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A mass-screening protocol for the diagnosis of anthrax from nasal swabs based on an enrichment step in liquid medium was devised. Incubation for growth was performed in autoclavable vials and racks which allow real-time PCR analysis of sterilized cultures. A dual-color PCR was set up with primers and probes for the chromosomal marker rpoB and the plasmid marker lef. Specific primer and probe sets were designed for the differentiation of Bacillus anthracis from B. cereus and for the differentiation of the Sterne vaccine strain from field isolates and the Ames strain, which was used in the recent anthrax bioterrorist attack. The present protocol thus combines the high specificity and sensitivity of real-time PCR with excellent biosafety and the low hands-on time necessary for the processing of large numbers of samples, which is extremely important during control programs involving the processing of large numbers of samples.

Protocol for real-time PCR identification of anthrax spores from nasal swabs after broth enrichment / Oggioni, Mr; Meacci, F; Carattoli, A; Ciervo, A; Orru, G; Cassone, A; Pozzi, G.. - In: JOURNAL OF CLINICAL MICROBIOLOGY. - ISSN 1098-660X. - 40:11(2002), pp. 3956-3963. [10.1128/JCM.40.11.3956-3963.2002]

Protocol for real-time PCR identification of anthrax spores from nasal swabs after broth enrichment

Carattoli A;
2002

Abstract

A mass-screening protocol for the diagnosis of anthrax from nasal swabs based on an enrichment step in liquid medium was devised. Incubation for growth was performed in autoclavable vials and racks which allow real-time PCR analysis of sterilized cultures. A dual-color PCR was set up with primers and probes for the chromosomal marker rpoB and the plasmid marker lef. Specific primer and probe sets were designed for the differentiation of Bacillus anthracis from B. cereus and for the differentiation of the Sterne vaccine strain from field isolates and the Ames strain, which was used in the recent anthrax bioterrorist attack. The present protocol thus combines the high specificity and sensitivity of real-time PCR with excellent biosafety and the low hands-on time necessary for the processing of large numbers of samples, which is extremely important during control programs involving the processing of large numbers of samples.
2002
primer DNA, anthrax; article; Bacillus anthracis; Bacillus cereus; bacterial strain; bacterium culture; bacterium identification; biological warfare; biosafety; chromosome marker; color; culture medium; diagnostic accuracy; diagnostic value; human; Italy; mass screening; nonhuman; nose smear; nucleotide sequence; polymerase chain reaction; priority journal; sensitivity and specificity; time, Anthrax; Bacillus anthracis; Bacterial Typing Techniques; Bioterrorism; Culture Media; Humans; Italy; Mass Screening; Nasal Mucosa; Polymerase Chain Reaction; Sensitivity and Specificity; Specimen Handling; Spores, Bacterial, Anthrax; Bacillus anthracis; Bacillus cereus; Bacteria (microorganisms); Posibacteria
01 Pubblicazione su rivista::01a Articolo in rivista
Protocol for real-time PCR identification of anthrax spores from nasal swabs after broth enrichment / Oggioni, Mr; Meacci, F; Carattoli, A; Ciervo, A; Orru, G; Cassone, A; Pozzi, G.. - In: JOURNAL OF CLINICAL MICROBIOLOGY. - ISSN 1098-660X. - 40:11(2002), pp. 3956-3963. [10.1128/JCM.40.11.3956-3963.2002]
01a Articolo in rivista
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11573/1284887
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