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用单克隆抗体对癌胚抗原进行表位作图并建立一种新的改良放射免疫分析系统。

Epitope mapping of the carcinoembryonic antigen by monoclonal antibodies and establishment of a new improved radioimmunoassay system.

作者信息

Kuroki M, Arakawa F, Higuchi H, Matsunaga A, Okamoto N, Takakura K, Matsuoka Y

出版信息

Jpn J Cancer Res. 1987 Apr;78(4):386-96.

PMID:2438262
Abstract

A comprehensive mapping of epitopes on the carcinoembryonic antigen (CEA) molecule has been achieved by analyses of the specificities of 146 monoclonal antibodies (MAbs) from more than 300 hybridomas established recently. The reactivities of MAbs were analyzed by radioimmunoassays (RIA) with highly purified preparations of CEA and related antigens including normal fecal antigen-1 (NFA-1), NFA-2 in normal adult feces, nonspecific cross-reacting antigen (NCA) in lung and NCA-2 in meconium. The MAbs could be divided into five groups: group I, 23 clones directed to the NCA-common part of the CEA molecule; group II, 31 clones directed to the normal fecal cross-reacting antigen (NFCA)-common part; group III, 46 clones directed to the NFA-1-common part; group IV, 33 clones reactive with the heterogeneous carbohydrate part; and group V, 13 clones directed to the CEA-distinctive part which seemed to be highly specific for CEA. Mutual inhibitions of CEA binding between MAbs of the individual groups revealed that at least 25 different subgroups can be defined i.e., 4, 7, 8, 4, and 2 subgroups in groups I to V, respectively. The epitopes recognized by the group IV MAbs were found to be sensitive to oxidation with periodate, while the epitopes defined by MAbs of the other groups were resistant to this treatment. A solid-phase sandwich-type RIA system for CEA was established by using 2 MAbs from groups II and III as the CEA catcher and an MAb of group V as the tracer. This assay was shown to exhibit improved cancer-specificity and accuracy in the estimation of serum CEA levels.

摘要

通过对最近建立的300多个杂交瘤产生的146种单克隆抗体(MAb)的特异性进行分析,已实现对癌胚抗原(CEA)分子表位的全面定位。采用放射免疫分析(RIA),利用CEA及相关抗原的高度纯化制剂,包括正常粪便抗原-1(NFA-1)、正常成人粪便中的NFA-2、肺中的非特异性交叉反应抗原(NCA)和胎粪中的NCA-2,分析了MAb的反应性。这些MAb可分为五组:第一组,23个克隆针对CEA分子的NCA共同部分;第二组,31个克隆针对正常粪便交叉反应抗原(NFCA)共同部分;第三组,46个克隆针对NFA-1共同部分;第四组,33个克隆与异质性碳水化合物部分反应;第五组,13个克隆针对CEA独特部分,这部分似乎对CEA具有高度特异性。各单组MAb之间CEA结合的相互抑制作用表明,至少可定义25个不同的亚组,即第一至五组分别为4、7、8、4和2个亚组。发现第四组MAb识别的表位对高碘酸盐氧化敏感,而其他组MAb定义的表位对这种处理具有抗性。通过使用来自第二组和第三组的2种MAb作为CEA捕获剂,以及第五组的1种MAb作为示踪剂,建立了一种用于CEA的固相夹心型RIA系统。该检测方法在血清CEA水平估计中显示出提高的癌症特异性和准确性。

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