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人类红细胞阴离子交换蛋白(AE1)即带3蛋白的克隆与特性分析

Cloning and characterization of band 3, the human erythrocyte anion-exchange protein (AE1).

作者信息

Lux S E, John K M, Kopito R R, Lodish H F

机构信息

Division of Hematology/Oncology, Children's Hospital, Boston, MA 02115.

出版信息

Proc Natl Acad Sci U S A. 1989 Dec;86(23):9089-93. doi: 10.1073/pnas.86.23.9089.

Abstract

The human erythrocyte anion-exchange protein (band 3 or AE1) was cloned from a fetal liver cDNA library. Three overlapping clones, encompassing 3637 nucleotides, were analyzed in detail. These encode a 911-amino acid protein (Mr 101,791) and detect a single 4.7-kilobase species in human reticulocyte RNA. The corresponding gene is located on chromosome 17. The protein is similar in structure to other anion exchangers and is divided into three regions: a hydrophilic, cytoplasmic domain that interacts with a variety of membrane and cytoplasmic proteins (residues 1-403); a hydrophobic, transmembrane domain that forms the anion antiporter (residues 404-882); and an acidic, C-terminal domain of unknown function (residues 883-911). The N-terminal domain contains several conserved sections (e.g., residues 57-86, 102-164, 219-347, and 375-403), some of which may contribute to binding sites for ankyrin, protein 4.1, or protein 4.2. The membrane domain is highly conserved with the exception of a single segment (residues 543-567) that contains several sites for cleavage of the protein by extracellular proteases. Based on hydropathy analyses and the wealth of available topographical and functional data, a model is proposed in which the protein crosses the membrane 14 times.

摘要

人红细胞阴离子交换蛋白(带3或AE1)是从胎儿肝脏cDNA文库中克隆出来的。对三个重叠克隆进行了详细分析,这些克隆包含3637个核苷酸。它们编码一个911个氨基酸的蛋白质(分子量101,791),并在人网织红细胞RNA中检测到一个单一的4.7千碱基的物种。相应的基因位于17号染色体上。该蛋白质在结构上与其他阴离子交换剂相似,分为三个区域:一个亲水的胞质结构域,与多种膜蛋白和胞质蛋白相互作用(第1 - 403位氨基酸);一个疏水的跨膜结构域,形成阴离子反向转运体(第404 - 882位氨基酸);以及一个功能未知的酸性C末端结构域(第883 - 911位氨基酸)。N末端结构域包含几个保守区域(例如,第57 - 86、102 - 164、219 - 347和375 - 403位氨基酸),其中一些可能有助于与锚蛋白、蛋白4.1或蛋白4.2的结合位点。除了一个单一的片段(第543 - 567位氨基酸)外,膜结构域高度保守,该片段包含几个细胞外蛋白酶切割该蛋白质 的位点。基于亲水性分析以及大量可用的拓扑学和功能数据,提出了一个该蛋白质跨膜14次的模型。

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