An increase

in number of HEp-2 cells without any adhering

An increase

in number of HEp-2 cells without any adhering bacteria was observed in the presence of either antiserum, accordingly (Figure 2). However, pre-incubation with normal rabbit sera at 1:5 OICR-9429 purchase dilution (data not shown) showed the same selleck kinase inhibitor diffuse, moderate adherence as in the absence of any antisera (Additional file 2, Figure 3 panel B and Figure 2). Figure 3 Adherence patterns of O157 strains on HEp-2 cells, in the presence of D + Mannose and +/− antisera. Panel A, O157 strain EDL933, in the presence of “pooled antisera” against LEE. Intimin and flagellar H7 proteins, and the anti-Intimin antisera alone, at 1:100 and 1:10 dilutions, respectively. Panel B, O157 strain EDL933, in the absence of any sera (No sera). Panel C, O157 strain 86–24 (Intimin-positive) and Selleck CHIR 99021 its mutant derivatives, 86-24eae Δ10 (Intimin-negative), and 86-24eae Δ10 (pEB310) (Initmin-positive) in the absence of any sera. The immunofluorescence (IF) stained slides are shown at 40x magnification. O157 have green fluorescence, actin filaments of HEp-2 cells have orange-red fluorescence, and their nuclei have blue fluorescence. The results observed with the adherence inhibition assays were further verified by the adherence patterns of

O157 strain 86–24 (86–24) and its mutant derivatives on HEp-2 and RSE cells (Figure 3, panel C, Figures 4 and 2). The intimin-negative mutant 86-24eae Δ10 did not adhere well to the HEp-2 cells compared to the intimin-positive, wild-type 86–24 or complemented mutant, 86-24eae Δ10(pEB310) that demonstrated diffuse, moderate adherence (Figure 3, panel C, Figure 2, and Additional file 2). Actin accumulation observed in the majority of HEp-2 cells with 100x magnification only in the presence of 86–24

and Methane monooxygenase 86-24eae Δ10(pEB310), along with an increase in the number of HEp-2 cells without adhering bacteria in the presence of 86-24eae Δ10, further verified these observations (data not shown). This confirmed the role of intimin in O157 adherence to HEp-2 cells. On the otherhand, 86–24 and all its mutant derivatives demonstrated diffuse, strong adherence to RSE cells, irrespective of intimin expression (Figures 4 and 2, and Additional file 1). Infact with 86-24eae Δ10, the number of RSE cells with adhering bacteria actually increased, which suggested that intimin did not have a role in the adherence of O157 to RSE cells. Figure 4 Adherence patterns of O157 strain 86–24 (Intimin-positive) and its mutant derivatives, 86-24 eae Δ10 (Intimin-negative) and 86-24 eae Δ10 (pEB310) (Initmin-positive), on RSE cells, in the presence of D + Mannose. The immunofluorescence (IF) stained slides are shown at 40x magnification. O157 have green fluorescence, cytokeratins’ of RSE cells have orange-red fluorescence, and their nuclei have blue fluorescence.

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