MinD-like ATPase FlhG effects location and number of bacterial flagella during C-ring assembly

The number and location of flagella, bacterial organelles of locomotion, are species specific and appear in regular patterns that represent one of the earliest taxonomic criteria in microbiology. However, the mechanisms that reproducibly establish these patterns during each round of cell division are poorly understood. FlhG (previously YlxH) is a major determinant for a variety of flagellation patterns. Here, we show that FlhG is a structural homolog of the ATPase MinD, which serves in cell-division site determination. Like MinD, FlhG forms homodimers that are dependent on ATP and lipids. It interacts with a complex of the flagellar C-ring proteins FliM and FliY (also FliN) in the Gram-positive, peritrichous-flagellated Bacillus subtilis and the Gram-negative, polar-flagellated Shewanella putrefaciens. FlhG interacts with FliM/FliY in a nucleotide-independent manner and activates FliM/FliY to assemble with the C-ring protein FliG in vitro. FlhG-driven assembly of the FliM/FliY/FliG complex is strongly enhanced by ATP and lipids. The protein shows a highly dynamic subcellular distribution between cytoplasm and flagellar basal bodies, suggesting that FlhG effects flagellar location and number during assembly of the C-ring. We describe the molecular evolution of a MinD-like ATPase into a flagellation pattern effector and suggest that the underappreciated structural diversity of the C-ring proteins might contribute to the formation of different flagellation patterns.Most bacteria move by flagella. The flagellar architecture is conserved and can be divided into the cytoplasmic C-ring, the basal body, the rod, and the exterior hook and filament structures (1). Bacterial species differ in the number and arrangement of their flagella (flagellation pattern) (2). However, the mechanisms that allow bacteria to establish their specific flagellation patterns reproducibly during each cell division are poorly understood. The protein FlhG (also known as “YlxH,” “MinD2,” “FleN,” or “MotR”) is essential for the correct flagellation pattern of polar- (3–5), lophotrichous- (6), amphitrichous- (7), and peritrichous-flagellated bacteria (8, 9). Deletion of flhG in polar-flagellated bacteria leads to hyperflagellation and impaired motility (3–5). In the amphitrichous-flagellated Campylobacter jejuni, ∼40% of the cells of a ΔflhG strain exhibited more than one flagellum at one pole and were impaired in motility (7). The peritrichous-flagellated bacterium Bacillus subtilis exhibits ∼26 flagellar basal bodies arranged symmetrically around midcell in a gridlike pattern (8). Furthermore, flagella are discouraged at the cell pole. Deletion of flhG does not result in swimming or swarming defects, although multiple flagella appear in tufts from constrained loci on the cell, and flagellar basal bodies often are aggregated (8). FlhG acts in concert with the signal recognition particle (SRP)-GTPase FlhF (10–14) that recruits the flagellar protein FliF to the cell pole in the polar-flagellated Vibrio cholerae (15). FlhG is predicted to belong to the MinD/ParA ATPase family (6, 16) whose characterized members act in orchestrated spatiotemporal processes (e.g., cell-division site determination and plasmid/chromosome partitioning (summarized in ref. 17). Together with MinC, MinD constitutes the conserved center of the Min system which regulates bacterial cell division by restricting cytokinetic Z-ring assembly to midcell (reviewed in ref. 18). MinD forms ATP-dependent homodimers (19) that interact with the inner membrane through a C-terminal amphipathic helix (membrane-targeting sequence, MTS) (20, 21). By this mechanism, MinD recruits MinC to the membrane where MinC inhibits polymerization of FtsZ into the Z-ring (22). Interestingly, Campylobacter jejuni does not contain a Min system, and FlhG is involved in flagellation pattern control and regulation of cell division (7). In contrast to MinD, the molecular framework in which the putative MinD-like ATPase FlhG controls flagellation is unknown. Also, it is enigmatic how conserved homologs of FlhG can control different flagellation patterns in different species. Here, we investigated the mechanism and function of FlhG in the Gram-positive, peritrichous-flagellated B. subtilis (Bs) and the Gram-negative, polar-flagellated Shewanella putrefaciens (Sp).