Abstract

A novel high performance liquid chromatography method is presented for the separation and identification of intact molecular species of phosphatidylethanolamine (PE). After isocratic separation, detection of species can be achieved by measurement of UV absorbance as well as by the quantitative method of light scattering detection. A mathematical relationship exists between i) the relative retention time of a PE molecular species and ii) the number of carbon atoms and double bonds in the aliphatic groups of the species. This relationship can aid in the identification of the species. Furthermore, the absence of non-volatile components in the solvent allows the use of electrospray mass spectrometry to identify the eluting components and to establish the position of the individual radyl groups at the glycerol backbone. Using this method, samples of bovine heart PE (rich in plasmalogens) and rat liver PE (rich in diacyl species) have been analyzed.

Highlights

  • A novel high performance liquid chromatography method is presented for the separation and identification of intact molecular species of phosphatidylethanolamine (PE)

  • Among the best studied are the asymmetric distribution in the plasma membrane of cells and the particular richness of ether-linked aliphatic groups often found in this phospholipid class

  • In this paper we describe an high performance liquid chromatography (HPLC) method for the rapid analysis of intact PE molecular species, which is capable of good component separation and quantification

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Summary

Introduction

A novel high performance liquid chromatography method is presented for the separation and identification of intact molecular species of phosphatidylethanolamine (PE). Analysis of intact molecular species of phospholipids by high performance liquid chromatography (HPLC) is nowadays the method of choice. We published a method for the quantitative analysis of intact molecular species of PC using a light scattering detector [8].

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