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一种具有钙调蛋白结合活性的新型红细胞膜相关蛋白。鉴定与纯化。

A new erythrocyte membrane-associated protein with calmodulin binding activity. Identification and purification.

作者信息

Gardner K, Bennett V

出版信息

J Biol Chem. 1986 Jan 25;261(3):1339-48.

PMID:3511042
Abstract

A new protein that binds calmodulin has been identified and purified to greater than 95% homogeneity from the Triton X-100-insoluble residue of human erythrocyte ghost membranes (cytoskeletons) by DEAE chromatography and preparative rate zonal sucrose gradient sedimentation. This ghost calmodulin-binding protein is an alpha/beta heterodimer with subunits of Mr = 103,000 (alpha) and 97,000 (beta). The protein exhibits a Stokes radius of 6.9 nm and a sedimentation coefficient of 6.8 S, corresponding to a molecular weight of 197,000. Moreover, the protein is cross-linked by Cu2+/phenanthroline to a dimer of Mr = 200,000. The Mr = 97,000 beta subunit was identified as the calmodulin-binding site by photoaffinity labeling with 125I-azidocalmodulin. A 230 nM affinity for calmodulin was estimated by displacement of two different concentrations of the 125I-azidocalmodulin with unmodified calmodulin and subsequent Dixon plot analysis. This calmodulin-binding protein is present in erythrocytes at 30,000 copies/cell and is associated exclusively with the membrane. It is tightly bound to a site on red cell cytoskeletons and is totally solubilized in the low ionic strength extract derived from red cell ghost membranes. Visualization of this calmodulin-binding protein in the electron microscope by rotary shadowing, negative staining, and unidirectional shadowing indicates that it is a flattened circular molecule with a 12.4-nm diameter and a 5.4-nm height. Affinity-purified antibodies against the calmodulin-binding protein identify a cross-reacting Mr = 100,000 polypeptide(s) in brain membranes.

摘要

一种与钙调蛋白结合的新蛋白质已从人红细胞血影膜(细胞骨架)的Triton X - 100不溶性残渣中,通过DEAE柱层析和制备性速率区带蔗糖梯度沉降法被鉴定并纯化至均一性大于95%。这种血影钙调蛋白结合蛋白是一种α/β异二聚体,其亚基的分子量分别为103,000(α)和97,000(β)。该蛋白质的斯托克斯半径为6.9纳米,沉降系数为6.8 S,对应分子量为197,000。此外,该蛋白质通过铜离子/邻菲罗啉交联形成分子量为200,000的二聚体。通过用125I - 叠氮钙调蛋白进行光亲和标记,确定分子量为97,000的β亚基为钙调蛋白结合位点。通过用未修饰的钙调蛋白取代两种不同浓度的125I - 叠氮钙调蛋白并随后进行狄克逊图分析,估计其对钙调蛋白的亲和力为230 nM。这种钙调蛋白结合蛋白在红细胞中的含量为每个细胞30,000个拷贝,并且仅与膜相关。它紧密结合于红细胞细胞骨架上的一个位点,并且在源自红细胞血影膜的低离子强度提取物中完全溶解。通过旋转投影、负染色和单向投影在电子显微镜下观察这种钙调蛋白结合蛋白,表明它是一种扁平的圆形分子,直径为12.4纳米,高度为5.4纳米。针对钙调蛋白结合蛋白的亲和纯化抗体在脑膜中鉴定出一种分子量为100,000的交叉反应多肽。

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