Decoding the Fucose Migration Product during Mass‐Spectrometric analysis of Blood Group Epitopes

Author:

Lettow Maike12ORCID,Greis Kim12ORCID,Mucha Eike1ORCID,Lambeth Tyler R.3,Yaman Murat45,Kontodimas Vasilis4,Manz Christian12ORCID,Hoffmann Waldemar12ORCID,Meijer Gerard1ORCID,Julian Ryan R.3ORCID,von Helden Gert1,Marianski Mateusz45ORCID,Pagel Kevin12ORCID

Affiliation:

1. Fritz-Haber-Intitut der Max-Planck-Gesellschaft Germany

2. Institute of Chemistry and Biochemistry Freie Universität Berlin Germany

3. Department of Chemistry University of California Riverside USA

4. Department of Chemistry and Biochemistry Hunter College The City University of New York USA

5. The PhD Program in Chemistry and Biochemistry The Graduate Center The City University of New York USA

Abstract

AbstractFucose is a signaling carbohydrate that is attached at the end of glycan processing. It is involved in a range of processes, such as the selectin‐dependent leukocyte adhesion or pathogen‐receptor interactions. Mass‐spectrometric techniques, which are commonly used to determine the structure of glycans, frequently show fucose‐containing chimeric fragments that obfuscate the analysis. The rearrangement leading to these fragments—often referred to as fucose migration—has been known for more than 25 years, but the chemical identity of the rearrangement product remains unclear. In this work, we combine ion‐mobility spectrometry, radical‐directed dissociation mass spectrometry, cryogenic IR spectroscopy of ions, and density‐functional theory calculations to deduce the product of the rearrangement in the model trisaccharides Lewis x and blood group H2. The structural search yields the fucose moiety attached to the galactose with an α(1→6) glycosidic bond as the most likely product.

Funder

Fonds National de la Recherche Luxembourg

Directorate for Mathematical and Physical Sciences

National Institute of General Medical Sciences

H2020 European Research Council

Publisher

Wiley

Subject

General Chemistry,Catalysis

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