Sequence analysis of three Bacillus cereus loci carrying PlcR-regulated genes encoding degradative enzymes and enterotoxin The EMBL accession numbers for the sequences reported in this paper are given in Table 1 T1 .

Økstad, Ole Andreas; Gominet, Myriam; Purnelle, Bénédicte; Rose, Matthias; Lereclus, Didier; Kolstø, Anne‐Brit

doi:10.1099/00221287-145-11-3129

Cited by 104 publications

(67 citation statements)

References 51 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…The B. cereus group isolates were widely distributed in a phylogenetic tree constructed by multilocus enzyme electrophoresis analysis (13; E. Helgason, personal communication) and were all found to harbor the bcr1 repeat, while no repeats were identified in the 11 Bacillus strains outside the group (Table 1). This finding suggests that bcr1 may be ubiquitous and specific to members of the B. cereus group of bacteria and could be Table 1 (25,26), bcr1 could be found as a full-length repeat of ϳ155 bp or as shorter versions containing parts of the fulllength sequence. Here, our sequence searches detected 272 partial bcr1 elements (of a minimal defined length of 30 bp) in the three chromosomes altogether, and the ratio of full-length to partial copies was highly divergent among the strains (0. bcr1 chromosomal orientation and localization.…”

Section: Resultsmentioning

confidence: 87%

“…Default values were employed for all other BLASTN parameters. A 141-bp sequence from the bcr1 element bcr1_trp1 (26) was originally used as the seed for the process. However, a comparison of the flanking regions of the sequences obtained after the first BLASTN run revealed that the bcr1 repeat could be redefined as a ϳ160-bp sequence flanked by TTTAT motifs.…”

Section: Methodsmentioning

confidence: 99%

“…Oligonucleotide primers for amplification of bcr1 elements were designed from the bcr1 element bcr1_trp1 (Bc14579_19R [Fig. 4]) located in the upstream region of the transcriptional regulator trp1 in B. cereus ATCC 14579 (26) (left primer, bcr1forBam [5Ј-CCC GGA TCC GGC AGT AAG ACC TCC ACC TC-3Ј]; right primer, bcr1revBam [5Ј-GCG GGA TCC ATA AAG TGA AAC TTT AAT CAG TGG G-3Ј]). Both primers contained BamHI restriction sites at the ends (underlined) to facilitate cloning of PCR products.…”

Section: Methodsmentioning

confidence: 99%

See 2 more Smart Citations

The bcr1 DNA Repeat Element Is Specific to the Bacillus cereus Group and Exhibits Mobile Element Characteristics

et al. 2004

Self Cite

View full text Add to dashboard Cite

Bacillus cereus strains ATCC 10987 and ATCC 14579 harbor a ϳ155-bp repeated element, bcr1, which is conserved in B. cereus, B. anthracis, B. thuringiensis, and B. mycoides but not in B. subtilis and B. licheniformis. In this study, we show by Southern blot hybridizations that bcr1 is present in all 54 B. cereus group strains tested but absent in 11 Bacillus strains outside the group, suggesting that bcr1 may be specific and ubiquitous to the B. cereus group. By comparative analysis of the complete genome sequences of B. cereus ATCC 10987, B. cereus ATCC 14579, and B. anthracis Ames, we show that bcr1 is exclusively present in the chromosome but absent from large plasmids carried by these strains and that the numbers of full-length bcr1 repeats for these strains are 79, 54, and 12, respectively. Numerous copies of partial bcr1 elements are also present in the three genomes (91, 128, and 53, respectively). Furthermore, the genomic localization of bcr1 is not conserved between strains with respect to chromosomal position or organization of gene neighbors, as only six full-length bcr1 loci are common to at least two of the three strains. However, the intergenic sequence surrounding a specific bcr1 repeat in one of the three strains is generally strongly conserved in the other two, even in loci where bcr1 is found exclusively in one strain. This finding indicates that bcr1 either has evolved by differential deletion from a very high number of repeats in a common ancestor to the B. cereus group or is moving around the chromosome. The identification of bcr1 repeats interrupting genes in B. cereus ATCC 10987 and ATCC 14579 and the presence of a flanking TTTAT motif in each end show that bcr1 exhibits features characteristic of a mobile element.

show abstract

Section: Resultsmentioning

confidence: 87%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

See 1 more Smart Citation

The bcr1 DNA Repeat Element Is Specific to the Bacillus cereus Group and Exhibits Mobile Element Characteristics

et al. 2004

Self Cite

View full text Add to dashboard Cite

show abstract

“…The mini-Tn10 transposon conferred resistance to spectinomycin in E. coli (60 g/ml), making it possible to select clones transformed with fragments containing the insertion locus. The chromosomal DNA flanking the insertion locus was sequenced, primarily with primers binding to the extremities of the transposon, and the sequence obtained was extended by chromosome walking, using the chromosome of strain B. thuringiensis 407(Cry Ϫ ), as described in the work of Okstad et al (21). Part of this extended sequence was determined by M. Rose (Institut für Mikrobiologie, J. W. Göethe Universität, Frankfurt, Germany).…”

Section: Methodsmentioning

confidence: 99%

An ABC Transporter from Bacillus thuringiensis Is Essential for β-Exotoxin I Production

et al. 2002

Self Cite

View full text Add to dashboard Cite

␤-Exotoxin I is a nonspecific insecticidal metabolite secreted by some Bacillus thuringiensis strains. Several studies of B. thuringiensis strains that have lost the capacity to produce ␤-exotoxin I have suggested that there is a strong correlation between high levels of ␤-exotoxin I production and the ability to synthesize crystal proteins. In this study, we showed that a mutant strain, B. thuringiensis 407-1(Cry ؊ )(Pig ؉ ), with no crystal gene, produced considerable amounts of ␤-exotoxin I together with a soluble brown melanin pigment. Therefore, ␤-exotoxin I production can take place after a strain has lost the plasmids bearing the cry genes, which suggests that these curable plasmids probably contain determinants involved in the regulation of ␤-exotoxin I production. Using a mini-Tn10 transposon, we constructed a library of strain 407-1(Cry ؊ )(Pig ؉ ) mutants. We screened for nonpigmented mutants with impaired ␤-exotoxin I production and identified a genetic locus harboring two genes (berA and berB) essential for ␤-exotoxin I production. The deduced amino acid sequence of the berA gene displayed significant similarity to the ATP-binding domains of the DRI (drug resistance and immunity) family of ATP-binding cassette (ABC) proteins involved in drug resistance and immunity to bacteriocins and lantibiotics. The berB gene encodes a protein with six putative transmembrane helices, which probably constitutes the integral membrane component of the transporter. The demonstration that berAB is required for ␤-exotoxin I production and/or resistance in B. thuringiensis adds an adenine nucleotide analog to the wide range of substrates of the superfamily of ABC proteins. We suggest that berAB confers ␤-exotoxin I immunity in B. thuringiensis, through active efflux of the molecule.

show abstract

“…Bacteria of the Bacillus cereus phylogenetic group (B. cereus and Bacillus thuringiensis), to which B. anthracis belongs, secrete a diversity of factors that are essential for virulence, including toxins, hemolysins, proteases, and lecithinases. Notably, in these bacteria the secretion of certain virulence factors is regulated by a pleiotropic regulator, PlcR (2,82,87,110), which is inactive in B. anthracis (2). It has been suggested that the evolutionary inactivation of the PlcR regulon in B. anthracis was due to incompatibility with the AtxAcontrolled regulon and reflects the fact that the PlcR target genes are not essential for anthrax pathogenicity (96).…”

mentioning

confidence: 99%

Differential Proteomic Analysis of theBacillus anthracisSecretome: Distinct Plasmid and Chromosome CO₂-Dependent Cross Talk Mechanisms Modulate Extracellular Proteolytic Activities

et al. 2006

View full text Add to dashboard Cite

The secretomes of a virulent Bacillus anthracis strain and of avirulent strains (cured of the virulence plasmids pXO1 and pXO2), cultured in rich and minimal media, were studied by a comparative proteomic approach. More than 400 protein spots, representing the products of 64 genes, were identified, and a unique pattern of protein relative abundance with respect to the presence of the virulence plasmids was revealed. In minimal medium under high CO 2 tension, conditions considered to simulate those encountered in the host, the presence of the plasmids leads to enhanced expression of 12 chromosome-carried genes (10 of which could not be detected in the absence of the plasmids) in addition to expression of 5 pXO1-encoded proteins. Furthermore, under these conditions, the presence of the pXO1 and pXO2 plasmids leads to the repression of 14 chromosomal genes. On the other hand, in minimal aerobic medium not supplemented with CO 2 , the virulent and avirulent B. anthracis strains manifest very similar protein signatures, and most strikingly, two proteins (the metalloproteases InhA1 and NprB, orthologs of gene products attributed to the Bacillus cereus group PlcR regulon) represent over 90% of the total secretome. Interestingly, of the 64 identified gene products, at least 31 harbor features characteristic of virulence determinants (such as toxins, proteases, nucleotidases, sulfatases, transporters, and detoxification factors), 22 of which are differentially regulated in a plasmid-dependent manner. The nature and the expression patterns of proteins in the various secretomes suggest that distinct CO 2 -responsive chromosome-and plasmid-encoded regulatory factors modulate the secretion of potential novel virulence factors, most of which are associated with extracellular proteolytic activities.Bacillus anthracis is a gram-positive spore-forming bacterium that is the etiological agent of anthrax, a lethal disease sporadically affecting humans and animals, in particular herbivores. In its most severe manifestation, B. anthracis infection is initiated by inhalation of spores, which are taken up by alveolar macrophages and germinate into fast-dividing vegetative cells which secrete toxins and virulence factors during growth (81,99). If untreated by prompt antibiotic administration, the bacteria invade the bloodstream, resulting in massive bacteremia and consequently generalized systemic failure and death. B. anthracis is considered to represent a potential biothreat agent, owing to the severity of the anthrax disease, the ease of respiratory contamination, and the perpetual environmental stability of the infective spores. The recent deliberate dissemination of B. anthracis (15) accelerated the efforts to identify new B. anthracis virulence-related determinants for the design of novel diagnostic, preventive, and/or therapeutic strategies.Fully virulent B. anthracis strains harbor two native plasmids, pXO1 and pXO2, which encode critical pathogenicity factors. The absence of either one of the two plasmids results in a pronounce...

show abstract

Sequence analysis of three Bacillus cereus loci carrying PlcR-regulated genes encoding degradative enzymes and enterotoxin The EMBL accession numbers for the sequences reported in this paper are given in Table 1 T1 .

Cited by 104 publications

References 51 publications

The bcr1 DNA Repeat Element Is Specific to the Bacillus cereus Group and Exhibits Mobile Element Characteristics

The bcr1 DNA Repeat Element Is Specific to the Bacillus cereus Group and Exhibits Mobile Element Characteristics

An ABC Transporter from Bacillus thuringiensis Is Essential for β-Exotoxin I Production

Differential Proteomic Analysis of theBacillus anthracisSecretome: Distinct Plasmid and Chromosome CO₂-Dependent Cross Talk Mechanisms Modulate Extracellular Proteolytic Activities

Contact Info

Product

Resources

About

Sequence analysis of three Bacillus cereus loci carrying PlcR-regulated genes encoding degradative enzymes and enterotoxin The EMBL accession numbers for the sequences reported in this paper are given in Table 1 T1 .

Cited by 104 publications

References 51 publications

The bcr1 DNA Repeat Element Is Specific to the Bacillus cereus Group and Exhibits Mobile Element Characteristics

The bcr1 DNA Repeat Element Is Specific to the Bacillus cereus Group and Exhibits Mobile Element Characteristics

An ABC Transporter from Bacillus thuringiensis Is Essential for β-Exotoxin I Production

Differential Proteomic Analysis of theBacillus anthracisSecretome: Distinct Plasmid and Chromosome CO2-Dependent Cross Talk Mechanisms Modulate Extracellular Proteolytic Activities

Contact Info

Product

Resources

About

Differential Proteomic Analysis of theBacillus anthracisSecretome: Distinct Plasmid and Chromosome CO₂-Dependent Cross Talk Mechanisms Modulate Extracellular Proteolytic Activities