I'm currently trying to set up a standard curve of pure phytol to compare my plant extract and other samples. I've run the HPLC with pure phytol on a C18 column with 10% acetonitrile and 90% water but the separation does not give good peaks. The area under the curve does not give a gradual increase in concentration (concentrations ranging from 0.00001M to 1M) with similar concentrations for each peak.

My solvent for the phytol was isopropenol and I am using a PDA detector to analyse the HPLC results.

If anyone has a method I could look at or suggest any changes it would be greatly appreciated.

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