Sensitive quantitation of isoglobotriaosylceramide in the presence of isobaric components using electrospray ionization-ion trap mass spectrometry

doi:10.1093/glycob/cwm127

Glycobiology Advance Access originally published online on November 28, 2007
Glycobiology 2008 18(2):166-176; doi:10.1093/glycob/cwm127

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Sensitive quantitation of isoglobotriaosylceramide in the presence of isobaric components using electrospray ionization-ion trap mass spectrometry

Yunsen Li², Dapeng Zhou¹^,3, Chengfeng Xia⁴, Peng G. Wang⁴ and Steven B. Levery¹^,2

² Department of Chemistry, University of New Hampshire, Durham, NH 03824, USA
³ Department of Melanoma Medical Oncology, University of Texas M.D. Anderson Cancer Center, Houston, TX 77054, USA
⁴ Department of Biochemistry, The Ohio State University, Columbus, OH 43210, USA

¹ To whom correspondence should be addressed: Tel: +1-603-862-2529; e-mail: slevery{at}cisunix.unh.edu or Tel: +1-713-792-3134; e-mail: dzhou{at}mdanderson.org

Received on June 21, 2007; revised on October 15, 2007; accepted on November 19, 2007

Isoglobotriaosylceramide (iGb₃) is a stimulatory antigen fora unique type of T cell, Natural Killer T cells. Produced inthe lysosomal compartment by mammalian antigen-presenting cells,iGb₃ is one of the few clearly identified carbohydrate ligandsfor biological receptors. A major source of glycoconjugate structuraldiversity arises from the possibility of forming different linkagesbetween the same monosaccharide units. Globotriaosylceramide(Gb₃) exists as a natural isomer for iGb₃, and both isomersare frequently found together in mixtures of glycosphingolipidsextracted from mammalian cell membranes. Discriminating theseisomers has been feasible using monoclonal antibodies raisedagainst specific carbohydrate epitopes, or by unambiguous structuralcharacterization, which requires relatively large amounts ofpure compounds isolated from grams, or tens of grams, of biologicalsamples. However, the precise detection of iGb₃ from small amountsof biological samples, where it may be mixed with Gb₃ presentin much higher abundance, is a prerequisite for answering furtherimportant biological questions such as stimulation of NKT cells.Here we describe a specific and sensitive method based on iontrap mass spectrometry to discriminate iGb₃ from Gb₃. We alsodemonstrate its application to quantifying the amount of iGb₃in a prototype antigen-presenting cell, rat RBL-CD1d cells,using a chemically synthesized short N-acyl chain iGb₃ as internalstandard. This methodology may have wide implications for functionalglycosphingolipidomics of immune cells and glycosphingolipidbiomarker analysis.

Key words: CD1d / globotriaosylceramide / glycosphingolipid / NKT cell / thymocyte

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