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- Joined: Mon Feb 11, 2008 8:42 pm
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Discussions about HPLC, CE, TLC, SFC, and other "liquid phase" separation techniques.
If it never elutes completely, what's your reference then for complete elution? Did you check peak area without any column? (Assuming you dialyzed the sample extensively against your loading buffer.) And how much exactly are you missing? (Are you sure there are absolutely no aggregates in your sample? How did you determine concentration of the sample?I have a particular protein that binds nicely to all RP columns, but does not elute completely, even on the weakest RP phases. Avoiding the modes of HIC and IEX, if we stay with RP, does anyone have any experience with this problem and can recommend a stronger buffer system or different type of RP column that can hopefully elute this problem child.
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