Structure of human PINK1 at a mitochondrial TOM-VDAC array
成果类型:
Article
署名作者:
Callegari, Sylvie; Kirk, Nicholas S.; Gan, Zhong Yan; Dite, Toby; Cobbold, Simon A.; Leis, Andrew; Dagley, Laura F.; Glukhova, Alisa; Komander, David
署名单位:
Walter & Eliza Hall Institute; University of Melbourne; University of Melbourne; Monash University; Monash University
刊物名称:
SCIENCE
ISSN/ISSBN:
0036-13375
DOI:
10.1126/science.adu6445
发表日期:
2025-04-18
页码:
303-310
关键词:
cryo-em structure
mass-spectrometry
parkin
ubiquitin
complex
activation
mechanism
mitophagy
substrate
phosphorylation
摘要:
Mutations in the ubiquitin kinase PINK1 cause early-onset Parkinson's disease, but how PINK1 is stabilized at depolarized mitochondrial translocase complexes has remained poorly understood. We determined a 3.1-angstrom resolution cryo-electron microscopy structure of dimeric human PINK1 stabilized at an endogenous array of mitochondrial translocase of the outer membrane (TOM) and voltage-dependent anion channel (VDAC) complexes. Symmetric arrangement of two TOM core complexes around a central VDAC2 dimer is facilitated by TOM5 and TOM20, both of which also bind PINK1 kinase C-lobes. PINK1 enters mitochondria through the proximal TOM40 barrel of the TOM core complex, guided by TOM7 and TOM22. Our structure explains how human PINK1 is stabilized at the TOM complex and regulated by oxidation, uncovers a previously unknown TOM-VDAC assembly, and reveals how a physiological substrate traverses TOM40 during translocation.