Abstract
Recent studies introduced a novel view that the SecYEG translocon functions as a monomer and interacts with the dimeric SecA ATPase, which fuels the preprotein translocation reaction. Here, we used nanodisc-reconstituted SecYEG to characterize the functional properties of single copies of the translocon. Using a method based on intermolecular Forster resonance energy transfer, we show for the first time that isolated nanodisc-reconstituted SecYEG monomers support preprotein translocation. When several copies of SecYEG were co-reconstituted within a nanodisc, no change in translocation kinetics was observed, suggesting that SecYEG oligomers do not facilitate enhanced translocation. In contrast, nanodisc-reconstituted monomers of the PrIA4 variant of SecYEG showed increased translocation rates. Experiments based on intramolecular Forster resonance energy transfer within the nanodisc-isolated monomeric SecYEG demonstrated a nucleotide-dependent opening of the channel upon interaction with SecA. In conclusion, the nanodisc-reconstituted SecYEG monomers are functional for preprotein translocation and provide a new prospect for single-molecule analysis of dynamic aspects of protein translocation. (C) 2013 Elsevier Ltd. All rights reserved.
| Original language | English |
|---|---|
| Pages (from-to) | 4145-4153 |
| Number of pages | 9 |
| Journal | Journal of Molecular Biology |
| Volume | 425 |
| Issue number | 22 |
| DOIs | |
| Publication status | Published - 15-Nov-2013 |
Keywords
- protein transport
- secretion
- protein oligomerization
- protein dynamics
- membrane proteins
- BACTERIAL CYTOPLASMIC MEMBRANE
- PHOSPHOLIPID-BILAYER NANODISCS
- PROTEIN-TRANSLOCATION
- ESCHERICHIA-COLI
- SIGNAL SEQUENCE
- PREPROTEIN TRANSLOCATION
- PRECURSOR PROTEINS
- SECY COMPLEX
- CHANNEL
- ATPASE