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编码M1/69-J11d热稳定抗原的cDNA的表达克隆

Expression cloning of a cDNA encoding M1/69-J11d heat-stable antigens.

作者信息

Kay R, Takei F, Humphries R K

机构信息

Terry Fox Laboratory, B.C. Cancer Research Centre, Vancouver, Canada.

出版信息

J Immunol. 1990 Sep 15;145(6):1952-9.

PMID:2118158
Abstract

The differentiation Ag identified by the mAb M1/69 and J11d (commonly referred to as heat-stable Ag) are found in structurally heterogeneous forms on the surfaces of many types of murine hemopoietic cells. The extinction of expression of these antigens is associated with thymocyte maturation and Ig class switching in B cells, as well as terminal differentiation of macrophages. A cDNA encoding the M1/69-J11d peptide was cloned from a hemopoietic progenitor cell line by immunoselection of COS cells transfected with expression libraries. The cloned cDNA is a copy of a gene that is transcribed in M1/69-J11d+ lymphoid, myeloid, and erythroid cells. This gene could be responsible for the expression of all forms of the M1/69-J11d Ag, although there are homologous genes that may encode some forms of the Ag that are specifically expressed in bone marrow. The cloned cDNA encodes a surprisingly small peptide, predicted to contain only 30 amino acids after removal of a signal sequence and displacement of the C-terminal region by the glycosyl-phosphatidylinositol group that anchors the peptide to the cell surface. Almost all of the mass of the M1/69-J11d Ag accumulates through extensive N- and O-linked glycosylation at multiple sites in the short peptide. These carbohydrates are likely to execute the functions of M1/69-J11d Ag, which could be specialized to each cell type as a consequence of differential glycosylation.

摘要

单克隆抗体M1/69和J11d识别的分化抗原(通常称为热稳定抗原)以结构异质的形式存在于多种小鼠造血细胞表面。这些抗原表达的消失与胸腺细胞成熟、B细胞中的免疫球蛋白类别转换以及巨噬细胞的终末分化有关。通过对用表达文库转染的COS细胞进行免疫筛选,从造血祖细胞系中克隆出编码M1/69-J11d肽的cDNA。克隆的cDNA是一个在M1/69-J11d阳性的淋巴细胞、髓细胞和红细胞中转录的基因的拷贝。该基因可能负责所有形式的M1/69-J11d抗原的表达,尽管存在同源基因可能编码某些在骨髓中特异性表达的抗原形式。克隆的cDNA编码一个惊人的小肽,预测去除信号序列并通过将肽锚定到细胞表面的糖基磷脂酰肌醇基团置换C末端区域后仅含有30个氨基酸。M1/69-J11d抗原的几乎所有质量都是通过短肽中多个位点的广泛N-和O-连接糖基化积累的。这些碳水化合物可能执行M1/69-J11d抗原的功能,由于糖基化差异,其功能可能因细胞类型而异。

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