TatA and TatB generate a hydrophobic mismatch important for the function and assembly of the Tat translocon in Escherichia coli

• Published in: The Journal of biological chemistry Vol. 298; no. 9; p. 102236
• Main Authors: Mehner-Breitfeld, Denise, Ringel, Michael T., Tichy, Daniel Alexander, Endter, Laura J., Stroh, Kai Steffen, Lünsdorf, Heinrich, Risselada, Herre Jelger, Brüser, Thomas
• Format: Journal Article
• Language: English
• Published: Elsevier Inc 01.09.2022; American Society for Biochemistry and Molecular Biology
• Subjects: computational biology; hydrophobic mismatch; membrane proteins; membrane thinning; metal-tagging transmission electron microscopy (METTEM); protein translocation; stress response; Tat system; computational biology; COM; BN-PAGE; Tat; TMH; protein translocation; PEELS; membrane proteins; stress response; hydrophobic mismatch; METTEM; APH; Tat system; metal-tagging transmission electron microscopy (METTEM); membrane thinning
• ISSN: 0021-9258; 1083-351X
• DOI: 10.1016/j.jbc.2022.102236

The twin-arginine translocation (Tat) system serves to translocate folded proteins across energy-transducing membranes in bacteria, archaea, plastids, and some mitochondria. In Escherichia coli, TatA, TatB, and TatC constitute functional translocons. TatA and TatB both possess an N-terminal transmembrane helix (TMH) followed by an amphipathic helix. The TMHs of TatA and TatB generate a hydrophobic mismatch with the membrane, as the helices comprise only 12 consecutive hydrophobic residues; however, the purpose of this mismatch is unclear. Here, we shortened or extended this stretch of hydrophobic residues in either TatA, TatB, or both and analyzed effects on translocon function and assembly. We found the WT length helices functioned best, but some variation was clearly tolerated. Defects in function were exacerbated by simultaneous mutations in TatA and TatB, indicating partial compensation of mutations in each by the other. Furthermore, length variation in TatB destabilized TatBC-containing complexes, revealing that the 12-residue-length is important but not essential for this interaction and translocon assembly. To also address potential effects of helix length on TatA interactions, we characterized these interactions by molecular dynamics simulations, after having characterized the TatA assemblies by metal-tagging transmission electron microscopy. In these simulations, we found that interacting short TMHs of larger TatA assemblies were thinning the membrane and—together with laterally-aligned tilted amphipathic helices—generated a deep V-shaped membrane groove. We propose the 12 consecutive hydrophobic residues may thus serve to destabilize the membrane during Tat transport, and their conservation could represent a delicate compromise between functionality and minimization of proton leakage.