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2000
Volume 24, Issue 8
  • ISSN: 1871-5265
  • E-ISSN: 2212-3989

Abstract

Background: The toxin-antitoxin system is a genetic element that is highly present in (MTB), the causative agent of tuberculosis. The toxin-antitoxin system comprises toxin protein and antitoxin protein or non-encoded RNA interacting with each other and inhibiting toxin activity. has more classes of TA loci than non-tubercle bacilli and other microbes, including chaperone system, and hypothetical proteins. Aims: The study aims to demonstrate the genes encoded toxin-antitoxin system in strains from clinical samples. Materials and Methods: The pulmonary and extra-pulmonary tuberculosis clinical samples were collected, and smear microscopy (Ziehl-Neelsen staining) was performed for the detection of high bacilli (3+) count, followed by nucleic acid amplification assay. Bacterial culture and growth assay, genomic DNA extraction, and polymerase chain reaction were also carried out. Results: The positive PTB and EPTB samples were determined by 3+ in microscopy smear and the total count of tubercle bacilli determined by NAAT assay was 8.0×1005in sputum and 1.3×1004CFU/ml in tissue abscess. Moreover, the genomic DNA was extracted from culture, and the amplification of Rv1044 and Rv1045 genes in 624 and 412 base pairs (between 600-700 and 400-500 in ladder), respectively, in the H37Rv and clinical samples was observed. Conclusion: It has been found that Rv1044 and Rv1045 are hypothetical proteins with 624 and 882 base pairs belonging to the family of toxin-antitoxin loci. Moreover, the significant identification of TA-encoded loci genes may allow for the investigation of multidrugresistant and extensively drug-resistant tuberculosis.

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/content/journals/iddt/10.2174/0118715265274164240117104534
2024-12-01
2024-10-09
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