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New electrophoretic and chromatographic techniques for analysis of heparin and heparan sulfate

  • Manuela Viola
  • , Davide Vigetti
  • , Evgenia Karousou
  • , Barbara Bartolini
  • , Anna Genasetti
  • , Manuela Rizzi
  • , Moira Clerici
  • , Francesco Pallotti
  • , Giancarlo De Luca
  • , Alberto Passi

Research output: Contribution to journalArticlepeer-review

Abstract

Heparin (HE) and heparan sulfated glycosaminoglycans are well-known mediators of tissue development, maintenance and functions; the activities of these polysaccharides are depending mainly on their sulfate substitutions. The HE structure is also a very important feature in antithrombotic drug development, since the antithrombin binding site is composed by sequences of a specific sulfation pattern. The analysis of disaccharide composition is then a fundamental point of all the studies regarding HE/heparan sulfate glycosaminoglycan (and thereby proteoglycan) functions. The present work describes two analytical methods to quantify the disaccharides constituting HE and heparan sulfate chains. The use of PAGE of fluorophore-labeled saccharides and HPLC coupled with a fluorescence detector allowed in one run the identification of 90-95% of HE disaccharides and 74-100% of rat kidney purified heparan sulfate. Moreover, the protocol here reported avoid the N-sulfation disaccharides degradation, which may affect N-sulfated/ N-acetylated disaccharides ratio evaluation. These methods could be also very important in clinical treatments since they are useful for monitoring the availability kinetics of antithrombotic drugs, such as low-molecular-weight HEs.

Original languageEnglish
Pages (from-to)3168-3174
Number of pages7
JournalElectrophoresis
Volume29
Issue number15
DOIs
Publication statusPublished - Aug 2008
Externally publishedYes

Keywords

  • 2-Aminoacridone derivatization
  • Fluorescence
  • Glycosaminoglycan
  • Heparin
  • Polyacrylamide gel electrophoresis of fluorophore-labeled saccharides

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