Dynamic Localization of a Transcription Factor in Bacillus subtilis: the LicT Antiterminator Relocalizes in Response to Inducer Availability

Rothe, Fabian M.; Wrede, Christoph; Lehnik-Habrink, Martin; Görke, Boris; Stülke, Jörg

doi:10.1128/jb.00117-13

Cited by 12 publications

(14 citation statements)

References 49 publications

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“…Still, one difference between the two organisms is that in E. coli cells, the EI proteins from both species localize to the cell pole independent of growth conditions, whereas in B. subtilis cells, EI localization seems to depend on growth conditions. Thus, when grown in LB, the native B. subtilis EI showed very little if any distinct localization (data not shown), similar to the distribution documented previously (17). The reason for the dependence of the B. subtilis EI localization pattern on the medium, which is in contrast to the lack of such dependence for E. coli EI (15), is currently not known.…”

Section: Discussionsupporting

confidence: 88%

“…The PTS proteins known to localize to the poles are all soluble. They include EI, which remains at the poles independent of environmental conditions, HPr, which discharges from the poles in response to the presence of PTS sugars in the growth medium, and transcription factors that regulate PTS operons, i.e., BglG in E. coli and LicT in B. subtilis , which are recruited to the poles depending on the availability of sugars that are transported and metabolized by the products of the operons that they regulate (15, 17). The membrane-bound components of the PTS, the sugar permeases, do not localize specifically to the poles; rather, they are distributed around the cell circumference (15, 16).…”

Section: Discussionmentioning

confidence: 99%

“…Thus, BglG, a transcription factor that positively regulates transcription of the β-glucoside utilization operon ( bgl ) in E. coli , is sequestered near the membrane in an inactive form via interaction with the β-glucoside transporter, BglF (16); in the presence of β-glucosides, BglG is dephosphorylated by BglF and migrates to the cell poles, where it is activated by EI and HPr; consequently, the dimeric form of BglG is released to the cytoplasm, where it binds to the emerging bgl transcript and antiterminates transcription of the bgl operon (15). Similarly, LicT, a BglG homologue from B. subtilis , has recently been shown to be localized near the poles upon addition of β-glucosides to the medium (17). Spatiotemporal control of other transcription regulators by sugar permeases was also documented, i.e., repression of Mlc and MalT activity as positive regulators of glucose and maltose utilization genes in E. coli via interaction and membrane sequestration with the PTS glucose permease (18) and the maltose ABC transporter MalFGK 2 (19), respectively, and activation of MtlR as a positive regulator of mannitol operon expression in B. subtilis via interaction with the mannitol permease (20).…”

Section: Introductionmentioning

confidence: 99%

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The General Phosphotransferase System Proteins Localize to Sites of Strong Negative Curvature in Bacterial Cells

Govindarajan

Elisha

Nevo‐Dinur

et al. 2013

mBio

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The bacterial cell poles are emerging as subdomains where many cellular activities take place, but the mechanisms for polar localization are just beginning to unravel. The general phosphotransferase system (PTS) proteins, enzyme I (EI) and HPr, which control preferential use of carbon sources in bacteria, were recently shown to localize near the Escherichia coli cell poles. Here, we show that EI localization does not depend on known polar constituents, such as anionic lipids or the chemotaxis receptors, and on the cell division machinery, nor can it be explained by nucleoid occlusion or localized translation. Detection of the general PTS proteins at the budding sites of endocytotic-like membrane invaginations in spherical cells and their colocalization with the negative curvature sensor protein DivIVA suggest that geometric cues underlie localization of the PTS system. Notably, the kinetics of glucose uptake by spherical and rod-shaped E. coli cells are comparable, implying that negatively curved “pole-like” sites support not only the localization but also the proper functioning of the PTS system in cells with different shapes. Consistent with the curvature-mediated localization model, we observed the EI protein from Bacillus subtilis at strongly curved sites in both B. subtilis and E. coli. Taken together, we propose that changes in cell architecture correlate with dynamic survival strategies that localize central metabolic systems like the PTS to subcellular domains where they remain active, thus maintaining cell viability and metabolic alertness.

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Section: Discussionsupporting

confidence: 88%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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The General Phosphotransferase System Proteins Localize to Sites of Strong Negative Curvature in Bacterial Cells

Govindarajan

Elisha

Nevo‐Dinur

et al. 2013

mBio

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“…In the absence of a substrate, LicT is phosphorylated in its PRD1 by the PϳEIIB Bgl domain, and the antiterminator is equally distributed in the cell. In the presence of a substrate, LicT is no longer phosphorylated by the PϳEIIB Bgl domain and is located in subpolar regions (173). Although there is no evidence that the presence or absence of EIIB Bgl or PϳEIIB Bgl affects the activity of LicT by direct interaction, phosphorylation of the PRD1 of LicT by PϳEIIB Bgl seems to play an important role in the cellular localization of the antiterminator.…”

Section: Interaction With Phosphorylated Pts Proteinsmentioning

confidence: 98%

The Bacterial Phosphoenolpyruvate:Carbohydrate Phosphotransferase System: Regulation by Protein Phosphorylation and Phosphorylation-Dependent Protein-Protein Interactions

Deutscher

Aké

Derkaoui

et al. 2014

Microbiol Mol Biol Rev

341

374

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SUMMARY The bacterial phosphoenolpyruvate (PEP):carbohydrate phosphotransferase system (PTS) carries out both catalytic and regulatory functions. It catalyzes the transport and phosphorylation of a variety of sugars and sugar derivatives but also carries out numerous regulatory functions related to carbon, nitrogen, and phosphate metabolism, to chemotaxis, to potassium transport, and to the virulence of certain pathogens. For these different regulatory processes, the signal is provided by the phosphorylation state of the PTS components, which varies according to the availability of PTS substrates and the metabolic state of the cell. PEP acts as phosphoryl donor for enzyme I (EI), which, together with HPr and one of several EIIA and EIIB pairs, forms a phosphorylation cascade which allows phosphorylation of the cognate carbohydrate bound to the membrane-spanning EIIC. HPr of firmicutes and numerous proteobacteria is also phosphorylated in an ATP-dependent reaction catalyzed by the bifunctional HPr kinase/phosphorylase. PTS-mediated regulatory mechanisms are based either on direct phosphorylation of the target protein or on phosphorylation-dependent interactions. For regulation by PTS-mediated phosphorylation, the target proteins either acquired a PTS domain by fusing it to their N or C termini or integrated a specific, conserved PTS regulation domain (PRD) or, alternatively, developed their own specific sites for PTS-mediated phosphorylation. Protein-protein interactions can occur with either phosphorylated or unphosphorylated PTS components and can either stimulate or inhibit the function of the target proteins. This large variety of signal transduction mechanisms allows the PTS to regulate numerous proteins and to form a vast regulatory network responding to the phosphorylation state of various PTS components.

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“…Plasmids pCFPbglS and pYFPbglS served as templates for PCR to amplify the fluorophore-encoding cfp and yfp genes, respectively [54]. The plasmid pGP1870 was used for the construction of a gudB-gfp fusion [55] (Table S2). …”

Section: Methodsmentioning

confidence: 99%

Selection-Driven Accumulation of Suppressor Mutants in Bacillus subtilis: The Apparent High Mutation Frequency of the Cryptic gudB Gene and the Rapid Clonal Expansion of gudB+ Suppressors Are Due to Growth under Selection

et al. 2013

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Soil bacteria like Bacillus subtilis can cope with many growth conditions by adjusting gene expression and metabolic pathways. Alternatively, bacteria can spontaneously accumulate beneficial mutations or shape their genomes in response to stress. Recently, it has been observed that a B. subtilis mutant lacking the catabolically active glutamate dehydrogenase (GDH), RocG, mutates the cryptic gudBCR gene at a high frequency. The suppressor mutants express the active GDH GudB, which can fully replace the function of RocG. Interestingly, the cryptic gudBCR allele is stably inherited as long as the bacteria synthesize the functional GDH RocG. Competition experiments revealed that the presence of the cryptic gudBCR allele provides the bacteria with a selective growth advantage when glutamate is scarce. Moreover, the lack of exogenous glutamate is the driving force for the selection of mutants that have inactivated the active gudB gene. In contrast, two functional GDHs are beneficial for the cells when glutamate was available. Thus, the amount of GDH activity strongly affects fitness of the bacteria depending on the availability of exogenous glutamate. At a first glance the high mutation frequency of the cryptic gudBCR allele might be attributed to stress-induced adaptive mutagenesis. However, other loci on the chromosome that could be potentially mutated during growth under the selective pressure that is exerted on a GDH-deficient mutant remained unaffected. Moreover, we show that a GDH-proficient B. subtilis strain has a strong selective growth advantage in a glutamate-dependent manner. Thus, the emergence and rapid clonal expansion of the active gudB allele can be in fact explained by spontaneous mutation and growth under selection without an increase of the mutation rate. Moreover, this study shows that the selective pressure that is exerted on a maladapted bacterium strongly affects the apparent mutation frequency of mutational hot spots.

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Dynamic Localization of a Transcription Factor in Bacillus subtilis: the LicT Antiterminator Relocalizes in Response to Inducer Availability

Cited by 12 publications

References 49 publications

The General Phosphotransferase System Proteins Localize to Sites of Strong Negative Curvature in Bacterial Cells

The General Phosphotransferase System Proteins Localize to Sites of Strong Negative Curvature in Bacterial Cells

The Bacterial Phosphoenolpyruvate:Carbohydrate Phosphotransferase System: Regulation by Protein Phosphorylation and Phosphorylation-Dependent Protein-Protein Interactions

Selection-Driven Accumulation of Suppressor Mutants in Bacillus subtilis: The Apparent High Mutation Frequency of the Cryptic gudB Gene and the Rapid Clonal Expansion of gudB+ Suppressors Are Due to Growth under Selection

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