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Probing the Environment of Emerin by Enhanced Ascorbate Peroxidase 2 (APEX2)-Mediated Proximity Labeling

机译:通过增强的抗坏血酸过氧化物酶2(APEX2)介导的邻近标记探测翡翠的环境。

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摘要

Emerin is one of the best characterized proteins of the inner nuclear membrane, but can also occur at the level of the endoplasmic reticulum. We now use enhanced ascorbate peroxidase 2 (APEX2) to probe the environment of emerin. APEX2 can be used as a genetic tag that produces short-lived yet highly reactive biotin species, allowing the modification of proteins that interact with or are in very close proximity to the tagged protein. Biotinylated proteins can be isolated using immobilized streptavidin and analyzed by mass spectrometry. As an alternative to the standard approach with a genetic fusion of APEX2 to emerin, we also used RAPIDS (rapamycin- and APEX-dependent identification of proteins by SILAC), a method with improved specificity, where the peroxidase interacts with the protein of interest (i.e., emerin) only upon addition of rapamycin to the cells. We compare these different approaches, which, together, identify well-known interaction partners of emerin like lamin A and the lamina associated polypeptide 1 (LAP1), as well as novel proximity partners.
机译:Emerin是内核膜中最有特征的蛋白质之一,但也可以在内质网水平上发生。现在,我们使用增强型抗坏血酸过氧化物酶2(APEX2)来探测Emerin的环境。 APEX2可用作产生短寿命但反应性强的生物素物种的遗传标签,允许修饰与被标记蛋白质相互作用或非常接近的蛋白质。可以使用固定的抗生蛋白链菌素分离生物素化的蛋白质,并通过质谱分析。作为APEX2与Emerin遗传融合的标准方法的替代方法,我们还使用了RAPIDS(通过SILAC识别雷帕霉素和APEX依赖性蛋白质),该方法具有更高的特异性,其中过氧化物酶与目标蛋白质相互作用(仅在将雷帕霉素添加到细胞中后才可使用。我们比较了这些不同的方法,这些方法共同确定了emerin像层粘连蛋白A和层状相关多肽1(LAP1)以及新的邻近性伙伴的众所周知的相互作用伙伴。

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