The Y-axis shows percentage of CD3 CD19 double-negative lymphocytes out of total CD45 positive splenic lymphocytes. Columns SPI2pos and SPI2neg show average values for all mice clustered into two groups according to being infected with either any of the SPI-2 positive or the SPI-2 negative mutants. * – t-test different from SPI2neg at P < 0.01. Figure 5 Presence of NK cells in spleen of mice 5 days post infection with the wild type S . Enteritidis (wt) or ΔSPI2 mutant averaged from the animal infections OSI-906 2, 3 and 4. n.i. – non-infected mice. * – t-test different from the non-infected or ΔSPI2
mutant infected mice at P < 0.01. Next we investigated whether the depletion of NK cells was associated specifically with the presence of SPI-2 or whether it was rather a general indicator of S. Enteritidis virulence. In this experiment we infected mice with another two attenuated mutants with defects in lon or rfaL and monitored NK cells in the spleen of infected mice. As shown in Figure 6, the NK cells decreased
in the spleen only after the infection with the wild type S. Enteritidis, but not after the infection with the rfaL or lon mutants. Figure 6 Presence of NK cells in spleen of mice 5 days post infection with the wild type S . Enteritidis (wt) or attenuated ΔSPI2, rfaL or lon mutants as determined in the animal infection 2. n.i. – non-infected mice. The NK cells depletion was not specific for the ΔSPI2 mutant but was a general indicator of the mutant’s virulence or avirulence. Pexidartinib datasheet Since there were only 3 animals per group and greater variation was observed among the mice infected with the wild type S. Enteritidis, none of the differences in this GNE-0877 experiment reached LY2835219 mw statistical significance. Although it was obvious that the NK cells
decreased after infection with the wild type strain or virulent mutants, the reason for the NK cell depletion was unknown. We considered two alternative hypotheses – either the NK cells migrated out of the spleen possibly to the intestinal tract or they died as a result of the extensive killing of S. Enteritidis-positive splenocytes. To test these hypotheses, we performed two additional experiments. In the first experiment we analysed cytokine signaling in the intestinal tract of the infected mice and in the second experiment we determined NK cell counts not only in the spleen but also in blood and the caecal lamina propria. These experiments were performed only with the wild type S. Enteritidis and ΔSPI2 mutant. When the cytokine signaling in the ceacal samples was determined, we did not find any differences in the expression of IFNγ, iNOS and IL-12p40. Numerically low, but statistically significant induction of TNFα was observed in caecum of mice infected with the wild type S. Enteritidis. Mice also responded to S. Enteritidis infection by the upregulation of IL-18 although this cytokine was significantly upregulated in mice infected both by the wild type S. Enteritidis and the ΔSPI2 mutant (Figure 7).