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- Posts: 3
- Joined: Wed Oct 27, 2004 6:56 pm
Here's the problem:
Day 1 - HPLC system is up and running with 35/65 ACN/Acetone. Flushed for a couple hours and ran a sample of 1% soybean oil (SBO) dissolved in the mobile phase. Being more of a supplemental advisor of the operations (I have some HPLC experience) than the operator (a graduate student never used HPLC before who is working with someone who has limited HPLC experience as well) the UV was operating @ 254 nm (not good for what we wanted) and the DRI cell hadn't been purged.
Day 2 - After switching to 30/70 ACN/Acetone for better solubility and purging the DRI cell along with changing the UV wavelength to 209 nm (for ester in SBO) we obtained a decent chromatogram. The peaks were not as sharp as we would've liked and tailed some, but they resembled what had been done a couple years earlier on the same column. Both UV and DRI signals were in good agreement.
Day 3 - Switched to 70/30 ACN/Acetone ran a more polar small molecule (diester with 2 dioxane rings) that eluted with the solvent peak. Tried a sample of SBO and got a peak with/just after the solvent peak.
Day 4 - Switched back to 30/70 ACN/Acetone and have been unable to reproduce the SBO chromatogram. Some separation, but absolutely awful peak shapes and very small signals (0.06 AU now as opposed to 0.8 AU before) and essentially no signal from the DRI.
Days 5/6 - Flushed system with large amount of mobile phase, switched to strong solvent - THF and flushed. Went back to mobile phase and same problem, what peaks we do see are very small and distorted.
Thoughts I've had but not yet tried - back flushing the column and cleaning/testing the detectors for signal.
We are using a Novopak C18 300x3.9 mm column.
Day 1 - HPLC system is up and running with 35/65 ACN/Acetone. Flushed for a couple hours and ran a sample of 1% soybean oil (SBO) dissolved in the mobile phase. Being more of a supplemental advisor of the operations (I have some HPLC experience) than the operator (a graduate student never used HPLC before who is working with someone who has limited HPLC experience as well) the UV was operating @ 254 nm (not good for what we wanted) and the DRI cell hadn't been purged.
Day 2 - After switching to 30/70 ACN/Acetone for better solubility and purging the DRI cell along with changing the UV wavelength to 209 nm (for ester in SBO) we obtained a decent chromatogram. The peaks were not as sharp as we would've liked and tailed some, but they resembled what had been done a couple years earlier on the same column. Both UV and DRI signals were in good agreement.
Day 3 - Switched to 70/30 ACN/Acetone ran a more polar small molecule (diester with 2 dioxane rings) that eluted with the solvent peak. Tried a sample of SBO and got a peak with/just after the solvent peak.
Day 4 - Switched back to 30/70 ACN/Acetone and have been unable to reproduce the SBO chromatogram. Some separation, but absolutely awful peak shapes and very small signals (0.06 AU now as opposed to 0.8 AU before) and essentially no signal from the DRI.
Days 5/6 - Flushed system with large amount of mobile phase, switched to strong solvent - THF and flushed. Went back to mobile phase and same problem, what peaks we do see are very small and distorted.
Thoughts I've had but not yet tried - back flushing the column and cleaning/testing the detectors for signal.
We are using a Novopak C18 300x3.9 mm column.
- Jay Schlechte
