Ribosomal RNA Sequence Analysis of Brucella Infection Misidentified as Ochrobactrum anthropi Infection

Horvat, Rebecca T.; Atrouni, Wissam El; Hammoud, Kassem; Hawkinson, Dana; Cowden, Scott

doi:10.1128/jcm.01131-10

Cited by 36 publications

(33 citation statements)

References 37 publications

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“…Despite the publication of laboratory safety measures (15,16) and postexposure recommendations (17), laboratory exposures and laboratory-acquired brucellosis (LAB) cases continue to occur (18,19). In the United States, roughly 120 cases of brucellosis are reported annually.…”

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A Literature Review of Laboratory-Acquired Brucellosis

et al. 2013

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bBrucellosis is a bacterial zoonotic disease which has been associated with laboratory-acquired infections. No recent reviews have addressed the characteristics of laboratory-acquired brucellosis (LAB). English-language literature was reviewed to identify reports of laboratory exposures to Brucella spp. and LAB cases between 1982 and 2007. Evaluation of 28 case reports identified 167 potentially exposed laboratory workers, of whom 71 had LAB. Nine reports were identified that summarized an additional 186 cases of LAB. Only 18 (11%) exposures were due to laboratory accidents, 147 (88%) exposures were due to aerosolization of organisms during routine identification activities, and the circumstances of 2 (1%) exposures were unknown. Brucella melitensis was the causative agent in 80% (135/167) of the exposures. Workers with high-risk exposures were 9.3 times more likely to develop LAB than workers with low-risk exposures (95% confidence interval [CI], 3.0 to 38.6; P < 0.0001); they were also 0.009 times likelier to develop LAB if they took antimicrobial PEP than if they did not (95% CI, 0 to 0.042; P < 0.0001). The median incubation period in case and summary reports was 8 weeks (range 1 to 40 weeks). Antimicrobial PEP is effective in preventing LAB. The incubation period may be used to identify appropriate serological and symptom surveillance time frames for exposed laboratory workers.

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confidence: 99%

A Literature Review of Laboratory-Acquired Brucellosis

et al. 2013

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“…e read with interest the paper "Ribosomal RNA Sequence Analysis of Brucella Infection Misidentified as Ochrobactrum anthropi Infection" by Horvat and colleagues (1). The paper reported that a Brucella isolate was misidentified as Ochrobactrum anthropi.…”

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Mistaken Identity of Brucella Infection

et al. 2013

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We read with interest the paper "Ribosomal RNA Sequence Analysis of Brucella Infection Misidentified as Ochrobactrum anthropi Infection" by Horvat and colleagues (1). The paper reported that a Brucella isolate was misidentified as Ochrobactrum anthropi. The 16S rRNA results indicated that the isolates were Brucella species, with 100% agreement to rRNA sequences of known brucellae and low homology to Ochrobactrum anthropi sequences.Our laboratory has encountered such circumstances three times since December 2011. Strains were isolated from blood cultures of two patients suffering from fever without apparent cause and from a bone marrow culture of a patient with a left tibial lesion. They were initially identified as Bordetella bronchiseptica (1 case) and Ochrobactrum anthropi (2 cases) through the Vitek 2 Compact microbial identification system and Gram-negative (GN) identification card. As the first case (misidentified as Bordetella bronchiseptica) had brucellosis symptoms of splenomegaly, mildly elevated transaminase, typical undulant fever, and a significantly elevated lymphocyte level in his white blood cell count, 16S rRNA PCR amplification and sequencing were performed and results were analyzed using GenBank (accession numbers ACBJ01000075.1, ACEM01000005.1, NC_013118.1, and NC_009668.1). The results indicated that the highest level of identity was to Brucella abortus, Brucella melitensis, and Brucella microti among the Brucella spp., as well as Ochrobactrum anthropi ATCC 49188 (query coverage, 100%; maximum identity, 99%). However, Ochrobactrum anthropi could be excluded based on a negative result observed in the semisolid-medium motility test and flagellar staining. The results suggest that the automated microbial identification system is unreliable, so two preserved strains identified as Ochrobactrum anthropi by the Vitek test were subcultured and reevaluated. 16S rRNA PCR amplification, sequencing, and alignment were performed. The results were similar to those for the first strain; i.e., highest identity was to several isolates within the Brucella spp. and Ochrobactrum anthropi. Here again, Ochrobactrum anthropi was excluded based on a negative result from the semisolid-medium motility test and flagellar staining. We also performed the test which utilized real-time PCR followed by high-resolution melting (HRM) curve analysis to identify the Brucella strains. They were identified as Brucella melitensis. All three strains were confirmed as Brucella melitensis by the China CDC, and the patients' sera were positive for Brucella antibody using the Brucella microagglutination test. These three stains were serotyped as biovar type I.Brucella is a potential agent of bioterrorism and also a significant pathogen causing laboratory-acquired infections (2, 3). However, misidentification of Brucella species by some commercial bacterial identification systems has been previously reported (4, 5). Because of these recurring misidentifications, more and more laboratories are now relying on molecular methods to identify...

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“…Sequencing of the 16S rRNA gene, which is in widespread use for bacterial identification, can be misleading and Brucella organisms cannot be accurately distinguished from the closely related α-protobacterial Ochrobacterium species [72]. A novel recA gene-based, multi-primer, single-target PCR assay has been recently developed and succeeded in differentiating between brucellae and Ochrobacterium anthropi and O. intermedium [73], although the test has a more prolonged turnaround time and is more expensive than the FISH test.…”

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confidence: 99%

Blood Cultures for the Diagnosis of Human Brucellosis

Yagupsky¹

2015

Updates on Brucellosis

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Brucellosis represents a serious health threat to human populations living in areas endemic for the disease. The clinical manifestations of brucellosis are protean and nonspecific, and laboratory confirmation of the diagnosis is crucial for an adequate management of the patient and implementation of infection control measures aimed to control the disease in affected herds. Although brucellosis can be confirmed by serologic tests and nucleic acid amplification assays, culture detection of circulating Brucella organisms remains a diagnostic cornerstone. Traditionally, prolonged incubation of media and performance of blind subcultures of negative blood culture vials have been recommended to maximize isolation of the organism. In recent years, modern automated blood culture systems have revolutionized the diagnosis of human brucellosis by improving sensitivity and enabling detection of brucellae within the routine one-week incubation protocol followed in most Clinical Microbiology laboratories. Development of molecular techniques and mass-spectrometry technology have also shortened the time needed to identify members of the genus, whereas use of biological safety cabinets considerably reduce the risks of contagion to laboratory personnel.

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Ribosomal RNA Sequence Analysis of Brucella Infection Misidentified as Ochrobactrum anthropi Infection

Cited by 36 publications

References 37 publications

A Literature Review of Laboratory-Acquired Brucellosis

A Literature Review of Laboratory-Acquired Brucellosis

Mistaken Identity of Brucella Infection

Blood Cultures for the Diagnosis of Human Brucellosis

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