A Major Common Trisulfated Hexasaccharide Core Sequence, Hexuronic Acid(2-Sulfate)-Glucosamine(N-Sulfate)-Iduronic Acid-N-Acetylglucosamine-Glucuronic Acid-Glucosamine(N-Sulfate), Isolated from the Low Sulfated Irregular Region of Porcine Intestinal Heparin

Yamada, Shuhei; Yamane, Yukari; Tsuda, Hiromi; Yoshida, Koichiro; Sugahara, Kazuyuki

doi:10.1074/jbc.273.4.1863

Cited by 33 publications

(31 citation statements)

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“…Together, these data identify the nonreducing disaccharide structure as ⌬HexA(2S)-GlcNS(6S). The complete sequence of heparin hexasaccharide 6-27 identified by IGS was in full agreement with the known sequence established by NMR (16).…”

Section: Resultssupporting

confidence: 66%

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A strategy for rapid sequencing of heparan sulfate and heparin saccharides

Turnbull

Hopwood

Gallagher

1999

Proc. Natl. Acad. Sci. U.S.A.

143

108

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Sulfated glycosaminoglycans (GAGs) are linear polysaccharides of repeating disaccharide sequences on which are superimposed highly complex and variable patterns of sulfation, especially in heparan sulfate (HS). HS and the structurally related heparin exert important biological functions, primarily by interacting with proteins and regulating their activities. Evidence is accumulating that these interactions depend on specific saccharide sequences, but the lack of simple, direct techniques for sequencing GAG saccharides has been a major obstacle to progress. We describe how HS and heparin saccharides can be sequenced rapidly by using an integrated strategy with chemical and enzymic steps. Attachment of a reducing-end fluorescent tag establishes a reading frame. Partial selective chemical cleavage at internal N-sulfoglucosamine residues with nitrous acid then creates a set of fragments of defined sizes. Subsequent digestion of these fragments with combinations of exosulfatases and exoglycosidases permits the selective removal of specific sulfates and monosaccharides from their nonreducing ends. PAGE of the products yields a pattern of fluorescent bands from which the saccharide sequence can be read directly. Data are presented on sequencing of heparin tetrasaccharides and hexasaccharides of known structure; these data show the accuracy and versatility of this sequencing strategy. Data also are presented on the application of the strategy to the sequencing of an HS decasaccharide of unknown structure. Application and further development of this sequencing strategy, called integral glycan sequencing, will accelerate progress in defining the structure-activity relationships of these complex GAGs and lead to important insights into their biological functions.

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Section: Resultssupporting

confidence: 66%

“…26), and heparin hexasaccharide 6-27 was a gift from Kazuyuki Sugahara (University of Kobe, Kobe, Japan; ref. 16). Recombinant exoenzymes were prepared as described below and are available from Oxford Glycosciences (Abingdon, U.K.), which also supplies kits for 2-aminobenzoic acid (2AA)-labeling and PAGE gel solutions.…”

Section: Methodsmentioning

confidence: 99%

A strategy for rapid sequencing of heparan sulfate and heparin saccharides

Turnbull

Hopwood

Gallagher

1999

Proc. Natl. Acad. Sci. U.S.A.

143

108

View full text Add to dashboard Cite

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“…Such a comparison is especially feasible for GlcA/IdoA-containing heparin oligosaccharides, whose gs derivatives survive digestion with heparinase I but are susceptible of cleavage with heparinase II and are amenable to further analysis through their glycol-split derivatives. The structure of the major GlcA/IdoA-containing tetra- and hexasaccharides identified in porcine mucosal heparin (4,49,52,54,55) is shown on row A of Table 3, while row B shows the structures expected for the corresponding glycol-split oligosaccharides. It should be noted that four of the major six heparin tetrasaccharide fragments (Δ4,4,1-A; Δ4,4,1-B; Δ4,4,0-A, and Δ4,5,0) obtained from unmodified heparin upon treatment with heparinase I (4, 54, 55), terminate with a GlcNS,6S reducing residue.…”

Section: Resultsmentioning

confidence: 99%

Profiling glycol-split heparins by high-performance liquid chromatography/mass spectrometry analysis of their heparinase-generated oligosaccharides

Алексеева

Casu

Torri

et al. 2013

Analytical Biochemistry

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Glycol-split (gs) heparins, obtained by periodate oxidation / borohydride reduction of heparin currently used as anticoagulant and antithrombotic drug, are arousing increasing interest in anti-cancer and anti-inflammation therapies. These new medical uses are favored by the loss of anticoagulant activity associated with glycol-splitting-induced inactivation of the antithrombin III (AT) binding site. The structure of gs-heparins has not been studied yet in detail. In this work, an ion-pair reversed-phase chromatography (IPRP-HPLC) coupled with electrospray ionization mass spectrometry (ESI-MS) widely used for unmodified heparin has been adapted to the analysis of oligosaccharides generated by digestion with heparinases of gs-heparins usually prepared from porcine mucosal heparin. The method has been also found very effective in analyzing glycol-split derivatives obtained from heparins of different animal and tissue origin. Besides the major 2-O-sulfated disaccharides, heparinase digests of gs-heparins mainly contain tetra- and hexasaccharides incorporating one or two gs residues, with distribution patterns typical for individual gs-heparins. A heptasulfated, mono-N-acetylated hexasaccharide with two gs residues has been shown to be a marker of the gs-modified AT binding site within heparin chains.

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“…The HS-derived tetrasaccharides Tetra-H1-H3 were isolated from bovine kidney HS after heparitinase digestion (18). The HP-derived tetrasaccharides Tetra-H4 -H8 (19,20) and hexasaccharides Hexa-H1-H5 (21,22) were isolated from porcine intestinal HP after heparinase digestion, whereas the tetrasaccharides Tetra-H9 and H10 (20) were isolated from the same HP preparation 4 A. Kinoshita, T. Inui, and K. …”

Section: Methodsmentioning

confidence: 99%