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人红细胞带3跨膜结构域的N端区域。对膜插入和转运活性至关重要的残基。

The N-terminal region of the transmembrane domain of human erythrocyte band 3. Residues critical for membrane insertion and transport activity.

作者信息

Kanki Tomotake, Young Mark T, Sakaguchi Masao, Hamasaki Naotaka, Tanner Michael J A

机构信息

Department of Clinical Chemistry and Laboratory Medicine, Graduate School of Medical Sciences, Kyushu University, Fukuoka 812-8582, Japan.

出版信息

J Biol Chem. 2003 Feb 21;278(8):5564-73. doi: 10.1074/jbc.M211662200. Epub 2002 Dec 12.

DOI:10.1074/jbc.M211662200
PMID:12482865
Abstract

We studied the role of the N-terminal region of the transmembrane domain of the human erythrocyte anion exchanger (band 3; residues 361-408) in the insertion, folding, and assembly of the first transmembrane span (TM1) to give rise to a transport-active molecule. We focused on the sequence around the 9-amino acid region deleted in Southeast Asian ovalocytosis (Ala-400 to Ala-408), which gives rise to nonfunctional band 3, and also on the portion of the protein N-terminal to the transmembrane domain (amino acids 361-396). We examined the effects of mutations in these regions on endoplasmic reticulum insertion (using cell-free translation), chloride transport, and cell-surface movement in Xenopus oocytes. We found that the hydrophobic length of TM1 was critical for membrane insertion and that formation of a transport-active structure also depended on the presence of specific amino acid sequences in TM1. Deletions of 2 or 3 amino acids including Pro-403 retained transport activity provided that a polar residue was located 2 or 3 amino acids on the C-terminal side of Asp-399. Finally, deletion of the cytoplasmic surface sequence G(381)LVRD abolished chloride transport, but not surface expression, indicating that this sequence makes an essential structural contribution to the anion transport site of band 3.

摘要

我们研究了人类红细胞阴离子交换蛋白(带3;第361 - 408位氨基酸残基)跨膜结构域N端区域在首个跨膜片段(TM1)的插入、折叠和组装过程中所起的作用,该过程会产生一个具有转运活性的分子。我们重点关注了东南亚椭圆形红细胞增多症中缺失的9个氨基酸区域(丙氨酸 - 400至丙氨酸 - 408)周围的序列,该区域会导致无功能的带3产生,同时也关注了跨膜结构域N端的蛋白质部分(第361 - 396位氨基酸)。我们研究了这些区域的突变对非洲爪蟾卵母细胞内质网插入(使用无细胞翻译)、氯离子转运和细胞表面移动的影响。我们发现TM1的疏水长度对于膜插入至关重要,并且具有转运活性结构的形成还取决于TM1中特定氨基酸序列的存在。只要在天冬氨酸 - 399的C端一侧2或3个氨基酸位置上有一个极性残基,缺失包括脯氨酸 - 403在内的2或3个氨基酸仍能保留转运活性。最后,缺失胞质表面序列G(381)LVRD会消除氯离子转运,但不会影响表面表达,这表明该序列对带3的阴离子转运位点做出了重要的结构贡献。

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