RQ: Relative quantity. Expression of biofilm-associated genes STI571 chemical structure fnbAB, sasG and spa The agr-dysfunctional isolate 08–008, which showed increased biofilm accumulation in vitro and in vivo, had a significant increase (p=0.02) in fnbA transcripts (RQ fnbA =10.08±0.18) when compared with the isolate 96/05 RQ fnbA =4.91±0.19; Figure 8). However, no significant difference was detected when fnbB expression were analyzed (RQ96/05 =0.11±0.04; RQ08-008 =0.18±0.05; Figure 8). Similarly to fnbA, the expression of sasG
(Figure 8; p=0.03) and spa (Figure 8; p<0.001) was also increased in 08–008 (RQ sasG =1.13±0.11; RQ spa =52.8±0.17) compared with 96/05 isolate (RQ sasG =0.65±0.14; RQ spa =0.8±0.20). find more Adherence and invasion The naturally agr-dysfunctional isolate 08–008 showed significant increase (p<0.05) in the adherence to human airway cells, reaching
25.27%±0.4% at 3h30min of incubation. In contrast, at the same conditions, the adherence of the agr-functional (isolate 96/05) to airway cells occurred in much less extent (4.94%±0.2%). Similarly, invasion check details was also higher for the agr-dysfunctional isolate (6.37%±0.3%) when compared with the agr-functional (1.76%±0.2%) at 3h30min incubation (Figure 9, top). Likewise, an increased invasive ability in the stationary phase was observed for the agr-knockout MHC474 (10.6%±0.3%) when compared with the wild type (HC474; 2.8%±0.1%) and complemented construction CMHC474 (2.3%±0.1%; p=0.0033; Figure 9, bottom). Figure 9 Adherence and invasion assays using human bronchial epithelial cell line (16HBe14o – ). Top: 96/05 (agr-functional) and 08–008 (agr-dysfunctional). Bottom: Invasion assay was also determined after 3h30 min for the wild-type strain HC474, isogenic agr knockout MHC474 (Δagr::tetM) and the rnaIII-trans-complemented construction CMHC474 (Δagr::tetM, pbla-rnaIII). Discussion The great majority of the USA400-related isolates (50/60; 83.3%) were able to accumulate strong/moderate biofilms on polystyrene surfaces. The isolates remaining produced weak biofilms. The ability to accumulate biofilm increased when the surfaces
were covered with human fibronectin, as also reported by others [19, 29]. In opposition to our results, it was reported that MW2 3-mercaptopyruvate sulfurtransferase MRSA had a weak biofilm phenotype [30, 31]. Similarly, a slight biofilm accumulation (OD=0.25-0.3) was observed for another USA400 strain called BAA-1683 [32]. In addition, recent data from our laboratory (Ramundo MS & Figueiredo AMS, 2012; unpublished observations) showed that another SCCmecIV isolates (ST30 CA-MRSA) accumulated much lower amount of biofilm compared with ST1-SCCmecIV isolates. Previous data from our group [12] have also demonstrated that the ST1 isolates from Rio de Janeiro do not carry lukSF genes and have acquired a number of antimicrobial resistance traits.
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