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Emery-Dreifuss muscular dystrophy mutations impair TRC40-mediated targeting of emerin to the inner nuclear membrane.

机译:Emery-Dreifuss肌营养不良症突变损害TRC40介导的emerin靶向内核膜。

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摘要

Emerin is a tail-anchored protein that is found predominantly at the inner nuclear membrane (INM), where it associates with components of the nuclear lamina. Mutations in the emerin gene cause Emery-Dreifuss muscular dystrophy (EDMD), an X-linked recessive disease. Here, we report that the TRC40/GET pathway for post-translational insertion of tail-anchored proteins into membranes is involved in emerin-trafficking. Using proximity ligation assays, we show that emerin interacts with TRC40 in situ. Emerin expressed in bacteria or in a cell-free lysate was inserted into microsomal membranes in an ATP- and TRC40-dependent manner. Dominant-negative fragments of the TRC40-receptor proteins WRB and CAML (also known as CAMLG) inhibited membrane insertion. A rapamycin-based dimerization assay revealed correct transport of wild-type emerin to the INM, whereas TRC40-binding, membrane integration and INM-targeting of emerin mutant proteins that occur in EDMD was disturbed. Our results suggest that the mode of membrane integration contributes to correct targeting of emerin to the INM.
机译:Emerin是一种尾部锚定蛋白,主要存在于内核膜(INM)处,并与核层的成分结合。 Emerin基因的突变会导致Emery-Dreifuss肌营养不良(EDMD),一种与X连锁的隐性疾病。在这里,我们报告说,TRE40 / GET途径将尾锚蛋白翻译后插入膜中,参与了游走蛋白的运输。使用邻近结扎试验,我们显示了Emerin与TRC40原位相互作用。将细菌或无细胞裂解物中表达的Emerin以ATP和TRC40依赖性方式插入微粒体膜。 TRC40受体蛋白WRB和CAML(也称为CAMLG)的显性负片段抑制了膜的插入。基于雷帕霉素的二聚化分析显示野生型Emerin正确运输到INM,而在EDMD中发生的TRC40结合,膜整合和EmM突变蛋白的INM靶向受到干扰。我们的结果表明,膜整合的模式有助于正确地将Emerin靶向INM。

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