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用合成糖脂加载抗原呈递蛋白CD1d。

Loading of the antigen-presenting protein CD1d with synthetic glycolipids.

作者信息

Wallner Fredrik K, Chen Liying, Moliner Annalena, Jondal Mikael, Elofsson Mikael

机构信息

Organic Chemistry, Department of Chemistry, Umeå University, 90187 Umeå, Sweden.

出版信息

Chembiochem. 2004 Apr 2;5(4):437-44. doi: 10.1002/cbic.200300655.

Abstract

CD1 proteins present mammalian and microbial lipid and glycolipid antigens to different subsets of T cells. Few such antigens have been identified and the binding of these to CD1 molecules has mainly been studied by using responding T cells in cellular assays or recombinant solid-phase CD1 proteins. In the present study we use four different glycolipids, some of which contain tumor-associated carbohydrate antigens, to develop a procedure to easily detect binding of glycolipids to CD1 proteins on viable cells. Two of these glycolipids are novel glycoconjugates containing alpha-D-N-acetylgalactosamine (alpha-GalNAc) that were prepared by a combined solution and solid-phase approach. The key step, a Fischer glycosylation of 9-fluorenylmethoxycarbonylaminoethanol with GalNAc, furnished the alpha-glycoside 4 in 34% yield. Cells were incubated with glycolipids and stained with monoclonal antibodies specific for the carbohydrate part. The level of glycolipid bound to cells was then determined by flow cytometry with a secondary antibody labeled with fluorescein isothiocyanate. All four glycolipids were found to bind to CD1d but with different selectivity. The loading was dose dependent and could be inhibited by an established CD1d ligand, alpha-galactosylceramide. Through use of this procedure, glycolipids were selectively loaded onto CD1d expressed on professional antigen-presenting cells for future use as cellular vaccines. Moreover, the glycolipids described in this study represent novel CD1d-binding ligands that will be useful derivatives in the study of CD1d-dependent immune responses, for example, against tumors.

摘要

CD1蛋白将哺乳动物和微生物的脂质及糖脂抗原呈递给不同亚群的T细胞。已鉴定出的此类抗原较少,并且这些抗原与CD1分子的结合主要是通过在细胞检测中使用反应性T细胞或重组固相CD1蛋白来研究的。在本研究中,我们使用四种不同的糖脂,其中一些含有肿瘤相关碳水化合物抗原,来开发一种易于检测糖脂与活细胞上CD1蛋白结合的方法。其中两种糖脂是含有α-D-N-乙酰半乳糖胺(α-GalNAc)的新型糖缀合物,它们是通过溶液和固相相结合的方法制备的。关键步骤是9-芴甲氧羰基氨基乙醇与GalNAc的费歇尔糖基化反应,以34%的产率得到α-糖苷4。将细胞与糖脂一起孵育,并用对碳水化合物部分具有特异性的单克隆抗体进行染色。然后通过用异硫氰酸荧光素标记的二抗进行流式细胞术测定与细胞结合的糖脂水平。发现所有四种糖脂均与CD1d结合,但具有不同的选择性。负载呈剂量依赖性,并且可以被已确定的CD1d配体α-半乳糖基神经酰胺抑制。通过使用该方法,糖脂被选择性地负载到专业抗原呈递细胞上表达的CD1d上,以供将来用作细胞疫苗。此外,本研究中描述的糖脂代表了新型的CD1d结合配体,它们将是研究CD1d依赖性免疫反应(例如针对肿瘤的免疫反应)中有用的衍生物。

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