4 and 0.04 genome equivalent (ge) by reaction) of a known quantity of DNA extracted from four strains: M. avium, M. fortuitum, M. intracellulare and M. gordonae (identified from the national French reference laboratory collection). Specificity and sensitivity were estimated against 30 non-mycobacteria (negative) strains and 31 mycobacteria (PF-3084014 positive), respectively. The collection contained reference and
environmental strains of mycobacteria, as well as, strains of the closely related CNM group, and other non-actinobacteria strains isolated from the environment [17]. Mycobacteria collection included MTC (n = 2) and leprae species (n = 1), as well as species of slow growing NTM (n = 13), and rapid growing NTM (n = 15). TaqMan® real-time PCR were performed in duplicate using an ABI7500 real-time PCR system (Applied
Biosystems), a Lifetech 7500 software version 2.0.6 (Applied Biosystems) and TaqMan selleck chemical fast virus 1-STEP Master Mix with 6-carboxy-X-rhodamine (ROX) (Applied Biosystems). The TaqMan® probes were labeled (Eurogentec) with the fluorescent dyes 6-carboxyfluorescein (5′ end) and Black Hole Quencher (3′ end). All reactions were performed in a 25 μl reaction mixture volume (2.5 μl of DNA) with 500 nM of forward primer, 500 nM of reverse primer, 50 nM of probe and 5 mM of MgCl2. Reverse transcriptase was inactivated immediately (95 °C, 45 s) according
to the manufacturer instruction, HSP990 price and real-time PCR consisted in 40 cycles of denaturation (95°C for 3 s), annealing and extension (both steps at 60°C for 30 s). Determinations of cycle threshold were performed by setting the instrument’s threshold line at 0.02 Galeterone ∆Rn units (fluorescence gain above the baseline divided by the ROX channel signal). Environmental analyses In order to compare the new real-time PCR method to the culture method, 26 tap water distribution points in Paris (France) were sampled between April 2011 and July 2011, corresponding to 90 samples. Briefly, one liter of tap water was sampled in sterile plastic bottle, then centrifuged at 5000 × g for 2h and finally re-suspended in 1 ml of water. Mycobacteria density was estimated by culture (Method A) in all these samples following the procedure previously described by Le Dantec et al. [28]. In parallel, DNA was extracted using two different methods: i) a bacterial DNA extraction kit (QIAamp DNA mini kit, Qiagen) according to the manufacturer recommendations (Method B), and ii) a phenol-chloroform extraction procedure according to Radomski et al. [29] (Method C). Extracted DNA was 10 fold diluted and mycobacteria density was estimated in duplicate using the new real-time PCR method. Using environmental samples, the new atpE targeting method was also compared a previously described rrs targeting method [17].