| Literature DB >> 31600774 |
Yuhei Araiso1,2,3, Akihisa Tsutsumi4, Jian Qiu5,6,7, Kenichiro Imai8, Takuya Shiota9,10, Jiyao Song5, Caroline Lindau5,11, Lena-Sophie Wenz5,12, Haruka Sakaue1,2, Kaori Yunoki1, Shin Kawano1,2, Junko Suzuki1, Marilena Wischnewski5,13, Conny Schütze5, Hirotaka Ariyama14, Toshio Ando14, Thomas Becker5,15, Trevor Lithgow9, Nils Wiedemann5,15, Nikolaus Pfanner5,15, Masahide Kikkawa4, Toshiya Endo16,17.
Abstract
The translocase of the outer mitochondrial membrane (TOM) is the main entry gate for proteins1-4. Here we use cryo-electron microscopy to report the structure of the yeast TOM core complex5-9 at 3.8-Å resolution. The structure reveals the high-resolution architecture of the translocator consisting of two Tom40 β-barrel channels and α-helical transmembrane subunits, providing insight into critical features that are conserved in all eukaryotes1-3. Each Tom40 β-barrel is surrounded by small TOM subunits, and tethered by two Tom22 subunits and one phospholipid. The N-terminal extension of Tom40 forms a helix inside the channel; mutational analysis reveals its dual role in early and late steps in the biogenesis of intermembrane-space proteins in cooperation with Tom5. Each Tom40 channel possesses two precursor exit sites. Tom22, Tom40 and Tom7 guide presequence-containing preproteins to the exit in the middle of the dimer, whereas Tom5 and the Tom40 N extension guide preproteins lacking a presequence to the exit at the periphery of the dimer.Entities:
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Year: 2019 PMID: 31600774 DOI: 10.1038/s41586-019-1680-7
Source DB: PubMed Journal: Nature ISSN: 0028-0836 Impact factor: 49.962