Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMS

Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMS

Lipids are essential cellular constituents that have many critical roles in physiological functions. They are notably involved in energy storage and cell signaling as second messengers, and they are major constituents of cell membranes, including lipid rafts. As a consequence, they are implicated in...

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Main Authors: Pauline Le Faouder, Julia Soullier, Marie Tremblay-Franco, Anthony Tournadre, Jean-François Martin, Yann Guitton, Caroline Carlé, Sylvie Caspar-Bauguil, Pierre-Damien Denechaud, Justine Bertrand-Michel
Format: Article
Language:English
Published: MDPI AG 2021-05-01
Series:Metabolites
Subjects:
Lipidomic 1
Supercritical Fluids Chromatography 3
Plasma 3
Dry Blood Spot 4
Online Access:https://www.mdpi.com/2218-1989/11/5/305
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spelling doaj-4fc3b54e04f348998f7ad47d9ec30da22021-05-31T23:42:26ZengMDPI AGMetabolites2218-19892021-05-011130530510.3390/metabo11050305Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMSPauline Le Faouder0Julia Soullier1Marie Tremblay-Franco2Anthony Tournadre3Jean-François Martin4Yann Guitton5Caroline Carlé6Sylvie Caspar-Bauguil7Pierre-Damien Denechaud8Justine Bertrand-Michel9MetaboHUB-MetaToul-Lipidomique, MetaboHUB-ANR-11-INBS-0010, Inserm U1297/Université Paul Sabatier Toulouse III, 31432 Toulouse, FranceMetaboHUB-MetaToul-Lipidomique, MetaboHUB-ANR-11-INBS-0010, Inserm U1297/Université Paul Sabatier Toulouse III, 31432 Toulouse, FranceMetaboHUB-MetaToul-Axiom, MetaboHUB-ANR-11-INBS-0010, INRAE Toxalim, Université Paul Sabtier, 31027 Toulouse, FranceMetaboHUB-MetaToul-Lipidomique, MetaboHUB-ANR-11-INBS-0010, Inserm U1297/Université Paul Sabatier Toulouse III, 31432 Toulouse, FranceMetaboHUB-MetaToul-Axiom, MetaboHUB-ANR-11-INBS-0010, INRAE Toxalim, Université Paul Sabtier, 31027 Toulouse, FranceMELISA Core Facility, Laboratoire d’Etude des Résidus et Contaminants dans les Aliments (LABERCA), Oniris, INRΑE, 44307 Nantes, FranceLaboratoire de Biochimie, Hôpital Purpan, CHU Toulouse, 31059 Toulouse, FranceINSERM, UMR1297, Institute of Metabolic and Cardiovascular Diseases, University Paul Sabatier, 31432 Toulouse, FranceINSERM, UMR1297, Institute of Metabolic and Cardiovascular Diseases, University Paul Sabatier, 31432 Toulouse, FranceMetaboHUB-MetaToul-Lipidomique, MetaboHUB-ANR-11-INBS-0010, Inserm U1297/Université Paul Sabatier Toulouse III, 31432 Toulouse, FranceLipids are essential cellular constituents that have many critical roles in physiological functions. They are notably involved in energy storage and cell signaling as second messengers, and they are major constituents of cell membranes, including lipid rafts. As a consequence, they are implicated in a large number of heterogeneous diseases, such as cancer, diabetes, neurological disorders, and inherited metabolic diseases. Due to the high structural diversity and complexity of lipid species, the presence of isomeric and isobaric lipid species, and their occurrence at a large concentration scale, a complete lipidomic profiling of biological matrices remains challenging, especially in clinical contexts. Using supercritical fluid chromatography coupled with high-resolution mass spectrometry, we have developed and validated an untargeted lipidomic approach to the profiling of plasma and blood. Moreover, we have tested the technique using the Dry Blood Spot (DBS) method and found that it allows for the easy collection of blood for analysis. To develop the method, we performed the optimization of the separation and detection of lipid species on pure standards, reference human plasma (SRM1950), whole blood, and DBS. These analyses allowed an in-house lipid data bank to be built. Using the MS-Dial software, we developed an automatic process for the relative quantification of around 500 lipids species belonging to the 6 main classes of lipids (including phospholipids, sphingolipids, free fatty acids, sterols, and fatty acyl-carnitines). Then, we compared the method using the published data for SRM 1950 and a mouse blood sample, along with another sample of the same blood collected using the DBS method. In this study, we provided a method for blood lipidomic profiling that can be used for the easy sampling of dry blood spots.https://www.mdpi.com/2218-1989/11/5/305Lipidomic 1Supercritical Fluids Chromatography 3Plasma 3Dry Blood Spot 4
collection DOAJ
language English
format Article
sources DOAJ
author Pauline Le Faouder
Julia Soullier
Marie Tremblay-Franco
Anthony Tournadre
Jean-François Martin
Yann Guitton
Caroline Carlé
Sylvie Caspar-Bauguil
Pierre-Damien Denechaud
Justine Bertrand-Michel
spellingShingle Pauline Le Faouder
Julia Soullier
Marie Tremblay-Franco
Anthony Tournadre
Jean-François Martin
Yann Guitton
Caroline Carlé
Sylvie Caspar-Bauguil
Pierre-Damien Denechaud
Justine Bertrand-Michel
Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMS
Metabolites
Lipidomic 1
Supercritical Fluids Chromatography 3
Plasma 3
Dry Blood Spot 4
author_facet Pauline Le Faouder
Julia Soullier
Marie Tremblay-Franco
Anthony Tournadre
Jean-François Martin
Yann Guitton
Caroline Carlé
Sylvie Caspar-Bauguil
Pierre-Damien Denechaud
Justine Bertrand-Michel
author_sort Pauline Le Faouder
title Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMS
title_short Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMS
title_full Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMS
title_fullStr Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMS
title_full_unstemmed Untargeted Lipidomic Profiling of Dry Blood Spots Using SFC-HRMS
title_sort untargeted lipidomic profiling of dry blood spots using sfc-hrms
publisher MDPI AG
series Metabolites
issn 2218-1989
publishDate 2021-05-01
description Lipids are essential cellular constituents that have many critical roles in physiological functions. They are notably involved in energy storage and cell signaling as second messengers, and they are major constituents of cell membranes, including lipid rafts. As a consequence, they are implicated in a large number of heterogeneous diseases, such as cancer, diabetes, neurological disorders, and inherited metabolic diseases. Due to the high structural diversity and complexity of lipid species, the presence of isomeric and isobaric lipid species, and their occurrence at a large concentration scale, a complete lipidomic profiling of biological matrices remains challenging, especially in clinical contexts. Using supercritical fluid chromatography coupled with high-resolution mass spectrometry, we have developed and validated an untargeted lipidomic approach to the profiling of plasma and blood. Moreover, we have tested the technique using the Dry Blood Spot (DBS) method and found that it allows for the easy collection of blood for analysis. To develop the method, we performed the optimization of the separation and detection of lipid species on pure standards, reference human plasma (SRM1950), whole blood, and DBS. These analyses allowed an in-house lipid data bank to be built. Using the MS-Dial software, we developed an automatic process for the relative quantification of around 500 lipids species belonging to the 6 main classes of lipids (including phospholipids, sphingolipids, free fatty acids, sterols, and fatty acyl-carnitines). Then, we compared the method using the published data for SRM 1950 and a mouse blood sample, along with another sample of the same blood collected using the DBS method. In this study, we provided a method for blood lipidomic profiling that can be used for the easy sampling of dry blood spots.
topic Lipidomic 1
Supercritical Fluids Chromatography 3
Plasma 3
Dry Blood Spot 4
url https://www.mdpi.com/2218-1989/11/5/305
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