Hepatic receptor that specifically binds oligosaccharides containing fucosyl α1→3
            <i>N</i>
            -acetylglucosamine linkages

Prieels, Jean‐Paul; Pizzo, Salvatore V.; Glasgow, Lowrie R.; Paulson, James C.; Hill, Robert L.

doi:10.1073/pnas.75.5.2215

Cited by 166 publications

(66 citation statements)

References 22 publications

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“…Recently a fucose-binding from the present study, those for rat liver, kidney and brain from [lo], those for human erythrocytes from [12]. The hatched areas in erythrocytes refer to the portion found as poly(glycosy1)peptides [12] protein specific for the sequence Gal(/31+4)[Fuc-(a1 -+ 3)IGlcNAc has been described [5]. The amount of fucose was found to be very low in plasma glycoproteins and it appeared to be bound by other types of linkages, since almost no 3 or 3,4-disubstituted N-acetylglucosamine residues were found to be present.…”

Section: Discussionmentioning

confidence: 99%

Structural Features of the Carbohydrate Units of Plasma Glycoproteins

Finne

Krusius

1979

European Journal of Biochemistry

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For the characterization of the type and relative abundance of different carbohydrate structures in plasma glycoproteins, rat whole plasma was subjected to exhaustive proteolytic digestion and the resulting glycopeptides were fractionated into structurally district groups by chromatography on concanavalin-A-Sepharose followed by mild NaOH/NaBH4 treatment and gel filtration. The most abundant fraction was found to be the biantennary transferrin-type glycopeptides (71 % of recovered carbohydrate) followed by triantennary fetuin-type structures and a smaller proportion of more branched structures (together 24 %), neutral mannose-rich chains ( 2 %) and 0-glycosidic chains (3 x). Structural similarity of the two major fractions to the transferrin and fetuin glycopeptides was supported by similar elution volumes in gel filtration, similar behaviour in concanavalin A affinity chromatography and similar sugar composition and substitution pattern of sugars in methylation analysis.The glycopeptide pattern differs significantly from that observed previously for brain, kidney, liver or erythrocytes, where the more branched structures predominate, and which also contain higher amounts of the neutral mannose-rich chains. As indicated by methylation analysis, the plasma glycoproteins are characterized by carbohydrate units terminating in N-acetylneuraminic acid. The level of terminal galactose, N-acetylglucosamine and fucose residues was low. This finding is in correlation with the described occurrence of binding-activities in liver and other tissues which remove glycoproteins having these sugar terminals from the circulation.

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Section: Discussionmentioning

confidence: 99%

Structural Features of the Carbohydrate Units of Plasma Glycoproteins

Finne

Krusius

1979

European Journal of Biochemistry

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“…Fucose has been shown to be a part of antigenic determinants, including the so called X-antigen (34), and may be also be part of the receptor for the macrophage migration inhibitory factor (35) . A specific hepatic uptake system for the a l ---+ 3 linked fucose has also been described (36) . One of the WGARLots cell lines has been shown to differ from the parent cells with respect to cell adhesion and metastasis (11) .…”

Section: Discussionmentioning

confidence: 99%

Enzymatic basis for a lectin-resistant phenotype: increase in a fucosyltransferase in mouse melanoma cells.

Finne¹,

Burger²,

Prieels³

1982

The Journal of Cell Biology

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In the search for the biochemical basis of the control of glycosylation of cell surface carbohydrates, revertant clones were isolated from previously characterized wheat germ agglutinin-resistant clones of B16 mouse melanoma cells by selection for resistance to Lotus tetragonolobus lectin or to ricin. Comparison of the wheat germ agglutinin-resistant clones with the parent and revertant clones indicated that this phenotype was correlated with an increased sensitivity to the Lotus lectin, a 60-to 70-fold increase in a1 -* 3 fucosyltransferase activity and a decreased sialic acid content of the N-glycosidic chains of glycoproteins . The results suggest a novel type of control mechanism for lectin resistance, an increase in a glycosyltransferase activity . The presence of a1 ---> 3 bound fucose on N-acetylglucosamine residues would interfere with the addition of sialic acid by a2--> 3 linkages to galactose residues in the carbohydrate units, and this change could explain the resistance to wheat germ agglutinin and the increased sensitivity to the Lotus lectin . A change in a regulatory gene for the fucosyltransferase as a possible primary cause for the changed phenotype is discussed.The availability of lectin-resistant cell lines with altered carbohydrate moieties of cell surface glycoproteins and glycolipids has provided a powerful tool for the study of the biosynthesis and function of the complex carbohydrates in animal cells (1-4). Some of the variant cell lines appear to have a block at some level of the biosynthetic pathway of protein-bound oligosaccharides, but the enzymatic basis for the changed phenotype is usually not known . For the study of the biological role of glycoproteins and glycolipids, it would be important to know how the expression of cell surface carbohydrates is regulated.Many lectin-resistant variant cell lines differ from the parent lines with respect to more than one property (5-7). Because the occurrence of more than one genetic or epigenetic change even in single-step isolates cannot be ruled out, it is not known whether all the changes observed could be ascribed to one primary change. Other evidence should therefore be obtained by the isolation of independent variants or revenants (7,8) . The isolation of independent variants has so far been shown only for the lectin-resistant cells with a block in a specific Nacetylglucosaminyltransferase (9, 10), whereas the isolation of revenants has usually not been successful (1, 7) . We report here the isolation of variants and revenants that could be obtained repeatedly as well as their enzymic defect .Previous work from this laboratory has described a wheat THE JOURNAL OF CELL BIOLOGY " VOLUME 92 FEBRUARY 1982 277-282 © The Rockefeller University Press -0021-9525/82/02/0277/06 $1 .00 germ agglutinin (WGA)-resistant mouse melanoma cell line with many altered properties, including changes in cell adhesion and metastasis (11) . Analysis of the protein-bound carbohydrates revealed a structural change involving increased fucose-content and de...

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“…Cells (5 x 105) in 0.1 ml were layered over oil (4 parts silicon oil plus I part mineral oil) in Microfuge (Beckman) tubes. The interaction of ligand with cells was terminated by sedimentation for 30 (6). Previous work has shown that the rate at which -glucuronidase is cleared from plasma is sharply decreased by the simultaneous administration of mannose-or Nacetylglucosamine-terminated glycoproteins (6,8).…”

Section: Methodsmentioning

confidence: 99%

L-Fucose-terminated glycoconjugates are recognized by pinocytosis receptors on macrophages.

Shepherd¹,

Lee²,

Schlesinger³

et al. 1981

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

166

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'MI-Labeled L-fucose-albumin complex and rat preputial fi-glucuronidase are rapidly cleared from plasma after intravenous infusion. L-Fucose-albumin retards the plasma clearance of fi-glucuronidase whereas D-fucose-albumin is inactive. In vitro, '5I-labeled L-fucose-albumin is taken up into rat or rabbit alveolar macrophages by receptor-mediated pinocytosis. Uptake (37°C) is time-dependent, is saturable with increasing ligand concentration (KY e = 4.4 X 10-8M), and requires Ca2". i25ILabeled D-fucose-abumin is poorly taken up. Binding (4°C) is saturable and Ca2+ dependent. Binding and uptake are fully inhibited by yeast mannan. A series of neoglycoproteins, including Lfucose-albumin, were tested as inhibitors of uptake of '25I-labeled 3-glucuronidase into macrophages. The following order of potency was observed:L-Fucose-terminated oligosaccharides coupled to bovine serum albumin also block`5I-labeled (3-glucuronidase uptake into macrophages.

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Hepatic receptor that specifically binds oligosaccharides containing fucosyl α1→3 N -acetylglucosamine linkages

Cited by 166 publications

References 22 publications

Structural Features of the Carbohydrate Units of Plasma Glycoproteins

Structural Features of the Carbohydrate Units of Plasma Glycoproteins

Enzymatic basis for a lectin-resistant phenotype: increase in a fucosyltransferase in mouse melanoma cells.

L-Fucose-terminated glycoconjugates are recognized by pinocytosis receptors on macrophages.

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