culture of target cells (500mL is fine).
- Spin down the culture.
- Resuspend the culture in nanopure water and lyse by sonication.
- Spin down the cell debris.
- Freeze the supernatant and lyophilize.
- To the dry protein extract add up to 500uL of tagged protein (make sure you have at least 2mg of tagged protein).
- Add crosslinking buffer at RT, 2mL.
- Let sit at RT for 15 min and swirl gently every min.
- Quench reaction with 1.25M glycine.
- The solution is now ready to be purified with an affinity column.
Crosslinking Buffer:
- 1% paraformaldehyde
- 1x PBS buffer
- pH > 7, aim for 8
- Heat @70C for 1 hour or until paraformaldehyde is dissolved