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- Posts: 7
- Joined: Wed Jul 31, 2013 12:37 pm
Hi everybody, i am a new user on this chromatography forum.
I will try to explain my problem :
I have a difficulty with the last step evaporation/reconstitution under nitrogen after L/L extraction of serum/plasma. After evaporation, i can see a depot in the tube (i think it’s normal). But after reconstitution, i can’t resolubilise this depot and the solution is not limpid.
Anyone can give me a idea to solve my problem, or an advice.
More precision :
I work with a LC-MS/MS in reversed phase with a gradient of methanol in water, in therapeutic drug monitoring of antiepileptics.
The extraction solvant i evaporate is a mixture of acetonitrile and ethyl acetate.
The reconstitution solvant is a mixture of methanol/water (solvant used in the chromatography). I can’t use more than 30% of methanol in reconstitution solvant because of apparition of an “elutropic effet”.
Thank you for your help
I will try to explain my problem :
I have a difficulty with the last step evaporation/reconstitution under nitrogen after L/L extraction of serum/plasma. After evaporation, i can see a depot in the tube (i think it’s normal). But after reconstitution, i can’t resolubilise this depot and the solution is not limpid.
Anyone can give me a idea to solve my problem, or an advice.
More precision :
I work with a LC-MS/MS in reversed phase with a gradient of methanol in water, in therapeutic drug monitoring of antiepileptics.
The extraction solvant i evaporate is a mixture of acetonitrile and ethyl acetate.
The reconstitution solvant is a mixture of methanol/water (solvant used in the chromatography). I can’t use more than 30% of methanol in reconstitution solvant because of apparition of an “elutropic effet”.
Thank you for your help
