Comprehensive Assessment of the Regulons Controlled by the FixLJ-FixK2-FixK1Cascade inBradyrhizobium japonicum

Mesa, Socorro; Hauser, Felix; Friberg, Markus; Malaguti, Emmanuelle; Fischer, Hans‐Martin; Hennecke, Hauke

doi:10.1128/jb.00748-08

Cited by 116 publications

(209 citation statements)

References 67 publications

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“…S1, lanes 1-3). This result was unexpected, because previous studies showed a clear induction of fixK 2 gene expression in response to decreased oxygen concentrations, although a basal level of fixK 2 expression had been noticed even in aerobiosis (16,17,20 H2O2 sensitivity of the B. japonicum WT and the C183A-FixK2-expressing mutant strain 8854. Soft agar (0.9%) plates with PSY medium were inoculated with the indicated B. japonicum strains.…”

Section: Analysis Of the In Vivo Status Of The Fixk2mentioning

confidence: 80%

“…Signal intensity detection, normalization and statistical analysis were done as already established (17,45). Only those probe sets that were called ''present'' or ''marginal'' in Ն67% of the replicates of each experiment were considered for further analysis.…”

mentioning

confidence: 99%

“…Recently, the FixK 2 regulon was unraveled by using a transcriptomics approach (17). Also, DNA binding site predictions together with a FixK 2 -dependent in vitro transcription assay has identified 11 direct target genes or operons for FixK 2 .…”

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confidence: 99%

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Posttranslational control of transcription factor FixK ₂ , a key regulator for the Bradyrhizobium japonicum –soybean symbiosis

Mesa

Reutimann

Fischer

et al. 2009

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

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Rhizobial FixK-like proteins play essential roles in activating genes for endosymbiotic life in legume root nodules, such as genes for micro-oxic respiration. In the facultative soybean symbiont, Bradyrhizobium japonicum, the FixK 2 protein is the key player in a complex regulatory network. The fixK 2 gene itself is activated by the 2-component regulatory system FixLJ in response to a moderate decrease of the oxygen tension, and the FixK 2 protein distributes and amplifies this response to the level of approximately 200 target genes. Unlike other members of the cAMP receptor protein family, to which FixK 2 belongs, the FixK2 protein does not appear to be modulated by small effector molecules. Here, we show that a critical, single cysteine residue (C183) near the DNA-binding domain of FixK 2 confers sensitivity to oxidizing agents and reactive oxygen species. Oxidation-dependent inactivation occurs not only in vitro, as shown with cell-free transcription assays, but also in vivo, as shown by microarray-assisted transcriptome analysis of the FixK 2 regulon. The oxidation mechanism may involve a reversible dimerization by intermolecular disulfide-bridge formation and a direct, irreversible oxidation at the cysteine thiol, depending on the oxidizing agent. Mutational exchange of C183 to alanine renders FixK 2 resistant to oxidation, yet allows full activity, shown again both in vitro and in vivo. We hypothesize that posttranslational modification by reactive oxygen species is a means to counterbalance the cellular pool of active FixK 2, which would otherwise fill unrestrictedly through FixLJ-dependent synthesis.CPR/FNR ͉ gene regulation ͉ nitrogen fixation ͉ nodules ͉ rhizobia T he cAMP receptor protein (CRP)/fumarate-nitrate reductase regulator (FNR) family comprises transcription factors that mainly act as activators in a wide range of bacteria (reviewed in ref. 1). In all cases studied, the active form consists of homodimeric proteins in which each monomer contains an N-terminal sensor domain linked to the C-terminal DNA binding domain via a long ␣-helix that causes dimerization. These regulators control expression of specific sets of genes implicated in a broad spectrum of processes such as oxidative stress response, micro-oxic and anoxic metabolism, carbon catabolism, and stationary phase survival. The response to the respective environmental or intracellular stimuli is usually transduced through an interaction between a signaling molecule and the sensory domain, whereby a conformational change is induced that leads to the binding of the active dimer to operators near the promoters of the target genes (reviewed in ref.2). Three modes of signal perception have been described: (i) direct perception of a stressor, as in the Lactobacillus casei FLP protein (3); (ii) dependency on a prosthetic group such as a [4Fe-4S] 2ϩ cluster or heme in Escherichia coli FNR (4) or Rhodospirillum rubrum CooA (5), respectively; and (iii) binding of a small effector molecule like cAMP for E. coli CRP (6) or 2-oxoglutarate for cyanob...

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Section: Analysis Of the In Vivo Status Of The Fixk2mentioning

confidence: 80%

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confidence: 99%

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Posttranslational control of transcription factor FixK ₂ , a key regulator for the Bradyrhizobium japonicum –soybean symbiosis

Mesa

Reutimann

Fischer

et al. 2009

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

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“…Therefore, if the early increase in phaC2 transcript levels observed in this study results in a later increase in PhaC2 protein levels, this paralog would soon occupy the limited PhaC sites on the granule surface, thus disturbing the access of PhaC1, which might lead to a diminished biosynthetic activity, or it may preclude the access of a PHA depolymerase enzyme. The interplay between PhaC1 and PhaC2 might be relevant in nodules, where phaC2 expression is stimulated 6-fold by FixK2 (a transcription factor enhancer that is stimulated by low O 2 levels) (10). Surprisingly, phaC3, which was poorly expressed in the wild type, was upregulated at logarithmic growth phase in the ⌬phaC2 mutant.…”

Section: Discussionmentioning

confidence: 99%

Analysis of Two Polyhydroxyalkanoate Synthases in Bradyrhizobium japonicum USDA 110

Quelas

Mongiardini

Pérez-Giménez

et al. 2013

Journal of Bacteriology

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bBradyrhizobium japonicum USDA 110 has five polyhydroxyalkanoate (PHA) synthases (PhaC) annotated in its genome: bll4360 (phaC1), bll6073 (phaC2), blr3732 (phaC3), blr2885 (phaC4), and bll4548 (phaC5). All these proteins possess the catalytic triad and conserved amino acid residues of polyester synthases and are distributed into four different PhaC classes. We obtained mutants in each of these paralogs and analyzed phaC gene expression and PHA production in liquid cultures. Despite the genetic redundancy, only phaC1 and phaC2 were expressed at significant rates, while PHA accumulation in stationary-phase cultures was impaired only in the ⌬phaC1 mutant. Meanwhile, the ⌬phaC2 mutant produced more PHA than the wild type under this condition, and surprisingly, the phaC3 transcript increased in the ⌬phaC2 background. A double mutant, the ⌬phaC2 ⌬phaC3 mutant, consistently accumulated less PHA than the ⌬phaC2 mutant. PHA accumulation in nodule bacteroids followed a pattern similar to that seen in liquid cultures, being prevented in the ⌬phaC1 mutant and increased in the ⌬phaC2 mutant in relation to the level in the wild type. Therefore, we used these mutants, together with a ⌬phaC1 ⌬phaC2 double mutant, to study the B. japonicum PHA requirements for survival, competition for nodulation, and plant growth promotion. All mutants, as well as the wild type, survived for 60 days in a carbon-free medium, regardless of their initial PHA contents. When competing for nodulation against the wild type in a 1:1 proportion, the ⌬phaC1 and ⌬phaC1 ⌬phaC2 mutants occupied only 13 to 15% of the nodules, while the ⌬phaC2 mutant occupied 81%, suggesting that the PHA polymer is required for successful competitiveness. However, the bacteroid content of PHA did not affect the shoot dry weight accumulation.

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“…Escherichia coli strains grew in LB medium (18) at 37°C with the following antibiotics, added at the indicated final concentrations: ampicillin at 200 g/ml in solid medium and 100 g/ml in liquid medium, gentamicin at 10 g/ml, hygromycin B at 200 g/ml, kanamycin at 30 g/ml, streptomycin at 50 g/ml, and tetracycline at 10 g/ml. We cultivated B. diazoefficiens strains at 30°C in PSY medium (19) supplemented with 0.1% L-(ϩ)-arabinose and the following antibiotics at the indicated concentrations: chloramphenicol at 20 g/ml (for counterselection of E. coli), hygromycin B at 200 g/ml, kanamycin at 100 g/ml, spectinomycin at 100 g/ml, and tetracycline at 50 g/ml (solid medium) and 25 g/ml (liquid medium). Rhodopseudomonas palustris strains grew at 30°C in modified YPMS medium (20) (which has the same trace elements that exist in PSY medium) containing gentamicin where appropriate (800 g/ml for initial selection and 400 g/ml for routine cultures).…”

Section: Methodsmentioning

confidence: 99%

Versatile Vectors for Efficient Mutagenesis of Bradyrhizobium diazoefficiens and Other Alphaproteobacteria

Ledermann

Strebel

Kampik

et al. 2016

Appl Environ Microbiol

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Analysis of bacterial gene function commonly relies on gene disruption or replacement followed by phenotypic characterization of the resulting mutant strains. Deletion or replacement of targeted regions is commonly achieved via two homologous recombination (HR) events between the bacterial genome and a nonreplicating plasmid carrying DNA fragments flanking the region to be deleted. The counterselection of clones that have integrated the entire plasmid in their genome via a single HR event is crucial in this procedure. Various genetic tools and well-established protocols are available for this type of mutagenesis in model bacteria; however, these methods are not always efficiently applicable in less established systems. Here we describe the construction and application of versatile plasmid vectors pREDSIX and pTETSIX for marker replacement and markerless mutagenesis, respectively. Apart from an array of restriction sites optimized for cloning of GC-rich DNA fragments, the vector backbone contains a constitutively expressed gene for mCherry, enabling the rapid identification of clones originating from single or double HR events by fluorescence-assisted cell sorting (FACS). In parallel, we constructed a series of plasmids from which gene cassettes providing resistance against gentamicin, kanamycin, hygromycin B, streptomycin and spectinomycin, or tetracycline were excised for use with pREDSIX-based marker replacement mutagenesis. In proof-of-concept mutagenesis experiments, we demonstrated the potential for the use of the developed tools for gene deletion mutagenesis in the nitrogen-fixing soybean symbiont Bradyrhizobium diazoefficiens (formerly Bradyrhizobium japonicum) and three additional members of the alphaproteobacteria. IMPORTANCEMutation and phenotypic analysis are essential to the study of gene function. Efficient mutagenesis protocols and tools are available for many bacterial species, including various model organisms; however, genetic analysis of less-well-characterized organisms is often impaired by the lack of efficient methods. Here we describe a set of novel genetic tools for facilitated mutagenesis of the nitrogen-fixing soybean symbiont Bradyrhizobium diazoefficiens and related alphaproteobacteria. We demonstrated their usefulness by generating several mutant strains lacking defined genes. Isolation of both antibiotic resistance gene-containing and markerless deletion mutants is greatly facilitated because undesired clones which contain the entire mutagenic plasmid integrated in the genome can be identified on the basis of their fluorescent phenotype derived from the mCherry gene carried by the vector backbone. The possibility to generate markerless mutants assists with the isolation of strains carrying multiple deletions, which can be crucial while studying functionally redundant genes. Many functional studies of biological phenomena rely on the isolation of mutants and the availability of the respective genetic tools. Mutants are preferably constructed in a targeted manner, which traditi...

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Comprehensive Assessment of the Regulons Controlled by the FixLJ-FixK₂-FixK₁Cascade inBradyrhizobium japonicum

Cited by 116 publications

References 67 publications

Posttranslational control of transcription factor FixK ₂ , a key regulator for the Bradyrhizobium japonicum –soybean symbiosis

Posttranslational control of transcription factor FixK ₂ , a key regulator for the Bradyrhizobium japonicum –soybean symbiosis

Analysis of Two Polyhydroxyalkanoate Synthases in Bradyrhizobium japonicum USDA 110

Versatile Vectors for Efficient Mutagenesis of Bradyrhizobium diazoefficiens and Other Alphaproteobacteria

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Comprehensive Assessment of the Regulons Controlled by the FixLJ-FixK2-FixK1Cascade inBradyrhizobium japonicum

Cited by 116 publications

References 67 publications

Posttranslational control of transcription factor FixK 2 , a key regulator for the Bradyrhizobium japonicum –soybean symbiosis

Posttranslational control of transcription factor FixK 2 , a key regulator for the Bradyrhizobium japonicum –soybean symbiosis

Analysis of Two Polyhydroxyalkanoate Synthases in Bradyrhizobium japonicum USDA 110

Versatile Vectors for Efficient Mutagenesis of Bradyrhizobium diazoefficiens and Other Alphaproteobacteria

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Comprehensive Assessment of the Regulons Controlled by the FixLJ-FixK₂-FixK₁Cascade inBradyrhizobium japonicum

Posttranslational control of transcription factor FixK ₂ , a key regulator for the Bradyrhizobium japonicum –soybean symbiosis

Posttranslational control of transcription factor FixK ₂ , a key regulator for the Bradyrhizobium japonicum –soybean symbiosis