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使用猪纤维蛋白原作为模型糖蛋白来研究K88凝集素三种变体的结合特异性。

Use of porcine fibrinogen as a model glycoprotein to study the binding specificity of the three variants of K88 lectin.

作者信息

L'Hôte C, Berger S, Bourgerie S, Duval-Iflah Y, Julien R, Karamanos Y

机构信息

Institut de Biotechnologie, Université de Limoges, France.

出版信息

Infect Immun. 1995 May;63(5):1927-32. doi: 10.1128/iai.63.5.1927-1932.1995.

Abstract

Known glycoproteins were used to determine the differences occurring in the binding specificities of the three variants of the K88 lectin in an approach essentially based on lectin blotting. During the screening, it was demonstrated that each variant of the K88 lectin biotinylated via its amino groups (NbioK88) exhibited a characteristic binding to the three chains of porcine fibrinogen. NbioK88ab weakly bound to A alpha chains, NbioK88ac bound to B beta and gamma chains, and NbioK88ad bound only to the gamma chain. To validate this model, the oligosaccharide moieties of porcine fibrinogen were analyzed with glycosidases and by lectin blotting and sugar composition. Both the B beta chain and gamma chain carry biantennary N-glycans of the N-acetyllactosamine type that are not recognized by K88 lectins. A alpha chains are substituted by sialylated T antigen. O-glycans were also detected on B beta and gamma chains of porcine fibrinogen and contribute to the recognition of these chains by K88ac and K88ad fimbriae.

摘要

已知糖蛋白被用于确定K88凝集素三种变体在结合特异性上的差异,该方法主要基于凝集素印迹法。在筛选过程中,结果表明,通过其氨基生物素化的K88凝集素的每种变体(NbioK88)对猪纤维蛋白原的三条链都表现出特异性结合。NbioK88ab与Aα链弱结合,NbioK88ac与Bβ链和γ链结合,而NbioK88ad仅与γ链结合。为验证该模型,用糖苷酶、凝集素印迹法和糖组成分析了猪纤维蛋白原的寡糖部分。Bβ链和γ链都带有N-乙酰乳糖胺类型的双天线N-聚糖,而K88凝集素无法识别这些聚糖。Aα链被唾液酸化T抗原取代。在猪纤维蛋白原的Bβ链和γ链上也检测到了O-聚糖,它们有助于K88ac和K88ad菌毛对这些链的识别。

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