Hi, I think that a good choice, if your protein accept, is to try a gel filtration at high salt, with or without DNAse incubation before gel filtration. If your FPLC can do it, a monitoring at 280 and 260 nm will help you.
Michel
- [ccp4bb] How to remove nucleic acid contaminat... tony_htc
- Re: [ccp4bb] How to remove nucleic acid c... Ana Silva
- Re: [ccp4bb] How to remove nucleic ac... Pavan
- Re: [ccp4bb] How to remove nuclei... William Scott
- Re: [ccp4bb] How to remove nu... Jeffrey . Kieft
- Re: [ccp4bb] How to remo... Raji Edayathumangalam
- Re: [ccp4bb] How to ... Dominique Monferrer Ventura
- Re: [ccp4bb] How to remo... Benini, Stefano
- Re: [ccp4bb] How to ... Dominique Monferrer Ventura
- Re: [ccp4bb] How to remove nu... M T
- Re: [ccp4bb] How to remove nucleic acid c... Pierre Barraud
