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锚蛋白促进极化细胞中α1 - 钠钾 - ATP酶的细胞内运输。

Ankyrin facilitates intracellular trafficking of alpha1-Na+-K+-ATPase in polarized cells.

作者信息

Stabach Paul R, Devarajan Prasad, Stankewich Michael C, Bannykh Serguei, Morrow Jon S

机构信息

Dept. of Pathology, Yale Univ., 310 Cedar St., New Haven, CT 06520, USA.

出版信息

Am J Physiol Cell Physiol. 2008 Nov;295(5):C1202-14. doi: 10.1152/ajpcell.00273.2008. Epub 2008 Sep 3.

Abstract

Defects in ankyrin underlie many hereditary disorders involving the mislocalization of membrane proteins. Such phenotypes are usually attributed to ankyrin's role in stabilizing a plasma membrane scaffold, but this assumption may not be accurate. We found in Madin-Darby canine kidney cells and in other cultured cells that the 25-residue ankyrin-binding sequence of alpha(1)-Na(+)-K(+)-ATPase facilitates the entry of alpha(1),beta(1)-Na(+)-K(+)-ATPase into the secretory pathway and that replacement of the cytoplasmic domain of vesicular stomatitis virus G protein (VSV-G) with this ankyrin-binding sequence bestows ankyrin dependency on the endoplasmic reticulum (ER) to Golgi trafficking of VSV-G. Expression of the ankyrin-binding sequence of alpha(1)-Na(+)-K(+)-ATPase alone as a soluble cytosolic peptide acts in trans to selectively block ER to Golgi transport of both wild-type alpha(1)-Na(+)-K(+)-ATPase and a VSV-G fusion protein that includes the ankyrin-binding sequence, whereas the trafficking of other proteins remains unaffected. Similar phenotypes are also generated by small hairpin RNA-mediated knockdown of ankyrin R or the depletion of ankyrin in semipermeabilized cells. These data indicate that the adapter protein ankyrin acts not only at the plasma membrane but also early in the secretory pathway to facilitate the intracellular trafficking of alpha(1)-Na(+)-K(+)-ATPase and presumably other selected proteins. This novel ankyrin-dependent assembly pathway suggests a mechanism whereby hereditary disorders of ankyrin may be manifested as diseases of membrane protein ER retention or mislocalization.

摘要

锚蛋白缺陷是许多涉及膜蛋白定位错误的遗传性疾病的基础。此类表型通常归因于锚蛋白在稳定质膜支架中的作用,但这一假设可能并不准确。我们在犬肾Madin-Darby细胞和其他培养细胞中发现,α(1)-钠钾-ATP酶的25个氨基酸残基的锚蛋白结合序列促进了α(1),β(1)-钠钾-ATP酶进入分泌途径,并且用该锚蛋白结合序列替换水泡性口炎病毒G蛋白(VSV-G)的胞质结构域赋予了VSV-G从内质网(ER)到高尔基体运输的锚蛋白依赖性。单独作为可溶性胞质肽表达的α(1)-钠钾-ATP酶锚蛋白结合序列可反式作用,选择性地阻断野生型α(1)-钠钾-ATP酶和包含该锚蛋白结合序列的VSV-G融合蛋白从内质网到高尔基体的运输,而其他蛋白的运输则不受影响。小发夹RNA介导的锚蛋白R敲低或半透性细胞中锚蛋白的耗尽也会产生类似的表型。这些数据表明,衔接蛋白锚蛋白不仅在质膜起作用,还在分泌途径早期发挥作用,以促进α(1)-钠钾-ATP酶以及可能其他特定蛋白的细胞内运输。这种新的依赖锚蛋白的组装途径提示了一种机制,据此锚蛋白的遗传性疾病可能表现为膜蛋白在内质网滞留或定位错误的疾病。

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