Mechanism for iron-regulated transcription of the Escherichia coli cir gene: metal-dependent binding of fur protein to the promoters

Griggs, David W.; Konisky, J

doi:10.1128/jb.171.2.1048-1054.1989

Cited by 106 publications

(112 citation statements)

References 34 publications

(48 reference statements)

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“…A 21-bp Neisseria consensus that shares Ϸ80% homology to the E. coli consensus has been derived and proposed to be the binding sequence of the Neisseria Fur protein (23). Although the 19-and 21-bp consensuses serve as good indicators to identify a Furregulated gene, the Fur-binding sequence identified in the promoters of several Fur-regulated genes differed from the classical Fur-binding sequence (37)(38)(39)(40)(41)(42). In light of these results, the Fur-binding sequence has been reinterpreted to be a combination of three repeats of 6-bp 5Ј-NAT(A͞T)AT-3Ј rather than a 19-bp palindrome (24).…”

Section: Discussionmentioning

confidence: 99%

Identification of iron-activated and -repressed Fur-dependent genes by transcriptome analysis ofNeisseria meningitidisgroup B

Grifantini

Sebastian

Frigimelica

et al. 2003

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

180

203

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Iron is limiting in the human host, and bacterial pathogens respond to this environment by activating genes required for bacterial virulence. Transcriptional regulation in response to iron in Gramnegative bacteria is largely mediated by the ferric uptake regulator protein Fur, which in the presence of iron binds to a specific sequence in the promoter regions of genes under its control and acts as a repressor. Here we describe DNA microarray, computational and in vitro studies to define the Fur regulon in the human pathogen Neisseria meningitidis group B (strain MC58). After iron addition to an iron-depleted bacterial culture, 153 genes were up-regulated and 80 were down-regulated. Only 50% of the iron-regulated genes were found to contain Fur-binding consensus sequences in their promoter regions. Forty-two promoter regions were amplified and 32 of these were shown to bind Fur by gel-shift analysis. Among these genes, many of which had never been described before to be Fur-regulated, 10 were up-regulated on iron addition, demonstrating that Fur can also act as a transcriptional activator. Sequence alignment of the Fur-binding regions revealed that the N. meningitidis Fur-box encompasses the highly conserved (NATWAT)3 motif. Cluster analysis was effective in predicting Fur-regulated genes even if computer prediction failed to identify Fur-box-like sequences in their promoter regions. Microarray-generated gene expression profiling appears to be a very effective approach to define new regulons and regulatory pathways in pathogenic bacteria.

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Section: Discussionmentioning

confidence: 99%

Identification of iron-activated and -repressed Fur-dependent genes by transcriptome analysis ofNeisseria meningitidisgroup B

Grifantini

Sebastian

Frigimelica

et al. 2003

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

180

203

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“…The promoter of the operon responsible for the biosynthesis of the aerobactin siderophore (referred hereafter as Paer) is particularly interesting in this respect (26,32,33,34). Unlike other promoters controlled by Fur in which the operator involves a clear-cut target sequence (13,24,(27)(28)(29), Paer is bound by the repressor to three distinct extents depending on the concentration of the protein ( Fig. 1 and see below).…”

mentioning

confidence: 99%

Evidence of an Unusually Long Operator for the Fur Repressor in the Aerobactin Promoter of Escherichia coli

Escolar¹,

Pérez-Martı́n

Lorenzo

2000

Journal of Biological Chemistry

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Production of the siderophore aerobactin in Escherichia coli is transcriptionally metalloregulated through the iron-dependent binding of the Fur (ferric uptake regulator) to a large region (>100 base pairs) within the cognate promoter in the pColV-K30 plasmid. We show in this article that such an unusually long operator results from the specific addition of degenerate repeats 5-NAT(A/T)AT-3 and not from a fortuitous occupation of the DNA adjacent to the primary binding sites by an excess of the repressor. Furthermore, the protection pattern revealed by DNase I and hydroxyl radical footprinting reflected a side-by-side oligomerization of the protein along an extended DNA stretch. This type of DNA-protein interactions is more like those observed in some eukaryotic factors and nucleoid-associated proteins than typical of specific prokaryotic regulators.

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“…With concentrations of 1, 10, and 25 mM of Desferal, no reduction of growth was observed ( Figure 9A). This observed lack of effect was unusual since other bacteria like E. coli cease to grow in complex media in the presence of 100 µM Desferal (Griggs and Konisky, 1989). Similarly, no inhibition of growth was observed with dipyridyl at concentrations of 0.1 to 1 mM ( Figure 9B).…”

mentioning

confidence: 89%

“…The highest mRNA expression was observed in stationary phase cells; therefore, metalloregulation of secA-sod message was investigated in B. burgdorferi cells grown to stationary phase. Obviously, Fe was the first candidate to be tested because of the well-documented Fur regulation of sod genes (Griggs and Konisky, 1989;Neiderhoffer et al, 1990;Stojiljkovic et al, 1994;Zheng et al, 1999).…”

Section: Discussionmentioning

confidence: 99%

“…Iron uptake is regulated in Gram-negative bacteria by the repressor protein Fur (Bsat and Helmann, 1999;Griggs and Konisky, 1989;Stojiljkovic et al, 1994;Zheng et al, 1999 (Frechon and Cam, 1994;Ochsner et al, 1995). Analysis of such regions yielded a Fur-binding consensus sequence or "Fur box," which consisted of a 19-bp palindromic sequence, GATAATGATAATCATTATC.…”

Section: F Metalloregulation Of Oxidative Stressmentioning

confidence: 99%

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Characterization of secA-sod operon in Borrellia burgdorferi.

Nichols¹

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Borrelia burgdorferi, the causative agent of Lyme disease, has been characterized as a microaerophilic spirochete. O2 consumption and utilization potentially yield reactive oxygen intermediates, such as superoxide, hydroxyl radicals, and hydrogen peroxide. This study investigated the expression of the sod gene, which encodes the only, identified oxidative defense mechanism in B. burgdorferi. Using primer extension analysis and RT-PCR, it was found that sod and secA are organized as a single transcriptional unit under the control of σ 70 -like promoter upstream of the secA open reading frame. Generally, gene expression decreases with increased distance from the promoter; however, secA expression was observed to be relatively lower amounts than sod. Both genes were expressed in all phases of growth, with greatest expression observed in stationary phase. Because transcription of most sod genes is tightly regulated by iron concentration, the secA-sod gene expression was analyzed in borrelial cells grown in varying amounts of metal. Ironrestriction did not significantly affect growth nor did it affect transcription of secA or sod.Likewise, no major differences in transcription were observed with restricting or supplementing media with manganese. To test the possibility that the borrelial SOD may function with either iron or manganese as a cofactor as in cambialistic SODs, SOD activity was assayed and the highest activity was observed in increased manganese concentrations.Protein expression profiles of Sh-2-82 cultured in metal-defined media were investigated by one-and two-dimensional gel electrophoresis. Approximately 15 proteins were differentially expressed in response to metal concentration. iv ACKNOWLEDGMENTS

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Mechanism for iron-regulated transcription of the Escherichia coli cir gene: metal-dependent binding of fur protein to the promoters

Cited by 106 publications

References 34 publications

Identification of iron-activated and -repressed Fur-dependent genes by transcriptome analysis ofNeisseria meningitidisgroup B

Identification of iron-activated and -repressed Fur-dependent genes by transcriptome analysis ofNeisseria meningitidisgroup B

Evidence of an Unusually Long Operator for the Fur Repressor in the Aerobactin Promoter of Escherichia coli

Characterization of secA-sod operon in Borrellia burgdorferi.

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