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STX6-VTI1B-VAMP3 复合物通过调节再循环内体和自噬体之间的融合来促进异噬作用。

The STX6-VTI1B-VAMP3 complex facilitates xenophagy by regulating the fusion between recycling endosomes and autophagosomes.

机构信息

a Department of Microbiology , Graduate School of Medicine, Kyoto University , Kyoto , Japan.

出版信息

Autophagy. 2017 Jan 2;13(1):57-69. doi: 10.1080/15548627.2016.1241924. Epub 2016 Oct 28.

Abstract

Macroautophagy/autophagy plays a critical role in immunity by directly degrading invading pathogens such as Group A Streptococcus (GAS), through a process that has been named xenophagy. We previously demonstrated that autophagic vacuoles directed against GAS, termed GAS-containing autophagosome-like vacuoles (GcAVs), use recycling endosomes (REs) as a membrane source. However, the precise molecular mechanism that facilitates the fusion between GcAVs and REs remains unclear. Here, we demonstrate that STX6 (syntaxin 6) is recruited to GcAVs and forms a complex with VTI1B and VAMP3 to regulate the GcAV-RE fusion that is required for xenophagy. STX6 targets the GcAV membrane through its tyrosine-based sorting motif and transmembrane domain, and localizes to TFRC (transferrin receptor)-positive punctate structures on GcAVs through its H2 SNARE domain. Knockdown and knockout experiments revealed that STX6 is required for the fusion between GcAVs and REs to promote clearance of intracellular GAS by autophagy. Moreover, VAMP3 and VTI1B interact with STX6 and localize on the TFRC-positive puncta on GcAVs, and are also involved in the RE-GcAV fusion. Furthermore, knockout of RABGEF1 impairs the RE-GcAV fusion and STX6-VAMP3 interaction. These findings demonstrate that RABGEF1 mediates RE fusion with GcAVs through the STX6-VAMP3-VTI1B complex, and reveal the SNARE dynamics involved in autophagosome formation in response to bacterial infection.

摘要

自噬在免疫中起着关键作用,它通过一种被称为异噬(xenophagy)的过程,直接降解入侵的病原体,如 A 组链球菌(Group A Streptococcus,GAS)。我们之前的研究表明,针对 GAS 的自噬空泡,称为含 GAS 的自噬体样空泡(GAS-containing autophagosome-like vacuoles,GcAVs),使用再循环内体(recycling endosomes,REs)作为膜源。然而,促进 GcAVs 与 REs 融合的确切分子机制尚不清楚。在这里,我们证明 STX6(突触融合蛋白 6)被募集到 GcAVs 上,并与 VTI1B 和 VAMP3 形成复合物,调节异噬所需的 GcAV-RE 融合。STX6 通过其酪氨酸基分拣基序和跨膜结构域靶向 GcAV 膜,并通过其 H2 SNARE 结构域定位到 GcAV 上 TFRC(转铁蛋白受体)阳性点状结构。敲低和敲除实验表明,STX6 对于 GcAVs 与 REs 的融合是必需的,以促进自噬清除细胞内的 GAS。此外,VAMP3 和 VTI1B 与 STX6 相互作用并定位于 GcAV 上的 TFRC 阳性点状结构,并且也参与 RE-GcAV 融合。此外,RABGEF1 的敲除会损害 RE-GcAV 融合和 STX6-VAMP3 相互作用。这些发现表明,RABGEF1 通过 STX6-VAMP3-VTI1B 复合物介导 RE 与 GcAV 的融合,并揭示了参与细菌感染时自噬体形成的 SNARE 动力学。

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