Purification of cyclic fatty acid esters: a GC-MS study

Gas chromatographic analysis of cyclic monomeric concentrates and fractions from argentation chromatography on packed columns containing SE-30, OV-25 and Apiezon L stationary phases yielded incompletely separated peaks representing the various isomers present in the mixture. Somewhat better separation was achieved using a 6 ft×1/8 in. column packed with 15% EGS on Chromosorb W. This column, when coupled to a mass spectrometer, yielded information concerning the composition of each of the isomeric components. Comparable results were obtained using a 50 ft×0.02 in. S.C.O.T. column with DEGS stationary phase and a 150 ft×0.01 in. capillary column coated with Apiezon L. While argentation thin layer chromatography proved useful, an argentation column method using silicic acid coated with 10% AgNO₃ proved more efficient for larger scale preparations. Elution of the column with 2% diethyl ether in petroleum ether yielded material essentially free of conjugated linolenate. A comparison of the behavior upon argentation thin layer chromatography of conjugated methyl linolenate, methyl linoleate and cyclic monomer esters indicated that these esters migrated to the same relative position as methyl oleate. Presented at the AOCS Meeting, Los Angeles, April 1972. Abstracted in part from the dissertation to be submitted to the University of Illinois Graduate College in partial fulfillment of the requirements for the Ph.D. degree.