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- Posts: 9
- Joined: Fri Feb 04, 2011 3:26 am
i'm trying to separate inulin from other sugars (glucose and sucrose) with acetonitril and water as mobile phase, what is the best composition for inulin?
thank you
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Discussions about HPLC, CE, TLC, SFC, and other "liquid phase" separation techniques.
Can you be more specific?the result is not satisfied
I'm sorry to say that the short answer is "no". Those are two quite different separation mechanisms.using the anion column they can measure a total amount of inulin in a single peak. can i do that with propylamino column?
no possibilities at all?I'm sorry to say that the short answer is "no". Those are two quite different separation mechanisms.
What part of "no" is unclear?no possibilities at all?![]()
how about increasing the column temperature?
i mean inulin determination with propylamino column without hydrolysis is impossible ?What part of "no" is unclear?
what kind of chemistry interaction between that separation?The amino bonded phase column will separate the oligos by chain length.
Very few things are impossible. This one is very, very, very improbable.i mean inulin determination with propylamino column without hydrolysis is impossible ?
Carbohydrate separations on amino bonded-phase columns are based on what would be called "HILIC" (hydrophilic interaction chromatography); when they were first done 30+ years ago, it was simply called "normal phase". In essence the analyte molecules partition between a water-rich layer on the surface of the stationary phase (hydrated amino groups) and a relatively water-poor mobile phase (typically 25-35% water). The separation mechanism is based on differential solubility. Since each oligosaccharide has a slightly different solubility, they separate from one another, so you do not get a single peak for "inulin". If the column is efficient enough to completely resolve the oligos, you get a "picket fence" type pattern; it it is not very efficient, you get a "blob" that represents the envelope of the various unresolved oligos.what kind of chemistry interaction between that separation?
If the column is efficient enough to completely resolve the oligos, you get a "picket fence" type pattern; it it is not very efficient, you get a "blob" that represents the envelope of the various unresolved oligos.
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