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首页> 外文期刊>Nature Communications >STX17 dynamically regulated by Fis1 induces mitophagy via hierarchical macroautophagic mechanism
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STX17 dynamically regulated by Fis1 induces mitophagy via hierarchical macroautophagic mechanism

机译:由Fis1动态调节的STX17通过分级的巨自噬机制诱导线粒体吞噬

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Mitophagy is the selective autophagic targeting and removal of dysfunctional mitochondria. While PINK1/Parkin-dependent mitophagy is well-characterized, PINK1/Parkin-independent route is poorly understood. Using structure illumination microscopy (SR-SIM), we demonstrate that the SNARE protein Syntaxin 17 (STX17) initiates mitophagy upon depletion of outer mitochondrial membrane protein Fis1. With proteomics analysis, we identify the STX17-Fis1 interaction, which controls the dynamic shuffling of STX17 between ER and mitochondria. Fis1 loss results in aberrant STX17 accumulation on mitochondria, which exposes the N terminus and promotes self-oligomerization to trigger mitophagy. Mitochondrial STX17 interacts with ATG14 and recruits core autophagy proteins to form mitophagosome, followed by Rab7-dependent mitophagosome-lysosome fusion. Furthermore, Fis1 loss impairs mitochondrial respiration and potentially sensitizes cells to mitochondrial clearance, which is mediated through canonical autophagy machinery, closely linking non-selective macroautophagy to mitochondrial turnover. Our findings uncover a PINK1/Parkin-independent mitophagic mechanism in which outer mitochondrial membrane protein Fis1 regulates mitochondrial quality control.
机译:线粒体是功能性线粒体的选择性自噬靶向和去除。尽管PINK1 / Parkin依赖性线粒体的特征非常明确,但对PINK1 / Parkin依赖性途径的了解却很少。使用结构照明显微镜(SR-SIM),我们证明了SNARE蛋白Syntaxin 17(STX17)在线粒体外膜蛋白Fis1耗尽后引发线粒体。通过蛋白质组学分析,我们确定了STX17-Fis1相互作用,该相互作用控制ER和线粒体之间STX17的动态改组。 Fis1丢失导致线粒体上异常的STX17积累,从而暴露N端并促进自我寡聚化以触发线粒体。线粒体STX17与ATG14相互作用并募集核心自噬蛋白以形成线粒体,然后进行Rab7依赖性线粒体-溶酶体融合。此外,Fis1的缺失会损害线粒体呼吸,并可能使细胞对线粒体清除敏感,线粒体清除是通过规范自噬机制介导的,将非选择性的巨自噬与线粒体更新紧密联系在一起。我们的发现揭示了不依赖PINK1 / Parkin的线粒体机制,其中外部线粒体膜蛋白Fis1调节线粒体质量控制。

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