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Evaluating the Efficiency of Taqman Real-Time Pcr and Serological Methods in the Detection of Brucella Spp. in Clinical Specimens Collected From Suspected Patients in Ardabil, Iran Publisher Pubmed



Sabour S1 ; Arzanlou M1 ; Jeddi F2 ; Azimi T3, 4 ; Hosseiniasl S5 ; Naghizadehbaghi A6 ; Peeri Dogaheh H1
Authors
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Authors Affiliations
  1. 1. Department of Microbiology, School of Medicine, Ardabil University of Medical Science, Ardabil, Iran
  2. 2. Department of Genetics and pathology, School of Medicine, Ardabil University of Medical Sciences, Ardabil, Iran
  3. 3. Pediatric Infections Research Center, Shahid Beheshti University of Medical Sciences, Tehran, Iran
  4. 4. Department of Pathobiology, School of Public Health, Tehran University of Medical Sciences, Tehran, Iran
  5. 5. Molecular-Genetic Laboratory, Imam Khomeini Hospital, Ardabil University of Medical Sciences, Ardabil, Iran
  6. 6. Department of Physical Education and Sport Sciences, Faculty of Educational Sciences and Psychology, University of Mohaghegh Ardabili. Ardabil, Iran

Source: Journal of Microbiological Methods Published:2020


Abstract

Background: This study aims to evaluate the efficiency of the TaqMan real-time PCR and serological methods in detecting Brucella spp. in clinical specimens that have been collected from suspected patients in Ardabil, Iran. Methods: In this cross-sectional study, a total of 113 consecutive patients suspected of brucellosis who were referred to the three hospitals in Ardabil province were selected. In the first step, the diagnosis of brucellosis was performed by serological methods including the Rose Bengal slide agglutination test, Wright test, 2-ME test, and BrucellaCapt test. In the next step, TaqMan real-time PCR with primer and probe targeting the bcsp31 gene was used for the detection of Brucella spp. Specificity, sensitivity, and positive and negative predictive values of the TaqMan real-time PCR assay were calculated. Results: Among 113 suspected patients with different clinical manifestations, the Rose Bengal slide agglutination test, Wright test, and 2-ME test were positive in 60 cases; however, the BrucellaCapt test titer was 1:160 for one patient. Six patients had high initial serum antibody titers; 2-ME titers of ≥1:640; STA titers of ≥1:1280; BrucellaCapt titers of ≥ 1:2560. Among positive cases, no correlation was observed among gender, age, and life (residence) in urban or rural areas. The TaqMan real-time PCR was positive in 35% of all 60 positive cases. The comparison of the results of the BrucellaCapt and TaqMan real-time PCR methods revealed that 19 out of 54 (35.2%) and 2 out of 6 (33.4%) BrucellaCapt positive cases with titers of >1:320 and ≤ 1:320 were positive, respectively. The sensitivities and specificities of the TaqMan real-time PCR assay were 49.1% and 100% respectively. Conclusion: The sensitivity of the TaqMan real-time PCR assay was low in the diagnosis of brucellosis, while the BrucellaCapt test turned out to be a very valuable, sensitive, and specific test for the diagnosis of brucellosis in suspected patients and, thus, can provide reliable results in medical laboratories. © 2020 Elsevier B.V.