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Structure of the anion-transport protein of the human erythrocyte membrane. Further studies on the fragments produced by proteolytic digestion

机译:人红细胞膜的阴离子转运蛋白的结构。对蛋白水解消化产生的片段的进一步研究

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pThe topology of the human erythrocyte membrane anion-transport protein (band 3) has been investigated by isolation and peptide ‘mapping’ of the major and minor fragments derived from proteolytic cleavage of the lactoperoxidase 125I-labelled protein in erythrocytes and erythrocyte membranes. The content, in each fragment, of lactoperoxidase 125I-labelled sites (which have a known location in the extracellular or cytoplasmic domain of the protein), together with the location of the sites of proteolytic cleavage yielding the fragments, has allowed us to determine the alignment of the fragments on the linear amino acid sequence and to infer the topology of the polypeptide in the membrane. The results suggest that a region in the C-terminal portion of the polypeptide forms part of the cytoplasmic domain of the protein in addition to a large N-terminal segment. The membrane-bound regions of the protein are located in the C-terminal two-thirds of the molecule. In this region the polypeptide chain traverses the membrane at least four times and an additional loop of polypeptide is either embedded in the membrane or also penetrates through it to the other surface. The location of the lectin receptors on the protein and the site of binding of an anion-transport inhibitor have also been studied./p
机译:通过分离和乳化过氧化物酶125I标记的蛋白质在红细胞和红细胞膜中的蛋白水解裂解衍生的主要和次要片段,对人红细胞膜阴离子转运蛋白(带3)的拓扑结构进行了研究。 。乳过氧化物酶125I标记位点(在蛋白质的胞外或细胞质结构域中具有已知位置)的每个片段中的含量,以及产生该片段的蛋白水解切割位点的位置,使我们能够确定在线性氨基酸序列上对片段进行比对并推断膜中多肽的拓扑。结果表明,除了大的N-末端区段之外,多肽的C-末端部分中的区域形成蛋白质的胞质结构域的一部分。蛋白质的膜结合区位于分子的C末端的三分之二处。在该区域中,多肽链至少穿过膜四次,并且多肽的另一环嵌入膜中或穿透膜到达另一表面。还研究了凝集素受体在蛋白质上的位置以及阴离子转运抑制剂的结合位点。

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