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- Posts: 66
- Joined: Wed Jun 15, 2005 1:54 pm
Are there instances where it is better to not use glass wool? Unless it's headspace, I use glass wool all of the time.
Currently trying to complete the volatile organic impurities test on Alcohol (95%), USP. Resolution for Acetaldehyde and Methanol cannot be less than 1.5. Visually the two peaks are separated. However, the calulated result is 1.34 and when I blow up a print out of the 2 peaks and perform a manual measure, I get 1.33.
My problem is the asymmetry of the Methanol peak, it's over 2.0 and sticks out like a sore thumb. My column is the Restek Rxi-624MS-Sil: 30m x 0.32mm 1.8 µm film.
This column has been great and the test chromatogram that is included with the column shows a nice symetrical methanol peak along with everything else that was on the test injection. Everything I run on it seems to have better symmetry than when I used a different 624 column. So where is my problem.
I was able to correct some resolution issues by switching to a liner with a gooseneck at the bottom. However the peak shape of the Methanol didn't change drastically. I've varied my injection speed also with negligable impact. Currently it's 5µL/s. Past settings; 50, 25 10µl/s.
Detector: Flame ionization
Column: 0.32-mm × 30-m fused silica capillary column bonded with a 1.8-µm layer of phase G43
Split ratio: 20:1
Temperature
Detector: 280°C
Injector: 200°C
Column:
Initial Temperature: 40°C hold for 12 min
Temperature Ramp: 10°C/min
Final: 240°C for 10 min
Linear velocity: 35 cm/s
Carrier gas: Helium
Injection size: 1.0 µL
Currently trying to complete the volatile organic impurities test on Alcohol (95%), USP. Resolution for Acetaldehyde and Methanol cannot be less than 1.5. Visually the two peaks are separated. However, the calulated result is 1.34 and when I blow up a print out of the 2 peaks and perform a manual measure, I get 1.33.
My problem is the asymmetry of the Methanol peak, it's over 2.0 and sticks out like a sore thumb. My column is the Restek Rxi-624MS-Sil: 30m x 0.32mm 1.8 µm film.
This column has been great and the test chromatogram that is included with the column shows a nice symetrical methanol peak along with everything else that was on the test injection. Everything I run on it seems to have better symmetry than when I used a different 624 column. So where is my problem.
I was able to correct some resolution issues by switching to a liner with a gooseneck at the bottom. However the peak shape of the Methanol didn't change drastically. I've varied my injection speed also with negligable impact. Currently it's 5µL/s. Past settings; 50, 25 10µl/s.
Detector: Flame ionization
Column: 0.32-mm × 30-m fused silica capillary column bonded with a 1.8-µm layer of phase G43
Split ratio: 20:1
Temperature
Detector: 280°C
Injector: 200°C
Column:
Initial Temperature: 40°C hold for 12 min
Temperature Ramp: 10°C/min
Final: 240°C for 10 min
Linear velocity: 35 cm/s
Carrier gas: Helium
Injection size: 1.0 µL
