A UNG enzyme step (50 °C for 2 min) ensured hydrolysis of all sin

A UNG enzyme step (50 °C for 2 min) ensured hydrolysis of all single-stranded and double-stranded contaminating PCR products. Cycle threshold (CT) values >40 cycles were considered negative. The sensitivities of the IS2404/IPC and the IS2606/KR multiplex assays achieved in this setting were compared with the values described by Fyfe et al. (2007) by performing real-time PCR on serial dilutions of purified M. ulcerans DNA. Like Fyfe et al. (2007), our assays reliably detected two copies of IS2404, nine copies of IS2606,

and 1.5 to three copies of KR. We studied the effects of postponing a run of a prepared reaction plate on assay PARP inhibitor sensitivities in a similar way by keeping prepared plates at 4–8 °C for a period of >12 h before real-time PCR analysis was carried out, simulating the effects of a possible power cut before analysis could be started. This delay in analysis did not alter the sensitivities of the assays in any way. Pooled organs of 62 small mammals (36 Praomys spp., 10 Mastomys spp., five Lemniscomys spp., three Lophuromys spp., four Crocidura spp. Selleckchem GSK126 and four Mus spp.) caught in houses and around water bodies of a BU-endemic village (Ananekrom, in the Ashanti Region of Ghana; Fig. 1) as described before (Durnez et al.,

2008) were analyzed after DNA extraction using the modified Boom method (Boom et al., 1990; Durnez et al., 2009). Although none of the PCR reactions were inhibited, IS2404 was not detected in any of the specimens. A total of 148 environmental samples (13 water samples, 45 detritus samples,

45 trunk biofilm, and 45 plant biofilm samples) collected from water bodies near five BU endemic villages (n=117) and two BU nonendemic villages (n=31) (Fig. 1) were also analyzed. Although the DNA extraction procedure included a purification step using diatomaceous earth, reactions in 50 of the 148 environmental specimens were inhibited as they had CT values of the IPC three cycles higher than the nontemplate controls. These inhibited samples were successfully reanalyzed with a newly developed environmental master mix adapted for real-time PCR-based Glycogen branching enzyme detection in the presence of high levels of common environmental inhibitors (Applied Biosystems, TaqMan® Environmental Master Mix 2.0, ref. 4396838). Three samples (2.0%) were positive for IS2404, with CT values of 36.31, 38.45, and 37.95, respectively (Table 1). Of the three positive samples, only the water sample from Nshyieso also tested positive for IS2606 and KR, with a ΔCT (IS2606-IS2404) value of 1.96 (Table 1), suggesting that M. ulcerans DNA was detected and not DNA from other IS2404-containing mycobacteria that are known to have higher ΔCT values (Fyfe et al., 2007). The CT (IS2404) values of the other two IS2404-positive samples were higher than the sample that did contain IS2606 and KR, suggesting that the failure to detect KR and IS2606 was caused by a low DNA concentration, which is consistent with known differences in copy number per cell.

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