Interaction of the Extreme N-Terminal Region of FliH with FlhA Is Required for Efficient Bacterial Flagellar Protein Export

Hara, Noritaka; Morimoto, Yusuke V.; Kawamoto, Akihiro; Namba, Keiichi; Minamino, Tetsuo

doi:10.1128/jb.01028-12

Cited by 53 publications

(50 citation statements)

References 49 publications

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“…Both the identified minimal export signal of the flagellin and fulllength anti-s 28 factor FlgM have been successfully used as export signals for substrates which could subsequently cleaved by TEV protease [190,191]. As in the injectisome, both the peptide sequence and an mRNA signal seem to play a role in substrate recognition [189].…”

Section: Export Signalsmentioning

confidence: 99%

“…In E. coli, a class 1 master operon, flhDC, regulated by metabolic state and cell cycle, controls the expression of class 2 operons, which encode for the proximal structural components of the flagellum including its T3SS core. After completion of the T3SS, the anti-s 28 factor FlgM, a T3SS substrate, is exported, which allows the expression of class 3 genes, including the filament subunit, by the alternative sigma factor s 28 [64].…”

Section: Transcriptional and Post-transcriptional Regulation Of The T3ssmentioning

confidence: 99%

“…Environmental inputs control not only whether a bacterium needs a flagellum, but also how [28,29]. Flagellar model based on the study of Minamino & Imada [30]; injectisome model modified from [31]; based on cryo-electromicroscopic data [32]; F 0 F 1 -ATP synthase and structural homologies based on Ibuki et al [33].…”

Section: Transcriptional and Post-transcriptional Regulation Of The T3ssmentioning

confidence: 99%

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Type III secretion systems: the bacterial flagellum and the injectisome

Diepold

Armitage

2015

Phil. Trans. R. Soc. B

184

175

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One contribution of 12 to a theme issue 'The bacterial cell envelope'. The flagellum and the injectisome are two of the most complex and fascinating bacterial nanomachines. At their core, they share a type III secretion system (T3SS), a transmembrane export complex that forms the extracellular appendages, the flagellar filament and the injectisome needle. Recent advances, combining structural biology, cryo-electron tomography, molecular genetics, in vivo imaging, bioinformatics and biophysics, have greatly increased our understanding of the T3SS, especially the structure of its transmembrane and cytosolic components, the transcriptional, post-transcriptional and functional regulation and the remarkable adaptivity of the system. This review aims to integrate these new findings into our current knowledge of the evolution, function, regulation and dynamics of the T3SS, and to highlight commonalities and differences between the two systems, as well as their potential applications.

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Section: Export Signalsmentioning

confidence: 99%

Section: Transcriptional and Post-transcriptional Regulation Of The T3ssmentioning

confidence: 99%

Section: Transcriptional and Post-transcriptional Regulation Of The T3ssmentioning

confidence: 99%

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Type III secretion systems: the bacterial flagellum and the injectisome

Diepold

Armitage

2015

Phil. Trans. R. Soc. B

184

175

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“…The N-terminal region composed of residues 1-100 (FliH N ) is elongated, and the extreme N-terminal region is responsible for the interaction with FliN and FlhA to allow the FliI 6 ring to associate with the export gate (10)(11)(12)27). The middle region, residues 101-140, is essential for homodimer formation.…”

mentioning

confidence: 99%

Insight into the flagella type III export revealed by the complex structure of the type III ATPase and its regulator

Imada

Minamino

Uchida

et al. 2016

Proc. Natl. Acad. Sci. U.S.A.

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FliI and FliJ form the FliI 6 FliJ ATPase complex of the bacterial flagellar export apparatus, a member of the type III secretion system. The FliI 6 FliJ complex is structurally similar to the α 3 β 3 γ complex of F 1 -ATPase. The FliH homodimer binds to FliI to connect the ATPase complex to the flagellar base, but the details are unknown. Here we report the structure of the homodimer of a C-terminal fragment of FliH (FliH C2 ) in complex with FliI. FliH C2 shows an unusually asymmetric homodimeric structure that markedly resembles the peripheral stalk of the A/V-type ATPases. The FliH C2 -FliI hexamer model reveals that the C-terminal domains of the FliI ATPase face the cell membrane in a way similar to the F/A/V-type ATPases. We discuss the mechanism of flagellar ATPase complex formation and a common origin shared by the type III secretion system and the F/A/V-type ATPases.bacterial flagellum | type III protein export | crystal structure | F/A/V-type ATPase

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“…The first 20 N-terminal residues of FliI mediate self-oligomerization (18) and are involved in binding FliH (19,20). FliH is homologous to the β and δ subunits of the F o F 1 ATP synthase (21) and is thought to provide the support point for the association of the FliI ring to the export gate (22). FliJ, which is essential for the export of flagellum building blocks, binds to the center of the hexametric FliI ring in a manner similar to the way the γ subunit binds to the β subunit of F o F 1 ATP synthase (23).…”

mentioning

confidence: 99%

Recognition and targeting mechanisms by chaperones in flagellum assembly and operation

Khanra

Rossi

Economou

et al. 2016

Proc. Natl. Acad. Sci. U.S.A.

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The flagellum is a complex bacterial nanomachine that requires the proper assembly of several different proteins for its function. Dedicated chaperones are central in preventing aggregation or undesired interactions of flagellar proteins, including their targeting to the export gate. FliT is a key flagellar chaperone that binds to several flagellar proteins in the cytoplasm, including its cognate filament-capping protein FliD. We have determined the solution structure of the FliT chaperone in the free state and in complex with FliD and the flagellar ATPase FliI. FliT adopts a four-helix bundle and uses a hydrophobic surface formed by the first three helices to recognize its substrate proteins. We show that the fourth helix constitutes the binding site for FlhA, a membrane protein at the export gate. In the absence of a substrate protein FliT adopts an autoinhibited structure wherein both the binding sites for substrates and FlhA are occluded. Substrate binding to FliT activates the complex for FlhA binding and thus targeting of the chaperone-substrate complex to the export gate. The activation and targeting mechanisms reported for FliT appear to be shared among the other flagellar chaperones.flagellum | chaperones | assembly factors | NMR spectroscopy | type III secretion

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Interaction of the Extreme N-Terminal Region of FliH with FlhA Is Required for Efficient Bacterial Flagellar Protein Export

Cited by 53 publications

References 49 publications

Type III secretion systems: the bacterial flagellum and the injectisome

Type III secretion systems: the bacterial flagellum and the injectisome

Insight into the flagella type III export revealed by the complex structure of the type III ATPase and its regulator

Recognition and targeting mechanisms by chaperones in flagellum assembly and operation

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