I want to purify a 6XHis-tagged protein from 293T cells, what lysis buffer should I use? After the cell lysis I will use Nickel Resin to purify this protein. Thanks
Hi Yijun
In my experience the buffer choice needs to be made with not only the cell type but the protein you are going to be purifying. For example membrane proteins require different additives, also certain proteins need high salt concentrations to ensure they do not aggregate etc. So more information is needed regarding the protein you will be purifying
Hi, Angela
Thanks for your answer. The protein I want to purify is a cellular protein, not membrane protein. Do you have any suggestions for the normal condition?
Hi Yijun
I personally would start with a Tris base, but this you will have to check with your protein to ensure it is happy in tris. Some proteins need HEPES some need a phosphate base. Then I would add sodium chloride, if your protein tends to aggregate then a high salt concentration is needed. I then use a protease inhibitor of some description (PMSF or a cocktail from a supplier). The a small concentration of imadazole (5mM) because you will use a high concentration of imadazole to elute your protein from a nickel resin.
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