首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Detection of unique antigenic determinants on human plasma low density lipoprotein and on delipidated apolipoprotein B.
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Detection of unique antigenic determinants on human plasma low density lipoprotein and on delipidated apolipoprotein B.

机译:检测人血浆低密度脂蛋白和脱脂载脂蛋白B上独特的抗原决定簇。

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摘要

To obtain detailed information on the role played by apolipoprotein B (apo B) in determining the structural and functional properties of human plasma low density lipoprotein, we have initiated immunochemical studies of the polypeptide. We report here the establishment of six hybridoma lines that secrete monoclonal antibodies to low density lipoprotein. In addition to recognizing antigenic determinants on low density lipoprotein, all six monoclonal antibodies react with epitope(s) on very low density, but not high density, lipoproteins. The immunoreactivity of these antibodies with low density lipoprotein and with detergent-delipidated apo B was compared in an enzyme-linked immunosorbent assay. Although all six of the antibodies reacted with the apoprotein when it was prepared in a nonionic detergent known to maintain the secondary structure of the protein, three of the six antibodies showed partial or total loss of activity with NaDodSO4- delipidated apo B. The specificity of these antibodies was tested by the ability of affinity-purified biotinylated antibodies to compete with unlabeled antibodies for antigenic sites on low density lipoprotein in a competition enzyme-linked immunosorbent assay developed with avidin-peroxidase. This competition assay allowed us to divide the antibodies into a minimum of two groups (I and II) based on the antigenic determinants on apo B that they recognized. The epitope on apo B recognized by group II antibodies was perturbed in NaDodSO4, whereas the determinant(s) on the protein reactive with group I antibodies was unaffected.
机译:为了获得有关载脂蛋白B(apo B)在确定人血浆低密度脂蛋白的结构和功能特性中所起的作用的详细信息,我们已开始对该多肽进行免疫化学研究。我们在这里报告建立了六种杂交瘤细胞系,它们分泌针对低密度脂蛋白的单克隆抗体。除了识别低密度脂蛋白上的抗原决定簇外,所有六种单克隆抗体都以极低密度而不是高密度脂蛋白与抗原决定簇反应。在酶联免疫吸附试验中比较了这些抗体与低密度脂蛋白和去污剂脱脂载脂蛋白B的免疫反应性。尽管在已知可维持蛋白质二级结构的非离子去污剂中制备载脂蛋白时,所有六种抗体均与脱辅基蛋白反应,但六种抗体中的三种与NaDodSO4-脱脂的载脂蛋白B表现出部分或全部丧失活性。在亲和素过氧化物酶开发的竞争酶联免疫吸附试验中,通过亲和纯化的生物素化抗体与未标记抗体竞争低密度脂蛋白上抗原位点的能力来测试这些抗体。通过竞争分析,我们可以根据抗体识别的载脂蛋白B上的抗原决定簇将抗体分为至少两组(I和II)。被II组抗体识别的apo B上的表位在NaDodSO4中受到干扰,而与I组抗体反应的蛋白质上的决定簇则不受影响。

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