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- Posts: 52
- Joined: Mon Jun 25, 2007 1:12 pm
Hello,
How can I remove DBAA from a C18 column?
Previously, I wanted to remove TBAhydrogensulfate from a column and the advice was: try to flush it with the same buffer, but without IP agent.
When I apply the same theory in this case, I should flush the column with pure water? (the column I am tying to regenerate now is Synergi Hydro C18, Phenomenex, 250x2.0 mm 4um particle size). We were using 10 mM DBAA pH=7.
I want the IP agent removed, because after several runs, slight loss of retention was observed but the main problem is loss of separation.
Any suggestions? Thanks, PHOBIUS
How can I remove DBAA from a C18 column?
Previously, I wanted to remove TBAhydrogensulfate from a column and the advice was: try to flush it with the same buffer, but without IP agent.
When I apply the same theory in this case, I should flush the column with pure water? (the column I am tying to regenerate now is Synergi Hydro C18, Phenomenex, 250x2.0 mm 4um particle size). We were using 10 mM DBAA pH=7.
I want the IP agent removed, because after several runs, slight loss of retention was observed but the main problem is loss of separation.
Any suggestions? Thanks, PHOBIUS
