Cell Envelope Signaling in Escherichia coli

Moeck, Gregory S.; Coulton, James W.; Postle, Kathleen

doi:10.1074/jbc.272.45.28391

Cited by 89 publications

(37 citation statements)

References 55 publications

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“…Chemical cross-linking (12,30) and recent protein crystal structures (20,31) indicate that the Ton box interacts with TonB. There also is evidence that this Ton box-TonB interaction occurs in a substrate-dependent manner (12,32); thus, some signal transduction event must initiate this interaction. Genetic studies suggest that iron siderophore and vitamin B 12 transport systems compete for TonB (33), and regulation of the transporter-TonB interaction by a substratedependent signaling event would account for this observation and optimize the use of TonB, which is stoichiometrically limiting.…”

Section: Discussionmentioning

confidence: 99%

Substrate-dependent transmembrane signaling in TonB-dependent transporters is not conserved

Kim

Fanucci

Cafiso

2007

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

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Site-directed spin labeling (SDSL) was used to examine and compare transmembrane signaling events in the bacterial outermembrane transport proteins BtuB, FecA, and FhuA. These proteins extract energy for transport by coupling to the transperiplasmic protein TonB, an interaction that is thought to be mediated by the Ton box, a highly conserved energy-coupling motif in these transporters. In the ferric citrate transporter, FecA, SDSL indicates that the Ton box undergoes a substrate-induced disorder transition similar to that seen for BtuB, the vitamin B12 transporter. This conformational change produces an aqueous exposed, highly disordered protein fragment, which likely regulates transporter-TonB interactions. However, in the ferrichrome transporter, FhuA, SDSL does not reveal a substrate-induced unfolding transition. In this protein, with or without substrate, the Ton box conformation is found to be highly dynamic and constitutively unfolded. In addition, SDSL indicates that structural features seen in high-resolution models are not found in membrane-associated FhuA. Taken together, these data indicate that the Ton box of FhuA may always be available for interactions with TonB, implying that transporterTonB interactions in FhuA are either constitutive or not regulated by the Ton box configuration.EPR spectroscopy ͉ membrane protein ͉ site-directed spin labeling

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Section: Discussionmentioning

confidence: 99%

Substrate-dependent transmembrane signaling in TonB-dependent transporters is not conserved

Kim

Fanucci

Cafiso

2007

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

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“…A close apposition of the TonB box of the receptor with the Cterminal TonB region around Gln 160 has been inferred from in vivo experiments using tonB suppressor mutants (18), crosslinking data (8), disulfide formation in cysteine substitution mutants (9), and competitive binding of peptides (20). In vitro, complexes between receptors and TonB have been described that are more stable when the receptor contains bound ligand (17,10,21,22,44,45). Because of the crystallographic evidence for an allosteric conformational change at the periplasmic surface of the receptor, TonB could in principle bind there without significantly altering its conformation, but an induced fit of TonB upon binding cannot be excluded.…”

Section: Discussionmentioning

confidence: 99%

Crystal Structure of a 92-Residue C-terminal Fragment of TonB from Escherichia coli Reveals Significant Conformational Changes Compared to Structures of Smaller TonB Fragments

Ködding

Killig

Polzer

et al. 2005

Journal of Biological Chemistry

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Uptake of siderophores and vitamin B 12 through the outer membrane of Escherichia coli is effected by an active transport system consisting of several outer membrane receptors and a protein complex of the inner membrane. The link between these is TonB, a protein associated with the cytoplasmic membrane, which forms a large periplasmic domain capable of interacting with several outer membrane receptors, e.g.

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“…ToxR(1-210)-PhoA(27-472) and ToxR(1-210)-MalE(27-397) were used as positive and negative controls, respectively. In addition, cells were grown in the presence and absence of 1 mM citrate, since TonB may preferentially bind to FecA loaded with ferric citrate, as has been found for ferrichrome binding to FhuA (34,35) and ferric enterobactin binding to FepA (41). Binding to ferric citrate-loaded FecA may change the conformation of TonB and affect dimer formation.…”

Section: Tonb Dimersmentioning

confidence: 99%

“…In addition, the required energy is provided by the proton motive force of the cytoplasmic membrane (2), along with an energy-transducing device in the cytoplasmic membrane which is composed of the TonB, ExbB, and ExbD proteins (3,22,37). The N terminus of TonB (residues 13 to 32) anchors it to the inner membrane, while most of the protein is located in the periplasm, where it interacts with outer membrane transporters (7,15,35,40). The topography of ExbD resembles that of TonB (23), whereas ExbB spans the cytoplasmic membrane three times, with most of the protein being located in the cytoplasm (24).…”

mentioning

confidence: 99%

In Vivo Evidence for TonB Dimerization

2003

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TonB, in complex with ExbB and ExbD, is required for the energy-dependent transport of ferric siderophores across the outer membrane of Escherichia coli, the killing of cells by group B colicins, and infection by phages T1 and 80. To gain insights into the protein complex, TonB dimerization was studied by constructing hybrid proteins from complete TonB (containing amino acids 1 to 239) [TonB(1-239)] and the cytoplasmic fragment of ToxR which, when dimerized, activates the transcription of the cholera toxin gene ctx. ToxR(1-182)-TonB(1-239) activated the transcription of lacZ under the control of the ctx promoter (P ctx ::lacZ). Replacement of the TonB transmembrane region by the ToxR transmembrane region resulted in the hybrid proteins ToxR(1-210)-TonB(33-239) and ToxR(1-210)-TonB(164-239), of which only the latter activated P ctx ::lacZ transcription. Dimer formation was reduced but not abolished in a mutant lacking ExbB and ExbD, suggesting that these complex components may influence dimerization but are not strictly required and that the N-terminal cytoplasmic membrane anchor and the C-terminal region are important for dimer formation. The periplasmic TonB fragment, TonB(33-239), inhibits ferrichrome and ferric citrate transport and induction of the ferric citrate transport system. This competition provided a means to positively screen for TonB(33-239) mutants which displayed no inhibition. Single point mutations of inactive fragments selected in this manner were introduced into complete TonB, and the phenotypes of the TonB mutant strains were determined. The mutations located in the C-terminal half of TonB, three of which (Y163C, V188E, and R204C) were obtained separately by site-directed mutagenesis, as was the isolated F230V mutation, were studied in more detail. They displayed different activity levels for various TonB-dependent functions, suggesting function-related specificities which reflect differences in the interactions of TonB with various transporters and receptors.

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Cell Envelope Signaling in Escherichia coli

Cited by 89 publications

References 55 publications

Substrate-dependent transmembrane signaling in TonB-dependent transporters is not conserved

Substrate-dependent transmembrane signaling in TonB-dependent transporters is not conserved

Crystal Structure of a 92-Residue C-terminal Fragment of TonB from Escherichia coli Reveals Significant Conformational Changes Compared to Structures of Smaller TonB Fragments

In Vivo Evidence for TonB Dimerization

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