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人血清中钙离子依赖性F-肌动蛋白解聚蛋白的进一步特性研究。

Further characterization of the Ca2+-dependent F-actin-depolymerizing protein of human serum.

作者信息

Thorstensson R, Utter G, Norberg R

出版信息

Eur J Biochem. 1982 Aug;126(1):11-6. doi: 10.1111/j.1432-1033.1982.tb06738.x.

Abstract

The F-actin-depolymerizing factor (ADF) of human serum was purified and identified as a 93000-daltons protein. The concentration of ADF was calculated to 120-150 micrograms/ml in four normal sera and about half as much in three sera from leukemia patients treated with cytostatic drugs. In the presence of Ca2+ ADF shortened actin filaments into fragments, the size of which was correlated to the actin: ADF molar ratio, as judged by electron microscopy. The severing of F-actin was not necessarily followed by an increase in the quantities of monomeric actin, as determined by a DNase I inhibition assay and a sedimentation assay. The findings indicated that ADF shortens filamentous actin by breaking bonds between adjacent actin molecules thereby forming stable ADF-actin complexes, without a monomeric net release. The effect of ADF on F-actin was rapid and was reversed upon chelation of Ca2+. ADF cross-reacted immunologically and exhibited similarity in reaction mechanism with gelsolin, the Ca2+-dependent F-actin-severing protein from macrophages. This implies that the proteins are both structurally and functionally related. The physiological role of ADF may be to handle actin released at cell destruction, probably by forming ADF-G-actin 1:1 complexes thereby preventing formation of actin filaments.

摘要

人血清中的F-肌动蛋白解聚因子(ADF)被纯化并鉴定为一种93000道尔顿的蛋白质。在四份正常血清中,ADF的浓度经计算为120 - 150微克/毫升,而在接受细胞抑制药物治疗的白血病患者的三份血清中,其浓度约为正常血清的一半。在钙离子存在的情况下,ADF将肌动蛋白丝缩短成片段,通过电子显微镜判断,片段大小与肌动蛋白:ADF摩尔比相关。通过脱氧核糖核酸酶I抑制试验和沉降试验确定,F-肌动蛋白的切断并不一定会导致单体肌动蛋白数量的增加。研究结果表明,ADF通过断裂相邻肌动蛋白分子之间的键来缩短丝状肌动蛋白,从而形成稳定的ADF-肌动蛋白复合物,而不会有单体的净释放。ADF对F-肌动蛋白的作用迅速,并且在钙离子螯合后作用逆转。ADF在免疫反应上有交叉反应,并且在反应机制上与凝溶胶蛋白相似,凝溶胶蛋白是巨噬细胞中依赖钙离子的F-肌动蛋白切断蛋白。这意味着这两种蛋白质在结构和功能上都相关。ADF的生理作用可能是处理细胞破坏时释放的肌动蛋白,可能是通过形成ADF - G -肌动蛋白1:1复合物,从而防止肌动蛋白丝的形成。

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