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- Posts: 3
- Joined: Wed Sep 18, 2013 2:48 am
Hello,
I met some problems with our HPLC. Before I do more checks or cleaning, I'd like to hear some opinions. Thanks!
The HPLC is Shimadzu, SPD-M20A PDA detector. Binary gradient. Solvents are 0.1% formic acid and acetonitrile.
A few weeks ago I've seen spikes in the chromatogram across all wavelength (see picture.)
http://s42.photobucket.com/user/shennon ... e.png.html
According to the manual, the spikes are air bubbles flowing through flow cell. So I disassembled and cleaned the flow cell and replaced the lens. The spikes were gone.
Last week I ran some enzyme reaction products, and spikes were observed at the end when pressure dropped. I ran a lot of solvent washes because sample concentrations were too high in the reaction products. Then I started to see the abnormal spikes in my chromatograms when I ran blanks (50% methanol) (see picture).
http://s42.photobucket.com/user/shennon ... c.png.html
Later I started to see the wide absorption in the chromatogram (see picture) after I purged the autosampler (function of SIL-20AC).
http://s42.photobucket.com/user/shennon ... 5.png.html
I think spikes are bubbles in the flow cell. Wide absorption is caused by dirt in the flow cell. I'm thinking of trying the following things.
1. Remove column and wash the flow line with 95:5 acetonitrile/formic acid at 2 mL/min for hours. Hopefully, dirt and air will be washed out.
2. If the problem is not gone, take out the flow cell and flush with solvent.
Following is what I found on the forum. viewtopic.php?f=1&t=2394&start=0&hilit= ... +flow+cell
3. If this does not help, I will have to disassemble the flow cell and sonicate the lens and cell window.
A final question is about the spikes at the end. I guess air bubbles come out of solvent when pressure drops, like bubbles come out when you open a coke. But we have never seen that before.
We have a 2-foot narrow tubing after the outlet. Is there general guideline about how much tubing it needs?
We use house vacuum and filter to degas 0.1% formic acid and never degas acetonitrile. The vacuum is very weak than it used to be, taking longer to degas same amount of solvent now. Is it possible that degassing is not sufficient?
Any suggestions will be appreciated. Thank you a lot in advance!
I met some problems with our HPLC. Before I do more checks or cleaning, I'd like to hear some opinions. Thanks!
The HPLC is Shimadzu, SPD-M20A PDA detector. Binary gradient. Solvents are 0.1% formic acid and acetonitrile.
A few weeks ago I've seen spikes in the chromatogram across all wavelength (see picture.)
http://s42.photobucket.com/user/shennon ... e.png.html
According to the manual, the spikes are air bubbles flowing through flow cell. So I disassembled and cleaned the flow cell and replaced the lens. The spikes were gone.
Last week I ran some enzyme reaction products, and spikes were observed at the end when pressure dropped. I ran a lot of solvent washes because sample concentrations were too high in the reaction products. Then I started to see the abnormal spikes in my chromatograms when I ran blanks (50% methanol) (see picture).
http://s42.photobucket.com/user/shennon ... c.png.html
Later I started to see the wide absorption in the chromatogram (see picture) after I purged the autosampler (function of SIL-20AC).
http://s42.photobucket.com/user/shennon ... 5.png.html
I think spikes are bubbles in the flow cell. Wide absorption is caused by dirt in the flow cell. I'm thinking of trying the following things.
1. Remove column and wash the flow line with 95:5 acetonitrile/formic acid at 2 mL/min for hours. Hopefully, dirt and air will be washed out.
2. If the problem is not gone, take out the flow cell and flush with solvent.
Following is what I found on the forum. viewtopic.php?f=1&t=2394&start=0&hilit= ... +flow+cell
In this procedure, is flush done using syringe? Any tips about avoiding air using syringe? And what does 30% nitric acid do?Flowcell cleaning procedure:
Flush with methanol followed by water to remove all of the methanol.
Flush with up to 30% nitric acid. Leave the acid in the flowcell for 5-10 minutes then continue flushing.
Flush with water until ALL of the acid is removed then flush again with methanol.
If this doesn't work, you will have to find the detector manual and take apart the flowcell to clean the windows. Be aware that you may need to buy new flowcell windows and gaskets.
3. If this does not help, I will have to disassemble the flow cell and sonicate the lens and cell window.
A final question is about the spikes at the end. I guess air bubbles come out of solvent when pressure drops, like bubbles come out when you open a coke. But we have never seen that before.
We have a 2-foot narrow tubing after the outlet. Is there general guideline about how much tubing it needs?
We use house vacuum and filter to degas 0.1% formic acid and never degas acetonitrile. The vacuum is very weak than it used to be, taking longer to degas same amount of solvent now. Is it possible that degassing is not sufficient?
Any suggestions will be appreciated. Thank you a lot in advance!
