Amplicon DNA melting analysis for the simultaneous detection of Brucella spp and Mycobacterium tuberculosis complex. Potential use in rapid differential diagnosis between extrapulmonary tuberculosis and focal complications of brucellosis

Rocio Sanjuan-Jimenez; Juan D Colmenero; Pilar Bermúdez; Antonio Alonso; Pilar Morata

doi:10.1371/journal.pone.0058353

Amplicon DNA melting analysis for the simultaneous detection of Brucella spp and Mycobacterium tuberculosis complex. Potential use in rapid differential diagnosis between extrapulmonary tuberculosis and focal complications of brucellosis

PLoS One. 2013;8(3):e58353. doi: 10.1371/journal.pone.0058353. Epub 2013 Mar 8.

Authors

Rocio Sanjuan-Jimenez¹, Juan D Colmenero, Pilar Bermúdez, Antonio Alonso, Pilar Morata

Affiliation

¹ Biochemistry, Molecular Biology and Immunology Department, Faculty of Medicine, University of Malaga, Malaga, Spain.

Abstract

Some sites of extrapulmonary tuberculosis and focal complications of brucellosis are very difficult to differentiate clinically, radiologically, and even histopathologically. Conventional microbiological methods for the diagnosis of extrapulmonary tuberculosis and complicated brucellosis not only lack adequate sensitivity, they are also time consuming, which could lead to an unfavourable prognosis. The aim of this work was to develop a multiplex real-time PCR assay based on SYBR Green I to simultaneously detect Brucella spp and Mycobacterium tuberculosis complex and evaluate the efficacy of the technique with different candidate genes. The IS711, bcsp31 and omp2a genes were used for the identification of Brucella spp and the IS6110, senX3-regX3 and cfp31 genes were targeted for the detection of the M. tuberculosis complex. As a result of the different combinations of primers, nine different reactions were evaluated. A test was defined as positive only when the gene combinations were capable of co-amplifying both pathogens in a single reaction tube and showed distinguishable melting temperatures for each microorganism. According to the melting analysis, only three combinations of amplicons (senX3-regX3+bcsp31, senX3-regX3+IS711 and IS6110+IS711) were visible. Detection limits of senX3-regX3+bcsp31 and senX3-regX3+IS711 were of 2 and 3 genome equivalents for M. tuberculosis complex and Brucella while for IS6110+IS711 they were of 200 and 300 genome equivalents, respectively. The three assays correctly identified all the samples, showing negative results for the control patients. The presence of multicopy elements and GC content were the components most influencing the efficiency of the test; this should be taken into account when designing a multiplex-based SYBR Green I assay. In conclusion, multiplex real time PCR assays based on the targets senX3-regX3+bcsp31 and senX3-regX3+IS711 using SYBR Green I are highly sensitive and reproducible. This may therefore be a practical approach for the rapid differential diagnosis between extrapulmonary tuberculosis and complicated brucellosis.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Brucella / genetics*
Brucellosis / diagnosis*
Brucellosis / genetics
Brucellosis / microbiology
DNA, Bacterial / chemistry*
DNA, Bacterial / isolation & purification
DNA, Bacterial / metabolism
Diagnosis, Differential
Genes, Bacterial*
Humans
Mycobacterium tuberculosis / genetics*
Polymerase Chain Reaction / methods*
Sensitivity and Specificity
Tuberculosis / diagnosis
Tuberculosis / genetics
Tuberculosis / microbiology

Substances

DNA, Bacterial

Grants and funding

This work received financial support from the Consejería de Innovación Ciencia y Empresa (grant CTS-276 and P-08-CTS-3969) both of the Junta de Andalucía (Spain). Rocio Sanjuan-Jimenez is a fellow attached to the project P-08-CTS-3969. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.