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首页> 外文期刊>Journal of Molecular Biology >Oligomerization of the UapA Purine Transporter Is Critical for ER-Exit, Plasma Membrane Localization and Turnover
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Oligomerization of the UapA Purine Transporter Is Critical for ER-Exit, Plasma Membrane Localization and Turnover

机译:UapA嘌呤转运蛋白的低聚化对于ER出口,血浆膜定位和周转至关重要

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摘要

Central to the process of transmembrane cargo trafficking is the successful folding and exit from the ER (endoplasmic reticulum) through packaging in COPII vesicles. Here, we use the UapA purine transporter of Aspergillus nidulans to investigate the role of cargo oligomerization in membrane trafficking. We show that UapA oligomerizes (at least dimerizes) and that oligomerization persists upon UapA endocytosis and vacuolar sorting. Using a validated bimolecular fluorescence complementation assay, we provide evidence that a UapA oligomerization is associated with ER-exit and turnover, as ER-retained mutants due to either modification of a Tyr-based N-terminal motif or partial misfolding physically associate but do not associate properly. Co-expression of ER-retained mutants with wild-type UapA leads to in trans plasma membrane localization of the former, confirming that oligomerization initiates in the ER. Genetic suppression of an N-terminal mutation in the Tyr motif and mutational analysis suggest that transmembrane a-helix 7 affects the oligomerization interface. Our results reveal that transporter oligomerization is essential for membrane trafficking and turnover and is a common theme in fungi and mammalian cells. (C) 2015 Elsevier Ltd. All rights reserved.
机译:跨膜货物运输过程的核心是通过将其包装在COPII囊泡中而成功折叠并从ER(内质网)中退出。在这里,我们使用构巢曲霉的UapA嘌呤转运蛋白来研究货物低聚在膜运输中的作用。我们显示UapA寡聚(至少二聚化),并且在UapA内吞作用和液泡排序后,寡聚持续存在。使用经过验证的双分子荧光互补测定,我们提供证据表明UapA寡聚化与ER出口和营业额相关,因为ER保留的突变体由于基于Tyr的N端基序的修饰或部分错折叠而物理缔合,但没有正确地关联。 ER保留的突变体与野生型UapA的共表达导致前者在跨质膜中定位,这证实了寡聚在ER中启动。 Tyr基序中N末端突变的遗传抑制和突变分析表明跨膜a-螺旋7影响寡聚化界面。我们的结果表明转运蛋白低聚对于膜运输和更新至关重要,并且是真菌和哺乳动物细胞的共同主题。 (C)2015 Elsevier Ltd.保留所有权利。

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