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链球菌脂磷壁酸的红细胞结合特性

Erythrocyte binding properties of streptococcal lipoteichoic acids.

作者信息

Beachey E H, Dale J B, Simpson W A, Evans J D, Knox K W, Ofek I, Wicken A J

出版信息

Infect Immun. 1979 Mar;23(3):618-25. doi: 10.1128/iai.23.3.618-625.1979.

DOI:10.1128/iai.23.3.618-625.1979
PMID:378832
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC414210/
Abstract

The lipoteichoic acids (LTA) of gram-positive bacteria are known to bind spontaneously to a variety of animal cell membranes. We investigated the biological and biochemical characteristics of the binding of LTA of Streptococcus pyogenes and S. faecalis to human and sheep erythrocytes. The kinetics of the binding of the radiolabeled LTA ([(3)H]LTA) from each of these organisms to erythrocytes was similar. The dissociation constants for sheep and adult human erythrocytes were 1.6 muM and 4.5 muM, respectively, whereas that of human cord blood erythrocytes was approximately 10-fold higher, 31 muM. The number of binding sites for sheep erythrocytes was calculated to be 7.2 x x 10(6) per cell, and that of human erythrocytes, 29 x 10(6) per cell. Binding was reversible. More than 50% of bound [(3)H]LTA was displaced from erythrocytes by a 50-fold excess of unlabeled LTA. LTA prepared from heterologous species of gram-positive bacteria were all inhibitory to the binding of [(3)H]LTA whether derived from S. pyogenes or from S. faecalis. Among a number of potential receptor analogues and other inhibitors tested, including serum albumin, gangliosides Gm(2) and Gm(3), lipopolysaccharide of gram-negative bacteria, and various sugars, only albumin and the gangliosides significantly inhibited LTA binding. Trypsin or neuraminidase treatment of erythrocytes had no effect on LTA binding. Deacylation of [(3)H]LTA abolished binding ability and binding was restored by esterification of the deacylated material with stearoyl chloride, indicating that ester-linked lipids are necessary for membrane binding.

摘要

已知革兰氏阳性菌的脂磷壁酸(LTA)能自发结合多种动物细胞膜。我们研究了化脓性链球菌和粪肠球菌的LTA与人及绵羊红细胞结合的生物学和生化特性。这些生物体中每种的放射性标记LTA([³H]LTA)与红细胞结合的动力学相似。绵羊和成人红细胞的解离常数分别为1.6 μM和4.5 μM,而人脐血红细胞的解离常数约高10倍,为31 μM。计算得出绵羊红细胞的结合位点数为每个细胞7.2×10⁶个,人红细胞的结合位点数为每个细胞29×10⁶个。结合是可逆的。50倍过量的未标记LTA可使红细胞中超过50%的结合[³H]LTA被置换出来。从革兰氏阳性菌的异源物种制备的LTA对[³H]LTA的结合均有抑制作用,无论该[³H]LTA源自化脓性链球菌还是粪肠球菌。在测试的许多潜在受体类似物和其他抑制剂中,包括血清白蛋白、神经节苷脂Gm₂和Gm₃、革兰氏阴性菌的脂多糖以及各种糖类,只有白蛋白和神经节苷脂能显著抑制LTA结合。用胰蛋白酶或神经氨酸酶处理红细胞对LTA结合无影响。[³H]LTA的脱酰作用消除了其结合能力,而用硬脂酰氯对脱酰材料进行酯化可恢复结合能力,这表明酯连接的脂质对于膜结合是必需的。

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