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An extended method for separating and quantitating molecular species of phospholipids
Author(s) -
Wiley Margaret G.,
Przetakiewicz Marek,
Takahashi Mareyuki,
Lowenstein John M.
Publication year - 1992
Publication title -
lipids
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.601
H-Index - 120
eISSN - 1558-9307
pISSN - 0024-4201
DOI - 10.1007/bf02536479
Subject(s) - chromatography , phospholipid , derivatization , chemistry , absorbance , quantitative analysis (chemistry) , silica gel , high performance liquid chromatography , biochemistry , membrane
AN improved and extended method for separating and quantitating molecular species of four phospholipid classes is presented. Crude lipid extract is first separated into phospholipid classes on a silica column. Each phospholipid class is then separated into molecular species without derivatization using high‐performance liquid chromatography on columns packed with octadecyl silica. Quantitation of individual species is achieved by measuring absorbance at 205 nm. Factors for converting absorbancies to mol fractions have been determined. Quantitation by absorbance at 205 nm agrees well with quantitation by gas chromatography which is preferred to quantitation by phosphate analysis. One hundred phospholipid species have been identified. A table of relative retention times of molecular species is provided. Examples of quantitative analyses of species composition are presented.