Establishment and evaluation of a new fluorescent probe method based on loop‐mediated isothermal amplification for the detection of Mycobacterium tuberculosis complex

Abstract

AbstractWe aimed to develop a novel diagnostic method called multiplex fluorescence of loop primer upon self‐dequenching loop‐mediated isothermal amplification (mFLOS‐LAMP) for the rapid detection of Mycobacterium tuberculosis complex (MTBC). A set of specific primers was designed to target the detection of IS1081 and IS6110 genes, which are insertion sequences within the MTBC. The 110 sputum specimens collected were assessed using the established mFLOS‐LAMP method, multiplex polymerase chain reaction, Xpert MTB/RIF, and smear microscopy. The optimal reaction temperature and duration for mFLOS‐LAMP were determined to be 65°C and 30 min, respectively, by optimizing the entire system. The detection sensitivity of mFLOS‐LAMP was 6.0 × 101 CFU/mL, by Bacillus Calmette‐Guerin, and the mFLOS‐LAMP sensitivity of M. tuberculosis H37Rv genomic DNA was 500 fg, and the specificity was 100%. The sensitivity of mFLOS‐LAMP was 94.2% and the specificity was 96.6%, when Xpert MTB/RIF was used as the reference method. There was no statistically significant difference in their detection rate (χ2 = 0, P = 1.000), and the consistency was good (kappa = 0.909, P < 0.001). The receiver operating characteristic analysis yielded the maximum area under the curve of 0.954. The mFLOS‐LAMP method demonstrated high sensitivity and specificity, allowing for swift and accurate detection of MTBC.