The FF -ATP (F-ATP) synthase is essential for growth of , the causative agent of tuberculosis (TB). In addition to their synthase function most F-ATP synthases possess an ATP-hydrolase activity, which is coupled to proton-pumping activity. However, the mycobacterial enzyme lacks this reverse activity, but the reason for this deficiency is unclear. Here, we report that a -specific, 36-amino acid long C-terminal domain in the nucleotide-binding subunit α (α) of F-ATP synthase suppresses its ATPase activity and determined the mechanism of suppression. First, we employed vesicles to show that in intact membrane-embedded mycobacterial F-ATP synthases deletion of the C-terminal domain enabled ATPase and proton-pumping activity. We then generated a heterologous F-ATP synthase model system, which demonstrated that transfer of the mycobacterial C-terminal domain to a standard F-ATP synthase α subunit suppresses ATPase activity. Single-molecule rotation assays indicated that the introduction of this -specific domain decreased the angular velocity of the power-stroke after ATP binding. Solution X-ray scattering data and NMR results revealed the solution shape of α and the 3D structure of the subunit α C-terminal peptide PDEHVEALDEDKLAKEAVKV of (α(521-540)), respectively. Together with cross-linking studies, the solution structural data lead to a model, in which α(521-540) comes in close proximity with subunit γ residues 104-109, whose interaction may influence the rotation of the camshaft-like subunit γ. Finally, we propose that the unique segment α(514-549), which is accessible at the C terminus of mycobacterial subunit α, is a promising drug epitope.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC5500794PMC
http://dx.doi.org/10.1074/jbc.M117.784959DOI Listing

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