TY - JOUR KW - Animals KW - Calibration KW - DNA, Bacterial KW - DNA, Ribosomal KW - Escherichia coli KW - Hindlimb KW - Mice KW - Mice, Nude KW - Mycobacterium leprae KW - polymerase chain reaction KW - RNA, Ribosomal, 16S KW - Staphylococcus epidermidis KW - Streptococcus pyogenes AU - Truman RW AU - Andrews KP AU - Robbins N AU - Adams LW AU - Krahenbuhl JL AU - Gillis T AB -

Mycobacterium leprae is not cultivable in axenic media, and direct microscopic enumeration of the bacilli is complex, labor intensive, and suffers from limited sensitivity and specificity. We have developed a real-time PCR assay for quantifying M. leprae DNA in biological samples. Primers were identified to amplify a shared region of the multicopy repeat sequence (RLEP) specific to M. leprae and tested for sensitivity and specificity in the TaqMan format. The assay was specific for M. leprae and able to detect 10 fg of purified M. leprae DNA, or approximately 300 bacteria in infected tissues. We used the RLEP TaqMan PCR to assess the short and long-term growth results of M. leprae in foot pad tissues obtained from conventional mice, a gene knock-out mouse strain, athymic nude mice, as well as from reticuloendothelial tissues of M. leprae-infected nine-banded armadillos. We found excellent correlative results between estimates from RLEP TaqMan PCR and direct microscopic counting (combined r = 0.98). The RLEP TaqMan PCR permitted rapid analysis of batch samples with high reproducibility and is especially valuable for detection of low numbers of bacilli. Molecular enumeration is a rapid, objective and highly reproducible means to estimate the numbers of M. leprae in tissues, and application of the technique can facilitate work with this agent in many laboratories.

BT - PLoS neglected tropical diseases C1 - http://www.ncbi.nlm.nih.gov/pubmed/18982056?dopt=Abstract CN - TRUMAN 2008 DA - 2008 DO - 10.1371/journal.pntd.0000328 IS - 11 J2 - PLoS Negl Trop Dis LA - eng N2 -

Mycobacterium leprae is not cultivable in axenic media, and direct microscopic enumeration of the bacilli is complex, labor intensive, and suffers from limited sensitivity and specificity. We have developed a real-time PCR assay for quantifying M. leprae DNA in biological samples. Primers were identified to amplify a shared region of the multicopy repeat sequence (RLEP) specific to M. leprae and tested for sensitivity and specificity in the TaqMan format. The assay was specific for M. leprae and able to detect 10 fg of purified M. leprae DNA, or approximately 300 bacteria in infected tissues. We used the RLEP TaqMan PCR to assess the short and long-term growth results of M. leprae in foot pad tissues obtained from conventional mice, a gene knock-out mouse strain, athymic nude mice, as well as from reticuloendothelial tissues of M. leprae-infected nine-banded armadillos. We found excellent correlative results between estimates from RLEP TaqMan PCR and direct microscopic counting (combined r = 0.98). The RLEP TaqMan PCR permitted rapid analysis of batch samples with high reproducibility and is especially valuable for detection of low numbers of bacilli. Molecular enumeration is a rapid, objective and highly reproducible means to estimate the numbers of M. leprae in tissues, and application of the technique can facilitate work with this agent in many laboratories.

PY - 2008 EP - e328 T2 - PLoS neglected tropical diseases TI - Enumeration of Mycobacterium leprae using real-time PCR. UR - http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2570796/pdf/pntd.0000328.pdf VL - 2 SN - 1935-2735 ER -