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凝集素与变形链球菌细胞及型特异性多糖的结合及其对黏附的影响。

Binding of lectins to Streptococcus mutans cells and type-specific polysaccharides, and effect on adherence.

作者信息

Hamada S, Gill K, Slade H D

出版信息

Infect Immun. 1977 Dec;18(3):708-16. doi: 10.1128/iai.18.3.708-716.1977.

Abstract

The lectin concanavalin A (Con A) agglutinated the cells of 13 of 15 strains of the seven serotypes of Streptococcus mutans in an 18-h incubation period. Strains of types a, d, f, and g agglutinated within 2 h. Strains of a, d, and f were also agglutinated in 2 h by the castor bean lectin RCA. S. sanguis, S. salivarius, S. bovis, Actinomyces viscosus, A. naeslundii, and Lactobacillus plantarum were agglutinated within 2 h. The S. mutans type f polysaccharide was precipitated by Con A. The a, b, c, d, and e polysaccharides were not precipitated. Glucan from d and e strains of S. mutans and dextran T2000 were also precipitated by Con A. D-glucose inhibited the agglutination of type f cells by Con A and the agglutination of type d cells by D-galactose. The quantity of [acetyl-3H]Con A bound was not proportional to the degree of agglutination. Cells grown in sucrose medium bound more Con A than those grown in glucose medium. After treatment with dextranase, the sucrose-grown cells bound two- to fourfold more Con A. The binding of Con A to the type-specific polysaccharide or to teichoic acid could not be determined by the use of specific antibody due to the binding of Con A to the antibody globulin on the cell surface. Con A bound to S. mutans cells did not inhibit the activity of cell-bound glucosyltransferase, glucan synthesis, and in vitro adherence. Bound Con A also did not inhibit the ability of heat-treated cells to bind glucosyltransferase, synthesize glucan, and produce in vitro adherence.

摘要

在18小时的培养期内,凝集素伴刀豆球蛋白A(Con A)使变形链球菌7个血清型中15个菌株中的13个菌株的细胞发生凝集。a、d、f和g型菌株在2小时内发生凝集。a、d和f型菌株在2小时内也被蓖麻籽凝集素RCA凝集。血链球菌、唾液链球菌、牛链球菌、粘性放线菌、内氏放线菌和植物乳杆菌在2小时内发生凝集。变形链球菌f型多糖可被Con A沉淀。a、b、c、d和e型多糖不能被沉淀。变形链球菌d和e型菌株的葡聚糖以及葡聚糖T2000也可被Con A沉淀。D -葡萄糖抑制Con A对f型细胞的凝集以及D -半乳糖对d型细胞的凝集。结合的[乙酰 - 3H]Con A的量与凝集程度不成正比。在蔗糖培养基中生长的细胞比在葡萄糖培养基中生长的细胞结合更多的Con A。用葡聚糖酶处理后,在蔗糖培养基中生长的细胞结合的Con A多两到四倍。由于Con A与细胞表面的抗体球蛋白结合,无法通过使用特异性抗体来确定Con A与型特异性多糖或磷壁酸的结合。结合到变形链球菌细胞上的Con A不抑制细胞结合的葡糖基转移酶的活性、葡聚糖合成以及体外黏附。结合的Con A也不抑制热处理细胞结合葡糖基转移酶、合成葡聚糖以及产生体外黏附的能力。

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