21 February 2013 3 3K Report

I am currently trying to precipitate a protein for which I have an antibody targeting a peptide epitope. However, so far it seems likely that the epitope is buried.

I have heard that it is possible to do IP's under denaturing conditions, exposing any buried epitopes. This got me quite excited as it might be just what I need to precipitate my protein.

But I am wondering how do you avoid denaturing the antibodies during such a denatured IP? If the denaturing agent is in the present in the extraction buffer it will denature the antibodies during the binding step. However, I would suspect that removing the denaturing agent would result in refolding or worse.

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