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针对盘基网柄菌肌动蛋白制备的单克隆抗体:特性及与肌动蛋白的相互作用

Monoclonal antibodies prepared against Dictyostelium actin: characterization and interactions with actin.

作者信息

Simpson P A, Spudich J A, Parham P

出版信息

J Cell Biol. 1984 Jul;99(1 Pt 1):287-95. doi: 10.1083/jcb.99.1.287.

DOI:10.1083/jcb.99.1.287
PMID:6203918
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2275643/
Abstract

Three mouse monoclonal antibodies, Act I, Act II, and Act IV, against actin from the cellular slime mold Dictyostelium discoideum, have been made and characterized. All three antibodies are IgG1 and share the following properties: They form stable complexes with monomeric Dictyostelium actin, which prevents polymerization of the actin into filaments. On addition to preformed actin filaments, they cause a reduction in filament size and in the viscosity of the actin solution. They cross-react strongly with actins from the lower eucaryotes Physarum and Acanthamoeba, but not with alpha-actins from rabbit and human muscle or beta- and gamma-actins from human erythrocytes and a human B lymphoid cell line. Act II and Act IV recognize a similar antigenic determinant that is topographically distinct from that identified by Act I. In protein immunoblotting, only Act I bound strongly to Dictyostelium actin. Analysis of actin fragments with this technique showed that amino acids 13 to about 50 are required for Act I binding to actin. A comparison of the amino acid sequences of actins from lower eucaryotes and higher vertebrates implicates threonine 41 as a critical residue in the Act I antigenic site. The properties of Act II and Act IV suggest that they recognize antigenic sites involving the NH2-terminal six residues.

摘要

已制备并鉴定了三种针对细胞黏菌盘基网柄菌肌动蛋白的小鼠单克隆抗体,即Act I、Act II和Act IV。这三种抗体均为IgG1,具有以下共同特性:它们与单体盘基网柄菌肌动蛋白形成稳定复合物,从而阻止肌动蛋白聚合成丝。将其添加到预先形成的肌动蛋白丝中时,它们会导致丝的尺寸减小以及肌动蛋白溶液的粘度降低。它们与低等真核生物绒泡菌和棘阿米巴的肌动蛋白发生强烈交叉反应,但不与兔和人肌肉中的α-肌动蛋白或人红细胞及人B淋巴细胞系中的β-和γ-肌动蛋白发生交叉反应。Act II和Act IV识别相似的抗原决定簇,其拓扑结构与Act I所识别的不同。在蛋白质免疫印迹中,只有Act I与盘基网柄菌肌动蛋白强烈结合。用该技术对肌动蛋白片段进行分析表明,Act I与肌动蛋白结合需要氨基酸13至约50。对低等真核生物和高等脊椎动物肌动蛋白氨基酸序列的比较表明,苏氨酸41是Act I抗原位点中的关键残基。Act II和Act IV的特性表明它们识别涉及氨基末端六个残基的抗原位点。

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