Lecithin liposomes and microemulsions as new chromatographic phases

Susana Amézqueta; Alejandro Fernández-Pumarega; Sandra Farré; Daniel Luna; Elisabet Fuguet; Martí Rosés

doi:10.1016/j.chroma.2019.460596

Lecithin liposomes and microemulsions as new chromatographic phases

J Chromatogr A. 2020 Jan 25:1611:460596. doi: 10.1016/j.chroma.2019.460596. Epub 2019 Oct 2.

Authors

Susana Amézqueta¹, Alejandro Fernández-Pumarega², Sandra Farré², Daniel Luna², Elisabet Fuguet³, Martí Rosés²

Affiliations

¹ Departament de Química Analítica and Institut de Biomedicina (IBUB), Facultat de Química, Universitat de Barcelona, Martí i Franquès 1-11, 08028, Barcelona, Spain. Electronic address: samezqueta@ub.edu.
² Departament de Química Analítica and Institut de Biomedicina (IBUB), Facultat de Química, Universitat de Barcelona, Martí i Franquès 1-11, 08028, Barcelona, Spain.
³ Departament de Química Analítica and Institut de Biomedicina (IBUB), Facultat de Química, Universitat de Barcelona, Martí i Franquès 1-11, 08028, Barcelona, Spain; Serra Húnter Programme. Generalitat de Catalunya. Spain.

PMID: 31610920
DOI: 10.1016/j.chroma.2019.460596

Abstract

Lecithins are phospholipidic mixtures that can be part of microemulsions and liposomes. In this work, ready-to-use preparations of lecithin have been tested as pseudostationary and mobile phases in EKC and LC, respectively. The selectivity of two EKC systems, one based on lecithin microemulsions (LMEEKC) and another on liposomes (LLEKC), and of a LC system based on lecithin microemulsions (MELC) has been evaluated through the solvation parameter model. In all cases, solute volume and hydrogen-bond basicity are the main descriptors that drive the partition process. While solute volume favors the retention of solutes, hydrogen-bond basicity has the contrary effect. In lecithin-based EKC systems the hydrogen-bond acidity of the solute leads to a higher retention while in the lecithin-based LC system a minor retention is produced. The three lecithin systems have been compared through the solvation parameter model to other chromatographic systems, most of them containing phospholipids. Principal component analysis reveals that lecithin systems cluster together with the other EKC systems based on phospholipids, with an immobilized artificial membrane (IAM) LC system, with the octanol/water reference partition system, and with a SDS-based microemulsion. Thus, they all show similar selectivity. However, the great advantage of using the ready-to use lecithin systems is that the laborious liposome preparation is avoided, and that their commercial availability makes them more affordable than IAM LC columns. Finally, taking into account that lecithin has a high semblance to the mammalian cell membranes composition, the ability of the three lecithin systems to mimic the pass of the solutes through the membranes has been evaluated. Experimental determinations have demonstrated that the skin partition of neutral solutes can be easily emulated, especially using the lecithin-microemulsion EKC method. The model is robust and shows good prediction ability.

Keywords: Chromatography; Lecithin; Physicochemical characterization; Skin partition; Solvation parameter model; Surrogation.

MeSH terms

Chromatography, Liquid / instrumentation*
Chromatography, Liquid / methods
Emulsions / chemistry
Hydrogen Bonding
Lecithins / chemistry*
Liposomes / chemistry*
Membranes, Artificial
Octanols / chemistry
Phospholipids / chemistry
Principal Component Analysis

Substances

Emulsions
Lecithins
Liposomes
Membranes, Artificial
Octanols
Phospholipids