| Literature DB >> 33493196 |
Thoko Flav Kapalamula1, Jeewan Thapa1, Mwangala Lonah Akapelwa1, Kyoko Hayashida2,3, Stephen V Gordon3,4, Bernard Mudenda Hang' Ombe5,6, Musso Munyeme5,6, Eddie Samuneti Solo7, Precious Bwalya1,7, Mirriam Ethel Nyenje8, Aki Tamaru9, Yasuhiko Suzuki1,3, Chie Nakajima1,3.
Abstract
Bovine tuberculosis (TB) caused by Mycobacterium bovis is a significant health threat to cattle and a zoonotic threat for humans in many developing countries. Rapid and accurate detection of M. bovis is fundamental for controlling the disease in animals and humans, and for the proper treatment of patients as one of the first-line anti-TB drug, pyrazinamide, is ineffective against M. bovis. Currently, there are no rapid, simplified and low-cost diagnostic methods that can be easily integrated for use in many developing countries. Here, we report the development of a loop-mediated isothermal amplification (LAMP) assay for specific identification of M. bovis by targeting the region of difference 4 (RD4), a 12.7 kb genomic region that is deleted solely in M. bovis. The assay's specificity was evaluated using 139 isolates comprising 65 M. bovis isolates, 40 M. tuberculosis isolates, seven M. tuberculosis complex reference strains, 22 non-tuberculous mycobacteria and five other bacteria. The established LAMP detected only M. bovis isolates as positive and no false positives were observed using the other mycobacteria and non-mycobacteria tested. Our LAMP assay detected as low as 10 copies of M. bovis genomic DNA within 40 minutes. The procedure of LAMP is simple with an incubation at a constant temperature. Results are observed with the naked eye by a color change, and there is no need for expensive equipment. The established LAMP can be used for the detection of M. bovis infections in cattle and humans in resource-limited areas.Entities:
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Year: 2021 PMID: 33493196 PMCID: PMC7833227 DOI: 10.1371/journal.pntd.0008996
Source DB: PubMed Journal: PLoS Negl Trop Dis ISSN: 1935-2727