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Question about peak splitting Vit B1

Discussions about HPLC, CE, TLC, SFC, and other "liquid phase" separation techniques.

4 posts Page 1 of 1
Hi,

I am trying to separate the Vitamin B1 from hemolysed whole blood using a C18 collumn in a reversed phase HPLC system.

I am using a Phospahte buffer mobile phase in a gradient from 5 to 60% Methanol.
Sample hemolysed by temperature schock at -70 °C and then proteins are precipitated with methanol.
Derivatization with Potassium ferricyanide.

TDP (thiamine diphosphate) Calibrators prepared in water.

The problem that I have is that from time to time I get a second peak proportional to the concentration used that comes right after my peak (like a peak-split), even though they are pretty well separated.

Can anybody help me please?

Thanks a lot
Do replicate injections get the peak split from time to time? Or is it certain standards that do it and others don't? I would do 5 replicate injections from the same vial to make sure you get consistency. Split peaks usually come from blocked inlet frits in my experience.
I will try and let you know if it is the case.

Thanks
If it is possibly, please provide us two chromatograms (a good chromatogram and one with double-peak) where comparable conditions were used.
4 posts Page 1 of 1

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