Characterization of antigenic epitopes in anti-ulcer pectic polysaccharides from Bupleurum falcatum L. using several carbohydrases

Characterization of antigenic epitopes in anti-ulcer pectic polysaccharides from Bupleurum falcatum L. using several carbohydrases

A polyclonal antibody (anti-bupleuran 2IIc/PG-1-IgG) against the “ramified” region (PG-1) of an anti-ulcer pectic polysaccharide was prepared and its antigenic epitopes were analyzed by using several carbohydrases. Enzymatic removal of arabinosyl residues from PG-1 by endo-(1→5)- α- l-arabinanase (f...

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Veröffentlicht in:Carbohydrate research 1998-10, Vol.311 (4), p.219-229
Hauptverfasser: Sakurai, Masumi H., Kiyohara, Hiroaki, Matsumoto, Tsukasa, Tsumuraya, Yoichi, Hashimoto, Yohichi, Yamada, Haruki
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Antigenic epitopes
Bupleurum
Bupleurum falcatum L
Carbohydrases
Drugs, Chinese Herbal
Epitope Mapping
Epitopes - chemistry
Epitopes - immunology
Glycoside Hydrolases - metabolism
Pectic polysaccharides
Plant Extracts - immunology
Plant Roots
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container_end_page 229
container_issue 4
container_start_page 219
container_title Carbohydrate research
container_volume 311
creator Sakurai, Masumi H.
Kiyohara, Hiroaki
Matsumoto, Tsukasa
Tsumuraya, Yoichi
Hashimoto, Yohichi
Yamada, Haruki
description A polyclonal antibody (anti-bupleuran 2IIc/PG-1-IgG) against the “ramified” region (PG-1) of an anti-ulcer pectic polysaccharide was prepared and its antigenic epitopes were analyzed by using several carbohydrases. Enzymatic removal of arabinosyl residues from PG-1 by endo-(1→5)- α- l-arabinanase (from Aspergillus niger) did not reduce the binding ability of anti-bupleuran 2IIc/PG-1-IgG to PG-1. When the endo-(1→5)- α- l-arabinanase-resistant fraction (EA-1) was digested with rhamnogalacturonase A (rRGase A from A. aculeatus), a high-molecular-mass fragment fraction (RA-1) and an oligosaccharide fraction (RA-3) were obtained. RA-3 contained at least four kinds of oligosaccharides liberated from the rhamnogalacturonan core. This partial removal of the rhamnogalacturonan core in EA-1 also did not reduce the binding of the antibody to the polysaccharide. Further digestion of RA-1 with exo-(1→3)- β- d-galactanase (from Irpex lacteus), gave a high-molecular-mass fragment (EXG-1) and a trace of oligosaccharides (EXG-3). Methylation and FABMS analyses indicated that EXG-3 contained mono- and di-galactosyl oligosaccharides possessing terminal GlcA or GlcA4Me. Removal of the EXG-3 fraction from RA-1 by exo-(1→3)- β- d-galactanase significantly reduced the ability of the binding of the antibody to the polysaccharide. When PG-1 was digested with endo-(1→6)- β- d-galactanase (from Trichoderma viride) or β- d-glucuronidase (from A. niger), the reactivities of both enzyme-resistant fractions to the antibody were decreased in comparison with that of PG-1. Both radish arabinogalactan (containing GlcA4Me) and β- d-Glc pA-(1→6)- β- d-Gal p-(1→6)- d-Gal p were shown to inhibit the reactivity of PG-1 to the antibody by competitive ELISA. These results suggest that 6-linked galactosyl chains containing terminal GlcA or GlcA4Me attached to (1→3)- β- d-galactosyl chains, are important sugar residues in the antigenic epitopes of the “ramified” region of bupleuran 2IIc.
doi_str_mv 10.1016/S0008-6215(98)00217-1
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Removal of the EXG-3 fraction from RA-1 by exo-(1→3)- β- d-galactanase significantly reduced the ability of the binding of the antibody to the polysaccharide. When PG-1 was digested with endo-(1→6)- β- d-galactanase (from Trichoderma viride) or β- d-glucuronidase (from A. niger), the reactivities of both enzyme-resistant fractions to the antibody were decreased in comparison with that of PG-1. Both radish arabinogalactan (containing GlcA4Me) and β- d-Glc pA-(1→6)- β- d-Gal p-(1→6)- d-Gal p were shown to inhibit the reactivity of PG-1 to the antibody by competitive ELISA. 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Removal of the EXG-3 fraction from RA-1 by exo-(1→3)- β- d-galactanase significantly reduced the ability of the binding of the antibody to the polysaccharide. When PG-1 was digested with endo-(1→6)- β- d-galactanase (from Trichoderma viride) or β- d-glucuronidase (from A. niger), the reactivities of both enzyme-resistant fractions to the antibody were decreased in comparison with that of PG-1. Both radish arabinogalactan (containing GlcA4Me) and β- d-Glc pA-(1→6)- β- d-Gal p-(1→6)- d-Gal p were shown to inhibit the reactivity of PG-1 to the antibody by competitive ELISA. 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Enzymatic removal of arabinosyl residues from PG-1 by endo-(1→5)- α- l-arabinanase (from Aspergillus niger) did not reduce the binding ability of anti-bupleuran 2IIc/PG-1-IgG to PG-1. When the endo-(1→5)- α- l-arabinanase-resistant fraction (EA-1) was digested with rhamnogalacturonase A (rRGase A from A. aculeatus), a high-molecular-mass fragment fraction (RA-1) and an oligosaccharide fraction (RA-3) were obtained. RA-3 contained at least four kinds of oligosaccharides liberated from the rhamnogalacturonan core. This partial removal of the rhamnogalacturonan core in EA-1 also did not reduce the binding of the antibody to the polysaccharide. Further digestion of RA-1 with exo-(1→3)- β- d-galactanase (from Irpex lacteus), gave a high-molecular-mass fragment (EXG-1) and a trace of oligosaccharides (EXG-3). Methylation and FABMS analyses indicated that EXG-3 contained mono- and di-galactosyl oligosaccharides possessing terminal GlcA or GlcA4Me. Removal of the EXG-3 fraction from RA-1 by exo-(1→3)- β- d-galactanase significantly reduced the ability of the binding of the antibody to the polysaccharide. When PG-1 was digested with endo-(1→6)- β- d-galactanase (from Trichoderma viride) or β- d-glucuronidase (from A. niger), the reactivities of both enzyme-resistant fractions to the antibody were decreased in comparison with that of PG-1. Both radish arabinogalactan (containing GlcA4Me) and β- d-Glc pA-(1→6)- β- d-Gal p-(1→6)- d-Gal p were shown to inhibit the reactivity of PG-1 to the antibody by competitive ELISA. These results suggest that 6-linked galactosyl chains containing terminal GlcA or GlcA4Me attached to (1→3)- β- d-galactosyl chains, are important sugar residues in the antigenic epitopes of the “ramified” region of bupleuran 2IIc.</abstract><cop>Netherlands</cop><pub>Elsevier Ltd</pub><pmid>9825524</pmid><doi>10.1016/S0008-6215(98)00217-1</doi><tpages>11</tpages></addata></record>
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subjects Antigenic epitopes
Bupleurum
Bupleurum falcatum L
Carbohydrases
Drugs, Chinese Herbal
Epitope Mapping
Epitopes - chemistry
Epitopes - immunology
Glycoside Hydrolases - metabolism
Pectic polysaccharides
Plant Extracts - immunology
Plant Roots
title Characterization of antigenic epitopes in anti-ulcer pectic polysaccharides from Bupleurum falcatum L. using several carbohydrases
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