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针对人类B淋巴细胞标志物CD24的单克隆抗体BA-1识别肽上多价展示的唾液酸(N-乙酰神经氨酸)依赖性表位。

Monoclonal antibody BA-1 to the human B lymphocyte marker CD24 recognizes a sialic acid (N-acetylneuraminic acid) dependent epitope in multi-valent display on peptide.

作者信息

Mehmet H, Larkin M, Tang P W, Lebien T W, Feizi T

机构信息

Glycoconjugates Section, MRC Clinical Research Centre, Harrow, Middlesex, UK.

出版信息

Clin Exp Immunol. 1990 Sep;81(3):489-95. doi: 10.1111/j.1365-2249.1990.tb05361.x.

Abstract

Evidence is presented that monoclonal antibody BA-1, directed against a marker (CD24) of human lymphocytes of B cell lineage, recognizes a sialic acid-dependent epitope. This conclusion is based on a series of experiments exploiting the reaction of this antibody with bovine and ovine submaxillary mucins. Expression of the epitope was enhanced following alkaline saponification of bovine submaxillary mucin, which converts O-acetylated neuraminic acid residues to N-acetylneuraminic acid. The epitope was destroyed following neuraminidase or mild acid treatment of the mucins, and its expression was diminished following neuraminidase treatment of B lymphoblastoid cells. Glycopeptides obtained by digestion of the bovine mucin with papain, trypsin or pronase were lacking in antigenicity. However, antigenic activity could be regenerated after conjugation of pronase glycopeptides to poly-L-lysine. These results indicate that multivalent display of sialo-oligosaccharide on peptide rather than a protease-susceptible polypeptide domain is required for BA-1 antibody binding.

摘要

有证据表明,针对B细胞系人淋巴细胞标志物(CD24)的单克隆抗体BA-1识别一种唾液酸依赖性表位。这一结论基于一系列利用该抗体与牛和羊下颌下粘蛋白反应的实验。牛下颌下粘蛋白经碱性皂化后,表位的表达增强,碱性皂化可将O-乙酰化神经氨酸残基转化为N-乙酰神经氨酸。粘蛋白经神经氨酸酶或弱酸处理后,表位被破坏,经神经氨酸酶处理的B淋巴母细胞中表位表达降低。用木瓜蛋白酶、胰蛋白酶或链霉蛋白酶消化牛粘蛋白得到的糖肽缺乏抗原性。然而,链霉蛋白酶糖肽与聚-L-赖氨酸结合后可恢复抗原活性。这些结果表明,BA-1抗体结合需要唾液酸寡糖在肽上的多价展示,而不是蛋白酶敏感的多肽结构域。

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