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- Posts: 2
- Joined: Fri Oct 19, 2012 12:23 pm
Hi,
I'm having a problem with our RP method for insulin and I was wondering if anyone can suggest anything to help.
When we run our very shallow insulin gradient (30-32%) B the main peak elution time moves around by up to 5 minutes (it's only a 15 minute run including a 5min wash step and 2 min re-equilibration). This is causing me to miss some of the smaller peaks on either side we are interested in and sometimes moves the main peak out of range entirely, either into the wash step or into the phenol and cresol early eluting peaks. We have had this problem with both longer and shorter RP columns but it is a much bigger problem during the short runs.
Increasing the wash and re-equilibration times has helped a little but I still have this problem over the course of a run (~30 samples) and cannot increase the run time much further without having a serious impact on resources (the reason we switched to the small column). Initially the retention time got lower with every sample injected, however now I see the main peak moving without any apparent trends from one end of the chromatogram to the other.
I think that the presence of the aromatic preservatives in our samples is likely to be causing this problem but cannot pre-treat the sample to remove them.
Many thanks for any ideas
Nikki
Column: ACE 3 C18 100 x4 mm
Buffer A: Water/0.1% TFA
Buffer B: ACN/0.1% TFA
(a similar problem was encountered using buffers containing sodium sulphate)
I'm having a problem with our RP method for insulin and I was wondering if anyone can suggest anything to help.
When we run our very shallow insulin gradient (30-32%) B the main peak elution time moves around by up to 5 minutes (it's only a 15 minute run including a 5min wash step and 2 min re-equilibration). This is causing me to miss some of the smaller peaks on either side we are interested in and sometimes moves the main peak out of range entirely, either into the wash step or into the phenol and cresol early eluting peaks. We have had this problem with both longer and shorter RP columns but it is a much bigger problem during the short runs.
Increasing the wash and re-equilibration times has helped a little but I still have this problem over the course of a run (~30 samples) and cannot increase the run time much further without having a serious impact on resources (the reason we switched to the small column). Initially the retention time got lower with every sample injected, however now I see the main peak moving without any apparent trends from one end of the chromatogram to the other.
I think that the presence of the aromatic preservatives in our samples is likely to be causing this problem but cannot pre-treat the sample to remove them.
Many thanks for any ideas
Nikki
Column: ACE 3 C18 100 x4 mm
Buffer A: Water/0.1% TFA
Buffer B: ACN/0.1% TFA
(a similar problem was encountered using buffers containing sodium sulphate)
