LC-MS Analyses of Lipid Species in Skeletal Muscle Cells and Tissue

Marta Moreno-Torres; Jesper F Havelund; Nils J Faergeman

doi:10.1007/978-1-4939-8897-6_12

LC-MS Analyses of Lipid Species in Skeletal Muscle Cells and Tissue

Marta Moreno-Torres, Jesper F Havelund, Nils J Faergeman

Institut for Biokemi og Molekylær Biologi

Publikation: Kapitel i bog/rapport/konference-proceeding › Kapitel i bog › Forskning › peer review

Abstract

Liquid chromatography-mass spectrometry (LC-MS) is a widely used methodology for measuring lipids at a global level. Combined with an optimal extraction method LC-MS enables the detection and characterization of a wide range of lipid species even of low abundance. Here, we describe two extraction- and LC-MS-based quantitative analytical methods for lipid, acyl-CoA, and acyl-carnitine analyses from either mouse C2C12 myotubes or mouse skeletal tissue. We also describe the use of 13C16-palmitate and its incorporation into acyl-carnitines to show how stable isotope tracers are metabolized within cells and therefore can be implemented for lipidomic flux analysis.

Originalsprog	Engelsk
Titel	Myogenesis : Methods and protocols
Redaktører	Sissel Beate Rønning
Udgivelsessted	New York
Forlag	Humana Press
Publikationsdato	2019
Sider	213-228
Kapitel	12
ISBN (Trykt)	978-1-4939-8896-9
ISBN (Elektronisk)	978-1-4939-8897-6
DOI	https://doi.org/10.1007/978-1-4939-8897-6_12
Status	Udgivet - 2019

Navn	Methods in Molecular Biology
Nummer	1889
ISSN	1064-3745

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10.1007/978-1-4939-8897-6_12

SDU link

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Citationsformater

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title = "LC-MS Analyses of Lipid Species in Skeletal Muscle Cells and Tissue",

abstract = "Liquid chromatography-mass spectrometry (LC-MS) is a widely used methodology for measuring lipids at a global level. Combined with an optimal extraction method LC-MS enables the detection and characterization of a wide range of lipid species even of low abundance. Here, we describe two extraction- and LC-MS-based quantitative analytical methods for lipid, acyl-CoA, and acyl-carnitine analyses from either mouse C2C12 myotubes or mouse skeletal tissue. We also describe the use of 13C16-palmitate and its incorporation into acyl-carnitines to show how stable isotope tracers are metabolized within cells and therefore can be implemented for lipidomic flux analysis.",

keywords = "Acyl-CoA, Acyl-carnitine, C2C12 myotubes, Labeling, Lipidomics, Liquid chromatography, Mass spectrometry, Palmitate, Skeletal muscle tissue, Stable isotope tracers",

author = "Marta Moreno-Torres and Havelund, {Jesper F} and Faergeman, {Nils J}",

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doi = "10.1007/978-1-4939-8897-6_12",

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LC-MS Analyses of Lipid Species in Skeletal Muscle Cells and Tissue. / Moreno-Torres, Marta; Havelund, Jesper F ; Faergeman, Nils J.
Myogenesis: Methods and protocols. red. / Sissel Beate Rønning. New York: Humana Press, 2019. s. 213-228 (Methods in Molecular Biology; Nr. 1889).

Publikation: Kapitel i bog/rapport/konference-proceeding › Kapitel i bog › Forskning › peer review

TY - CHAP

T1 - LC-MS Analyses of Lipid Species in Skeletal Muscle Cells and Tissue

AU - Moreno-Torres, Marta

AU - Havelund, Jesper F

AU - Faergeman, Nils J

PY - 2019

Y1 - 2019

N2 - Liquid chromatography-mass spectrometry (LC-MS) is a widely used methodology for measuring lipids at a global level. Combined with an optimal extraction method LC-MS enables the detection and characterization of a wide range of lipid species even of low abundance. Here, we describe two extraction- and LC-MS-based quantitative analytical methods for lipid, acyl-CoA, and acyl-carnitine analyses from either mouse C2C12 myotubes or mouse skeletal tissue. We also describe the use of 13C16-palmitate and its incorporation into acyl-carnitines to show how stable isotope tracers are metabolized within cells and therefore can be implemented for lipidomic flux analysis.

AB - Liquid chromatography-mass spectrometry (LC-MS) is a widely used methodology for measuring lipids at a global level. Combined with an optimal extraction method LC-MS enables the detection and characterization of a wide range of lipid species even of low abundance. Here, we describe two extraction- and LC-MS-based quantitative analytical methods for lipid, acyl-CoA, and acyl-carnitine analyses from either mouse C2C12 myotubes or mouse skeletal tissue. We also describe the use of 13C16-palmitate and its incorporation into acyl-carnitines to show how stable isotope tracers are metabolized within cells and therefore can be implemented for lipidomic flux analysis.

KW - Acyl-CoA

KW - Acyl-carnitine

KW - C2C12 myotubes

KW - Labeling

KW - Lipidomics

KW - Liquid chromatography

KW - Mass spectrometry

KW - Palmitate

KW - Skeletal muscle tissue

KW - Stable isotope tracers

U2 - 10.1007/978-1-4939-8897-6_12

DO - 10.1007/978-1-4939-8897-6_12

M3 - Book chapter

C2 - 30367416

SN - 978-1-4939-8896-9

T3 - Methods in Molecular Biology

SP - 213

EP - 228

BT - Myogenesis

A2 - Rønning, Sissel Beate

PB - Humana Press

CY - New York

ER -

LC-MS Analyses of Lipid Species in Skeletal Muscle Cells and Tissue

Abstract

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