Utilization of the rpoB Gene as a Specific Chromosomal Marker for Real-Time PCR Detection of Bacillus anthracis

Abstract: The potential use of Bacillus anthracis as a weapon of mass destruction poses a threat to humans, domesticated animals, and wildlife and necessitates the need for a rapid and highly specific detection assay. We have developed a real-time PCR-based assay for the specific detection of B. anthracis by taking advantage of the unique nucleotide sequence of the B. anthracis rpoB gene. Variable region 1 of the rpoB gene was sequenced from 36 Bacillus strains, including 16 B. anthracis strains and 20 other related bac… Show more

“…Though discrimination of the closely related bacteria of the B. cereus group is possible with assays that utilize PCR [4][5][6], these techniques frequently require laboratory based equipment and skilled technicians. Immunoassays, such as lateral flow assays, offer advantages over PCR-based techniques in their simplicity, portability, and low cost allowing them to readily be deployed to the field.…”

Selection and Characterization of Single Domain Antibodies Specific for Bacillus anthracis Spore Proteins

“…Though discrimination of the closely related bacteria of the B. cereus group is possible with assays that utilize PCR [4][5][6], these techniques frequently require laboratory based equipment and skilled technicians. Immunoassays, such as lateral flow assays, offer advantages over PCR-based techniques in their simplicity, portability, and low cost allowing them to readily be deployed to the field.…”

Selection and Characterization of Single Domain Antibodies Specific for Bacillus anthracis Spore Proteins

“…Several chromosomally derived PCRprimers for identifying B. anthracis have been published, targeted against BA813 (Ramisse et al, 1996), saspB (Hoffmaster et al, 2002), rpoB (Qi et al, 2001), gyrA (Hurtle et al, 2004), a fragment crossing a hypothetical protein and a alpha/betahydrolase encoding genes (Bode et al, 2004) and plcR (Easterday et al, 2005).…”

Genetic distribution of 295 Bacillus cereus group members based on adk-screening in combination with MLST (Multilocus Sequence Typing) used for validating a primer targeting a chromosomal locus in B. anthracis

“…[13][14][15] Finally, a few single nucleotide polymorphisms (SNP) have also been considered for PCR markers. Target genes include rpoB, 24,[48][49][50][51] gyrA, 25,52,53 gyrB, 54,55 plc, 20,23,53,56 purA, 57 and the 16S-23S rDNA internal spacer sequences. [58][59][60] But, so far, only the nonsense mutation in the global regulator PlcR, which controls the transcription of secreted virulence factors in B. cereus and B. thuringiensis, have proved to be truly unique to B. anthracis strains.…”

“…16,20,59 False-positive signals have sometimes been recorded with closely related strains of the B. cereus group using the other published SNPs. 24,49,52,59,[61][62][63] In silico analysis About a hundred sequences corresponding to all primers and probes currently published were compiled and compared using the primer alignment function of the Gegenees software (www. gegenees.org).…”

“…Small alterations in these conditions can result in the loss of specificity, especially with hydrolysis probes, i.e., TaqMan chemistry. 18,[23][24][25] To evaluate the wide range of PCR methods used in laboratories for B. anthracis identification, a computer-based comparative analysis of more than 300 PCR-target sequences reported in the literature was conducted. All sequences were compared against all publicly available Bacillus genomes and sorted for specificity.…”

In silico and in vitro evaluation of PCR-based assays for the detection ofBacillus anthracischromosomal signature sequences