Improved de novo sequencing of heparin/heparan sulfate oligosaccharides by propionylation of sites of sulfation

Quntao Liang; Pradeep Chopra; Geert-Jan Boons; Joshua S Sharp

doi:10.1016/j.carres.2018.06.002

Improved de novo sequencing of heparin/heparan sulfate oligosaccharides by propionylation of sites of sulfation

Carbohydr Res. 2018 Jul 30:465:16-21. doi: 10.1016/j.carres.2018.06.002. Epub 2018 Jun 8.

Authors

Quntao Liang¹, Pradeep Chopra², Geert-Jan Boons², Joshua S Sharp³

Affiliations

¹ Department of BioMolecular Sciences, School of Pharmacy, University of Mississippi, MS, 38677, USA.
² Complex Carbohydrate Research Center, University of Georgia, Athens, GA, 30602, USA.
³ Department of BioMolecular Sciences, School of Pharmacy, University of Mississippi, MS, 38677, USA. Electronic address: jsharp@olemiss.edu.

Abstract

The structure of heparin and heparan sulfate (Hep/HS) oligosaccharides, as determined by the length and the pattern of sulfation, acetylation, and uronic acid epimerization, dictates their biological function through modulating interactions with protein targets. But fine structural determination is a very challenging task due to the lability of the sulfate modifications and difficulties in separating isomeric HS chains. Previously, we reported a strategy for chemical derivatization involving permethylation, desulfation, and trideuteroperacetylation, combined with standard reverse phase LC-MS/MS that enables the structural sequencing for heparin/HS oligosaccharides of sizes up to dodecasaccharide by positionally replacing all sulfates with more stable trideuteroacetyl groups, allowing for robust MS/MS sequencing. However, isomeric oligosaccharides that contain both N-sulfation and N-acetylation become isotopomers after labeling, differing only in the sites of deuteration. This prevents chromatographic separation of these different mixed domain sequences post-derivatization, and makes sequencing by MS/MS difficult due to co-fragmentation of the isotopomers leading to chimeric product ion spectra. In order to improve chromatographic separation of mixed domain oligosaccharides, we have introduced a propionylation step in place of trideuteroacetylation for labeling of sites of sulfation. HS standard disaccharides have been used to evaluate the efficiency of this improved chemical derivatization. The results show that we can quantitatively replace sulfation with propionyl groups with the same high efficiency as the previously reported trideuteroacetylation. After derivatization, we demonstrate the ability to chromatographically separate two mixed domain tetrasaccharide isomers differing solely by the order of N-sulfation and N-acetylation, allowing for full sequencing of each by MS/MS. These results represent a marked improvement in the ability of our previously reported derivatization strategy to analyze complex mixtures of Hep/HS oligosaccharides without a decrease in sensitivity.

Keywords: Chemical derivatization; Glycosaminoglycans; Heparin/heparan sulfate; LC-MS/MS.

MeSH terms

Carbohydrate Conformation
Heparin / chemical synthesis
Heparin / chemistry*
Heparitin Sulfate / chemical synthesis
Heparitin Sulfate / chemistry*
Oligosaccharides / chemical synthesis
Oligosaccharides / chemistry*
Propionates / chemistry*
Sulfates / chemistry*

Substances

Oligosaccharides
Propionates
Sulfates
Heparin
Heparitin Sulfate

Grants and funding

P41 GM103390/GM/NIGMS NIH HHS/United States