In a similar setting but using APCs, Lr1505 and Lr1506 also showe

In a similar setting but using APCs, Lr1505 and Lr1506 also showed a differential effect on the mRNA expression of

some cytokines as shown in Figure 1B. Although both strains stimulated adherent cells, Lr1505 showed a stronger enhancing influence than Lr1506 on the expression of mRNA coding for IL-1β, IFN-γ, IL-2, IL-12 and IL-10 (Figure 1B). Both lactobacilli slightly but significantly increased the mRNA synthesis of IL-6 and TNF-α to similar levels. In contrast to the results seen in PIE cells, there was no meaningful effect on the mRNA expression of type I IFN (Figure 1B). Furthermore, TGF-β mRNA levels were not affected by the stimulation with lactobacilli. L. rhamnosus selleck CRL1505 and CRL1506 stimulate PPs APCs and check details distinctly modulate cytokine production We next studied whether Lr1505 and Lr1506 were able to affect the expression of two cellular surface markers for APCs activation: MHC-II and CD80/CD86. Adherent cells isolated from

swine Peyer’s Patches can be grouped as CD172a+CD11R1high, CD172a−CD11R1low and CD172a+CD11R1− cells [21]. Although more detailed functional studies are needed to accurately define each AZD5153 research buy population, it has been suggested that CD172a+CD11R1high and CD172a−CD11R1low cells could be considered as DCs and CD172a+CD11R1− cells could be considered as macrophages [21]. In these three cell populations, both strains exerted an up-regulation of the antigen presenting and co-stimulatory molecules MHC-II and CD80/86, when compared to the non-stimulated control (Figure 1C) Janus kinase (JAK) indicating that these immunobiotic microorganisms were able to activate APCs. In all cases the MIF values in Lr1505-treated cells almost doubled the MIF presented by control cells (Figure 1C). APCs were similarly modulated by Lr1506 (data not shown). We also analysed by flow cytometry the levels of IL-1β, IL-6, IFN-γ, and IL-10 on the three populations of adherent cells: CD172a+CD11R1−, CD172a−CD11R1low and CD172a+CD11R1high (Figure 1D). In CD172a+CD11R1− cells

both strains Lr1505 and Lr1506 slightly but significantly enhanced the post-translational expression levels of IL-1β, IL-6, and IL-10, while the IFN-γ levels remained unchanged (Figure 1D). In CD172a−CD11R1low cells, both strains had a similar effect on the expression of IL-1β, IL-6 and IFN-γ, whereas IL-10 levels were not modified. In contrast, in CD172a−CD11R1high cells IL-10 protein levels were up-regulated by both strains, being Lr1505 the strain which showed the strongest stimulation (Figure 1D). In addition, IL-1β was modulated only by Lr1505 but neither IL-6 nor IFN-γ levels were affected by the stimulation of CD172a−CD11R1high cells with lactobacilli (Figure 1D). These results correlated with the mRNA expression profiles shown before (Figure 1B).

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