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人纤维胶凝蛋白的碳水化合物识别特性:糖芯片筛选揭示 M 型纤维胶凝蛋白的唾液酸结合特异性。

Carbohydrate recognition properties of human ficolins: glycan array screening reveals the sialic acid binding specificity of M-ficolin.

机构信息

Laboratoire d'Enzymologie Moléculaire, Institut de Biologie Structurale Jean-Pierre Ebel, Commissariat à l'Energie Atomique, CNRS UMR 5075, Université Joseph Fourier, 41 rue Jules Horowitz, Grenoble 38027 Cedex 1, France.

出版信息

J Biol Chem. 2010 Feb 26;285(9):6612-22. doi: 10.1074/jbc.M109.065854. Epub 2009 Dec 23.

Abstract

Ficolins are oligomeric innate immune recognition proteins consisting of a collagen-like region and a fibrinogen-like recognition domain that bind to pathogen- and apoptotic cell-associated molecular patterns. To investigate their carbohydrate binding specificities, serum-derived L-ficolin and recombinant H- and M-ficolins were fluorescently labeled, and their carbohydrate binding ability was analyzed by glycan array screening. L-ficolin preferentially recognized disulfated N-acetyllactosamine and tri- and tetrasaccharides containing terminal galactose or N-acetylglucosamine. Binding was sensitive to the position and orientation of the bond between N-acetyllactosamine and the adjacent carbohydrate. No significant binding of H-ficolin to any of the 377 glycans probed could be detected, providing further evidence for its poor lectin activity. M-ficolin bound preferentially to 9-O-acetylated 2-6-linked sialic acid derivatives and to various glycans containing sialic acid engaged in a 2-3 linkage. To further investigate the structural basis of sialic acid recognition by M-ficolin, point mutants were produced in which three residues of the fibrinogen domain were replaced by their counterparts in L-ficolin. Mutations G221F and A256V inhibited binding to the 9-O-acetylated sialic acid derivatives, whereas Y271F abolished interaction with all sialic acid-containing glycans. The crystal structure of the Y271F mutant fibrinogen domain was solved, showing that the mutation does not alter the structure of the ligand binding pocket. These analyses reveal novel ficolin ligands such as sulfated N-acetyllactosamine (L-ficolin) and gangliosides (M-ficolin) and provide precise insights into the sialic acid binding specificity of M-ficolin, emphasizing the essential role of Tyr(271) in this respect.

摘要

纤维胶凝蛋白是寡聚先天免疫识别蛋白,由胶原样区和纤维蛋白原样识别域组成,可与病原体和凋亡细胞相关的分子模式结合。为了研究它们的碳水化合物结合特异性,用荧光标记了血清来源的 L-纤维胶凝蛋白和重组 H-和 M-纤维胶凝蛋白,并通过聚糖阵列筛选分析了它们的碳水化合物结合能力。L-纤维胶凝蛋白优先识别双硫酸化 N-乙酰乳糖胺和含有末端半乳糖或 N-乙酰葡萄糖胺的三糖和四糖。结合对 N-乙酰乳糖胺与相邻碳水化合物之间键的位置和方向敏感。未检测到 H-纤维胶凝蛋白与探测到的 377 种糖中的任何一种的显著结合,这进一步证明了其较差的凝集素活性。M-纤维胶凝蛋白优先结合 9-O-乙酰化 2-6 连接的唾液酸衍生物和含有以 2-3 键结合的唾液酸的各种聚糖。为了进一步研究 M-纤维胶凝蛋白识别唾液酸的结构基础,在纤维蛋白原结构域中用 L-纤维胶凝蛋白的对应物替换了三个残基,产生了点突变体。突变 G221F 和 A256V 抑制与 9-O-乙酰化唾液酸衍生物的结合,而 Y271F 则使与所有含唾液酸的聚糖的相互作用丧失。Y271F 突变体纤维蛋白原结构域的晶体结构得到解决,表明突变不改变配体结合口袋的结构。这些分析揭示了新的纤维胶凝蛋白配体,如硫酸化 N-乙酰乳糖胺(L-纤维胶凝蛋白)和神经节苷脂(M-纤维胶凝蛋白),并提供了关于 M-纤维胶凝蛋白中唾液酸结合特异性的精确见解,强调了 Tyr(271)在这方面的重要作用。

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