Genome-scale reconstruction of the Lrp regulatory network in
            <i>Escherichia coli</i>

Cho, Byung-Kwan; Barrett, Christian; Knight, Eric M.; Park, Young Seoub; Palsson, Bernhard Ø.

doi:10.1073/pnas.0807227105

Cited by 163 publications

(238 citation statements)

References 29 publications

(34 reference statements)

Supporting

Mentioning

225

Contrasting

Unclassified

Order By: Relevance

“…Likewise, a shift to a lower antibiotic concentration for the ⌬hns and ⌬lrp backgrounds harboring pBAD-tosR-His 6 does not perturb TosR regulation itself; the lower antibiotic concentration did not perturb TosR-mediated regulation in the wild-type E. coli CFT073 background (data not shown). As for H-NS, Lrp is also a global regulator (19,22,(37)(38)(39)(59)(60)(61)(62)(63)(64)(65)(66)(67). Therefore, it remains unclear if additional gene products also supplement Lrp-and TosRmediated positive regulation of the tos operon.…”

Section: Resultsmentioning

confidence: 99%

See 1 more Smart Citation

Regulation of Expression of Uropathogenic Escherichia coli Nonfimbrial Adhesin TosA by PapB Homolog TosR in Conjunction with H-NS and Lrp

Engstrom

Mobley

2016

Infect Immun

View full text Add to dashboard Cite

Urinary tract infections (UTIs) are a major burden to human health. The overwhelming majority of UTIs are caused by uropathogenic Escherichia coli (UPEC) strains. Unlike some pathogens, UPEC strains do not have a fixed core set of virulence and fitness factors but do have a variety of adhesins and regulatory pathways. One such UPEC adhesin is the nonfimbrial adhesin TosA, which mediates adherence to the epithelium of the upper urinary tract. The tos operon is AT rich, resides on pathogenicity island aspV, and is not expressed under laboratory conditions. Because of this, we hypothesized that tosA expression is silenced by H-NS. Lrp, based on its prominent function in the regulation of other adhesins, is also hypothesized to contribute to tos operon regulation. Using a variety of in vitro techniques, we mapped both the tos operon promoter and TosR binding sites. We have now identified TosR as a dual regulator of the tos operon, which could control the tos operon in association with H-NS and Lrp. H-NS is a negative regulator of the tos operon, and Lrp positively regulates the tos operon. Exogenous leucine also inhibits Lrp-mediated tos operon positive regulation. In addition, TosR binds to the pap operon, which encodes another important UPEC adhesin, P fimbria. Induction of TosR synthesis reduces production of P fimbria. These studies advance our knowledge of regulation of adhesin expression associated with uropathogen colonization of a host. U rinary tract infections (UTIs), which are among the most common bacterial infections of humans (1), can occur in otherwise healthy individuals when bacteria colonizing the gastrointestinal tract gain access to the periurethral area. Most individuals with UTIs develop an infection of the bladder, referred to as cystitis (1). However, the infecting bacterium may ascend the ureters to infect the kidneys (pyelonephritis) and, in some cases, enter the bloodstream leading to bacteremia and sometimes fatal urosepsis (1-4).A diverse group of extraintestinal pathogenic Escherichia coli strains, referred to as uropathogenic E. coli (UPEC), cause the overwhelming majority of uncomplicated UTIs (2, 5). While numerous UPEC virulence factors have been identified, including adhesins, motility systems, toxins, and iron acquisition systems, a core set of virulence factors has not been strictly defined (6-8). However, it is critical to understand specific virulence factors and how they are regulated.Previous work identified and characterized the E. coli repeatsin-toxin (RTX) nonfimbrial adhesin TosA (i.e., type one secretion as the predicted secretion mechanism) (7, 9-13). In particular, it was noted that tosA and the other tos operon genes have poor in vitro expression (9-11). TosA, a Ͼ250-kDa surface-exposed protein, mediates UPEC adherence to epithelial cells derived from the upper urinary tract (9). This is in contrast to a number of other RTX proteins, which are fully secreted into the extracellular milieu and act as toxins (14-18). We estimated that ϳ32% of UPEC strains carry genes enc...

show abstract

Section: Resultsmentioning

confidence: 99%

“…The tos operon is localized to the PAI-aspV pathogenicity island in UPEC strain CFT073 (12). It is well accepted that genes on PAIs and other AT-rich sequences are often bound and regulated by nucleoid-structuring proteins, including H-NS and Lrp (41,43,44,67,79). A 400-bp region containing P tos is AT rich (74%).…”

Section: Resultsmentioning

confidence: 99%

Regulation of Expression of Uropathogenic Escherichia coli Nonfimbrial Adhesin TosA by PapB Homolog TosR in Conjunction with H-NS and Lrp

Engstrom

Mobley

2016

Infect Immun

View full text Add to dashboard Cite

show abstract

“…Initial methodological tests reveal that especially a combination of traditional ChIP-onchip and ChIP sequencing yields a more comprehensive list of functional TFBSs throughout genomes (85). Also, combining high-resolution ChIP-on-chip or ChIP-Seq data with gene expression data appears to be promising for the network reconstruction of specific regulons (51). The integration of transcriptomics and metabolomics will finally also reveal more insights into the role of small-molecule concentrations (for example, as small TF binding ligands or in riboswitch regulation) in regulating gene transcription on a global scale (202), which is especially important when integrating experimental data for organisms grown in different media.…”

Section: Conclusion and Future Perspectivesmentioning

confidence: 99%

Mechanisms and Evolution of Control Logic in Prokaryotic Transcriptional Regulation

Hijum

Medema

Kuipers

2009

Microbiol Mol Biol Rev

128

149

View full text Add to dashboard Cite

SUMMARY A major part of organismal complexity and versatility of prokaryotes resides in their ability to fine-tune gene expression to adequately respond to internal and external stimuli. Evolution has been very innovative in creating intricate mechanisms by which different regulatory signals operate and interact at promoters to drive gene expression. The regulation of target gene expression by transcription factors (TFs) is governed by control logic brought about by the interaction of regulators with TF binding sites (TFBSs) in cis-regulatory regions. A factor that in large part determines the strength of the response of a target to a given TF is motif stringency, the extent to which the TFBS fits the optimal TFBS sequence for a given TF. Advances in high-throughput technologies and computational genomics allow reconstruction of transcriptional regulatory networks in silico. To optimize the prediction of transcriptional regulatory networks, i.e., to separate direct regulation from indirect regulation, a thorough understanding of the control logic underlying the regulation of gene expression is required. This review summarizes the state of the art of the elements that determine the functionality of TFBSs by focusing on the molecular biological mechanisms and evolutionary origins of cis-regulatory regions.

show abstract

“…Before microarray hybridization, real-time quantitative PCR targeting previously known binding regions were carried out to verify enrichment of IP DNA fragments. qPCR and amplification of DNA was performed as previously described 8 . Microarray hybridization, wash and scan were performed in accordance with manufacturer's instruction (Roche Nimblegen).…”

Section: Methodsmentioning

confidence: 99%

“…These computational methods, however, do not account for condition-specific binding information, and thus cannot determine the functional state of the network. Therefore, experimental methods, such as chromatin immunoprecipitation coupled to microarray (ChIP-chip) or to sequencing (ChIP-seq), have recently been applied to determine condition-specific binding of s factors to DNA directly 7,8 .…”

mentioning

confidence: 99%

Characterizing the interplay between multiple levels of organization within bacterial sigma factor regulatory networks

et al. 2013

Self Cite

View full text Add to dashboard Cite

Bacteria contain multiple sigma factors, each targeting diverse, but often overlapping sets of promoters, thereby forming a complex network. The layout and deployment of such a sigma factor network directly impacts global transcriptional regulation and ultimately dictates the phenotype. Here we integrate multi-omic data sets to determine the topology, the operational, and functional states of the sigma factor network in Geobacter sulfurreducens, revealing a unique network topology of interacting sigma factors. Analysis of the operational state of the sigma factor network shows a highly modular structure with s N being the major regulator of energy metabolism. Surprisingly, the functional state of the network during the two most divergent growth conditions is nearly static, with sigma factor binding profiles almost invariant to environmental stimuli. This first comprehensive elucidation of the interplay between different levels of the sigma factor network organization is fundamental to characterize transcriptional regulatory mechanisms in bacteria.

show abstract

Genome-scale reconstruction of the Lrp regulatory network in Escherichia coli

Cited by 163 publications

References 29 publications

Regulation of Expression of Uropathogenic Escherichia coli Nonfimbrial Adhesin TosA by PapB Homolog TosR in Conjunction with H-NS and Lrp

Regulation of Expression of Uropathogenic Escherichia coli Nonfimbrial Adhesin TosA by PapB Homolog TosR in Conjunction with H-NS and Lrp

Mechanisms and Evolution of Control Logic in Prokaryotic Transcriptional Regulation

Characterizing the interplay between multiple levels of organization within bacterial sigma factor regulatory networks

Contact Info

Product

Resources

About