锌转运蛋白Dri 27/ZnT4在肠组织和细胞中的克隆、表达和水泡定位

C Murgia, I Vespignani, J Cerase, F Nobili, G Perozzi
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引用次数: 133

摘要

我们根据其在大鼠肠道发育过程中的上调表达,鉴定出了Dri 27 cDNA。它编码一个由430个氨基酸组成的疏水蛋白,与哺乳动物锌转运蛋白家族成员ZnT具有显著的同源性。Dri 27的小鼠同源物(命名为ZnT4)最近与小鼠突变“致死乳”有关。Dri 27/ZnT4的初级序列显示了多聚膜蛋白的特征。在本文中,我们发现Dri 27/ZnT4定位于胞内囊泡的膜上,其中大部分集中在极化肠细胞的基胞质区。在肠Caco-2细胞中短暂转染的Dri 27/ZnT4 myc标记构建物与转铁蛋白受体和网格蛋白接头复合物AP-1和AP-2的β亚基部分共定位在一个内体囊泡亚群中。通过亚克隆不同部分的蛋白与谷胱甘肽- s转移酶的框架,我们也提供了实验证据,他们的功能作为锌结合和蛋白-蛋白相互作用域。
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Cloning, expression, and vesicular localization of zinc transporter Dri 27/ZnT4 in intestinal tissue and cells.

We have identified the Dri 27 cDNA on the basis of its upregulated expression during rat intestinal development. It encodes a hydrophobic protein of 430 amino acids that shares significant homology with members of the mammalian zinc transporter family ZnT. The murine homologue of Dri 27 (named ZnT4) was recently associated with the mouse mutation "lethal milk." The primary sequence of Dri 27/ZnT4 displays features characteristic of polytopic membrane proteins. In this paper, we show that Dri 27/ZnT4 is localized in the membrane of intracellular vesicles, the majority of which concentrate in the basal cytoplasmic region of polarized enterocytes. A Dri 27/ZnT4 myc-tagged construct, transiently transfected in intestinal Caco-2 cells, partially colocalizes with the transferrin receptor and with the beta-subunits of the clathrin adaptor complexes AP-1 and AP-2 in a subpopulation of endosomal vesicles. By subcloning distinct portions of the protein in frame with glutathione-S-transferase, we also provide experimental evidence of their function as zinc-binding and protein-protein-interaction domains.

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