The molecular mechanism of cotranslational membrane protein recognition and targeting by SecA

Creators: Wang, Shuai; Jomaa, Ahmad; Jaskolowski, Mateusz; Yang, Chien-I; Ban, Nenad; Shan, Shu-ou

Abstract

Cotranslational protein targeting is a conserved process for membrane protein biogenesis. In Escherichia coli, the essential ATPase SecA was found to cotranslationally target a subset of nascent membrane proteins to the SecYEG translocase at the plasma membrane. The molecular mechanism of this pathway remains unclear. Here we use biochemical and cryoelectron microscopy analyses to show that the amino-terminal amphipathic helix of SecA and the ribosomal protein uL23 form a composite binding site for the transmembrane domain (TMD) on the nascent protein. This binding mode further enables recognition of charged residues flanking the nascent TMD and thus explains the specificity of SecA recognition. Finally, we show that membrane-embedded SecYEG promotes handover of the translating ribosome from SecA to the translocase via a concerted mechanism. Our work provides a molecular description of the SecA-mediated cotranslational targeting pathway and demonstrates an unprecedented role of the ribosome in shielding nascent TMDs.

Additional Information

© 2019 Springer Nature Limited. Received 04 May 2019; Accepted 12 August 2019; Published 30 September 2019. Data Availability: Cryo-EM maps are deposited in the electron microscopy databank (EMDB) with accession codes EMD-10073 (RNCRodZ–SecA) and EMD-10074 (SecA, local refinement), and model coordinates are deposited in the worldwide PDB with accession code PDB 6S0K. Other data are available from corresponding authors upon reasonable request. We thank A. McDowall and H. Wang for assistance with negative stain electron microscopy data collection, J. Rothman for sharing plasmid ApoE422k, D. Boehringer and A. Scaiola for the support with EM data collection and processing, M. Leibundgut and M. Saurer for the support with model building and members of the Shan and Ban groups for discussions and comments on the manuscript. We also thank T. Miller, M. Zimmer and F. Huber for helpful discussions. Cryo-EM data was collected at the Scientific Center for Optical and Electron Microscopy at the ETH Zurich (ScopeM). We gratefully acknowledge the support of NVIDIA Corporation for the Titan Xp GPU used in this research through a GPU Grant program awarded to A.J.; M.J. was supported by the internal research grant of the ETH to N.B. (ETH-40 16-2). This work was supported by National Institutes of Health grant GM107368A and the Gordon and Betty Moore Foundation through grant GBMF2939 to S.S. and by the Swiss National Science Foundation (SNSF) (grant number 310030B_163478), National Center of Excellence in Research (NCCR) RNA & Disease Program of the SNSF (grant number 51NF40_141735) to N.B. Author Contributions: S.W. and S.S. conceived the project. S.W. performed most of the biochemical experiments and analyzed data. A.J. acquired cryo-electron microscopy data and performed reconstructions and model building. M.J. performed initial sample preparation for cryo-EM analysis. C.Y. measured the association rate constant of SecA binding to RNCRodZ. N.B. and S.S. supervised the structural and biochemical experiments, respectively. All authors interpreted the data and contributed to the final versions of the manuscript. The authors declare no competing interests.

Attached Files

Accepted Version - nihms-1537248.pdf

Supplemental Material - 41594_2019_297_Fig10_ESM.jpg

Supplemental Material - 41594_2019_297_Fig11_ESM.jpg

Supplemental Material - 41594_2019_297_Fig12_ESM.jpg

Supplemental Material - 41594_2019_297_Fig13_ESM.jpg

Supplemental Material - 41594_2019_297_Fig14_ESM.jpg

Supplemental Material - 41594_2019_297_Fig15_ESM.jpg

Supplemental Material - 41594_2019_297_Fig8_ESM.jpg

Supplemental Material - 41594_2019_297_Fig9_ESM.jpg

Supplemental Material - 41594_2019_297_MOESM1_ESM.pdf

Supplemental Material - 41594_2019_297_MOESM2_ESM.pdf

Files

41594_2019_297_Fig13_ESM.jpg

Files (10.4 MB)

Name	Size	Download all
41594_2019_297_Fig13_ESM.jpg md5:50d8df2629134a5d44b9757cd3d4639b	258.7 kB	Preview Download
41594_2019_297_Fig11_ESM.jpg md5:1aa931cbafa24cc7fb75fbe4662a55df	205.7 kB	Preview Download
41594_2019_297_Fig12_ESM.jpg md5:cf2e0c51d6db8c4a803512d6086eb4c2	335.1 kB	Preview Download
41594_2019_297_Fig14_ESM.jpg md5:2682b66a91f9548d23ff693b09c0a4e7	288.1 kB	Preview Download
41594_2019_297_Fig15_ESM.jpg md5:34a86a6145218cf35b3db3dc20ec978a	445.2 kB	Preview Download
41594_2019_297_Fig8_ESM.jpg md5:1b6e4f1c926e228c6ef4deff6149a7b2	193.7 kB	Preview Download
41594_2019_297_Fig9_ESM.jpg md5:765415f3d6544c7f139ffd14396b69cd	217.0 kB	Preview Download
nihms-1537248.pdf md5:97bfafcb1bee39855e78f55cebd04190	2.9 MB	Preview Download
41594_2019_297_MOESM1_ESM.pdf md5:64b4de899abd4cd5170a99dfdc866699	3.1 MB	Preview Download
41594_2019_297_MOESM2_ESM.pdf md5:f439508e9fd8538762bc5026384660b3	2.3 MB	Preview Download
41594_2019_297_Fig10_ESM.jpg md5:efc070bfcc6b1fdd29022cac4459a10a	107.1 kB	Preview Download

Additional details

Views

Downloads

	All versions	This version
Views	0	0
Downloads	0	0
Data volume	0 Bytes	0 Bytes

More info on how stats are collected....

Resource type: Journal Article
Publisher: Nature Publishing Group
Published in: Nature Structural & Molecular Biology, 26(10), 919-929, ISSN: 1545-9985.