Fluorescent tools to analyse peroxisome-ER interactions in mammalian cells.

Alexa Bishop, Maki Kamoshita, Josiah B Passmore, Christian Hacker, Tina A Schrader, Hans R Waterham, Joseph L Costello, Michael Schrader
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引用次数: 9

Abstract

Peroxisomes and the endoplasmic reticulum (ER) cooperate extensively in lipid-related metabolic pathways, and the ER also provides phospholipids to enable the peroxisomal membrane to expand prior to division. Recently, we identified peroxisomal proteins ACBD5 and ACBD4, and the ER protein VAPB as tethering components which physically interact to foster peroxisome-ER associations at membrane contact sites. Overexpression or loss of these tether proteins alters the extent of peroxisome-ER interactions, impacting on lipid exchange between these two compartments. To facilitate further studies into peroxisome-ER associations at the level of membrane contact sites, their role, composition and regulation, we have developed two fluorescence-based systems to monitor peroxisome-ER interactions. We modified a proximity ligation assay and a split-fluorescence reporter system using split superfolder green fluorescent protein. Using the proximity ligation assay we were able to measure changes in peroxisome-ER interactions whilst the split-fluorescence reporter was more limited and only allowed us to label ER-peroxisome contacts. We show that both techniques can be useful additions to the toolkit of methods to study peroxisome-ER associations and explore the relative merits of each.

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荧光工具分析哺乳动物细胞中过氧化物酶体-内质网相互作用。
过氧化物酶体和内质网(ER)在脂质相关代谢途径中广泛合作,内质网还提供磷脂,使过氧化物酶体膜在分裂前扩张。最近,我们发现过氧化物酶体蛋白ACBD5和ACBD4,以及内质网蛋白VAPB作为系带组分,它们在膜接触部位物理相互作用,促进过氧化物酶体-内质网结合。这些系链蛋白的过表达或缺失会改变过氧化物酶体-内质网相互作用的程度,影响这两个隔室之间的脂质交换。为了进一步研究过氧化物酶体-内质网在膜接触位点水平上的关联,它们的作用、组成和调控,我们开发了两种基于荧光的系统来监测过氧化物酶体-内质网的相互作用。我们使用分裂超级文件夹绿色荧光蛋白改进了接近结扎试验和分裂荧光报告系统。使用接近连接法,我们能够测量过氧化物酶体-内质网相互作用的变化,而分裂荧光报告更有限,只允许我们标记er -过氧化物酶体接触。我们表明,这两种技术都可以成为研究过氧化物酶体-内质网关联的方法工具包的有用补充,并探索每种方法的相对优点。
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