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由同基因大鼠单克隆抗体所定义的小鼠神经胶质瘤相关抗原的部分纯化及特性分析

Partial purification and characterization of a murine glioma-associated antigen defined by syngeneic rat monoclonal antibodies.

作者信息

Lee Y S, Matthews T J, Pizzo S, Abernethy J L, Bigner D D

出版信息

J Neuroimmunol. 1986 Dec;13(2):203-16. doi: 10.1016/0165-5728(86)90065-2.

Abstract

A glioma-associated antigen was previously identified on an avian sarcoma virus-induced F-344 rat astrocytoma cell line S69-c15 by four rat monoclonal antibodies (7G4, 9F1, 10E3 and 10E7) produced after syngeneic immunization. Earlier data suggested all four antibodies reacted with a polypeptide-associated epitope. We report here that the antigen activity was detected in the supernatant of tumor homogenates and could pass through a 1000 Da molecular weight cut-off dialysis membrane, as determined by antibody binding inhibition in a cell surface radioimmunoassay. When the dialysate was fractionated by Bio-Gel P-2 chromatography, antibody inhibiting activity eluted in the range of 300-600 Da. A highly purified material was further isolated by ion exchange high pressure liquid chromatography. Parallel purification product from an antigen-negative cell line failed to demonstrate antibody inhibiting activity. We conclude that greater than 400-fold purification enrichment of antigen can be achieved. We postulate that the partially purified antigenic determinant is a glioma-associated determinant of highly restricted expression and is presented in hapten-carrier form by the glioma cells.

摘要

先前通过同基因免疫产生的四种大鼠单克隆抗体(7G4、9F1、10E3和10E7)在禽肉瘤病毒诱导的F-344大鼠星形细胞瘤细胞系S69-c15上鉴定出一种胶质瘤相关抗原。早期数据表明,所有四种抗体均与一种多肽相关表位发生反应。我们在此报告,通过细胞表面放射免疫分析中的抗体结合抑制测定,在肿瘤匀浆的上清液中检测到了抗原活性,并且该抗原活性可以通过截留分子量为1000 Da的透析膜。当透析液通过Bio-Gel P-2柱色谱进行分级分离时,抗体抑制活性在300-600 Da范围内洗脱。通过离子交换高压液相色谱进一步分离得到了一种高度纯化的物质。来自抗原阴性细胞系的平行纯化产物未显示出抗体抑制活性。我们得出结论,抗原可实现超过400倍的纯化富集。我们推测,部分纯化的抗原决定簇是一种表达高度受限的胶质瘤相关决定簇,并且由胶质瘤细胞以半抗原-载体形式呈递。

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