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Degradation of articular cartilage keratan sulphates using hydrazinolysis and nitrous acid. Environment of fucose residues

TLDR
Alkaline borohydride-reduced keratan sulphate chains from bovine articular cartilage (6-8-year-old animals) were fragmented by an anhydrous hydrazine/nitrous acid procedure, providing a sensitive fingerprinting technique for the assay of KS composition and sub-populations.
Abstract
Alkaline borohydride-reduced keratan sulphate (KS) chains from bovine articular cartilage (6-8-year-old animals) were fragmented by an anhydrous hydrazine/nitrous acid procedure, previously used on KS by Hopwood & Elliott to isolate the major disaccharides from the poly-N-acetyl-lactosamine repeat sequence [Hopwood & Elliott (1983) Carbohydr. Res. 117, 263-274]. The resulting oligosaccharides were reduced with NaB3H4 or NaBH4 and subjected to ion-exchange chromatography on a Nucleosil 5SB column. In addition to the major disaccharides, two fucose-containing oligosaccharides were examined by high-field 1H n.m.r. spectroscopy, and shown to have the following structures (where AnManOH is 2,5-anhydro-D-mannitol): [formula: see text] It is evident that the presence of fucose protects the N-acetylglucosamine residue from de-N-acetylation, and therefore fragments are produced which preserve the immediate environment of the fucose residue. It may be of biosynthetic significance that these two oligosaccharides contain an unsulphated galactose on the non-reducing side of the fucose residue. The hydrazine/nitrous acid/NaB3H4 method followed by h.p.l.c. provides a sensitive fingerprinting technique for the assay of KS composition and sub-populations.

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Structural characterization of the exopolysaccharide produced by Lactobacillus acidophilus LMG9433.

TL;DR: The exopolysaccharide produced by Lactobacillus acidophilus LMG9433 in a semi-defined medium was found to be a charged heteropolymer, with a composition of D-glucose, D-galactose, and 2-acetamido-2-deoxy-D- glucose in molar ratios of 2:1: 1:1.
Journal ArticleDOI

Keratan sulfate disaccharide composition determined by FACE analysis of keratanase II and endo-β-galactosidase digestion products

TL;DR: The data illustrate that the FACE procedure represents an improved approach for accurate compositional microanalyses of corneal and skeletal keratan sulfates, especially applicable to experimentation involving small amounts of this glycosaminoglycan.
Journal ArticleDOI

Human aggrecan keratan sulfate undergoes structural changes during adolescent development.

TL;DR: Alkaline borohydride-reduced keratan sulfate chains were isolated from human articular cartilage aggrecan from individuals of various ages and showed that from birth to early adolescence and during maturation the levels of fucosylation and galactose sulfation continue to increase and α(2–6)-sialylation of the chains occurs.
Journal ArticleDOI

Multiple non-reducing chain termini isolated from bovine corneal keratan sulfates.

TL;DR: Examination of the relative proportions of the capping to the repeat structures and knowledge of the average molecular size suggests that the sum of these non-reducing termini represents the caps of two antennae.
Journal ArticleDOI

An improved method for the structural profiling of keratan sulfates: analysis of keratan sulfates from brain and ovarian tumors.

TL;DR: Keratan sulfates from porcine brain phosphocan and human ovarian tumors have been examined using this methodology, and their structural features are discussed.
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