After the infection processes, anti-miR miR-141
was transfected again into the virus infected cells and incubated for another 24 hours. The results of this experiment showed that the click here anti-miR miR-141 inhibitor could cause an increase in TGF-β2 protein expression in H1N1 or H5N1 infected cells, as compared to cells only infected with H1N1 or H5N1 but without anti-miR miR-141 inhibitor treatment (Figure 3). The effect was also more prominent in H5N1 infection than that of H1N1. Figure 3 Measurement of TGF-β2 mRNA and protein level. NCI-H292 cells with or without treatment of miR-141 inhibitor, were infected with influenza A virus subtypes: H1N1/2002 or H5N1/2004 viruses at m.o.i. = 1, respectively for 24 hours. qRT-PCR were used to quantitify the TGF-β2 mRNA levels and fold-changes were calculated by ΔΔCT method as compared with non-infection cell control (mock) and using endogeneous actin mRNA level for normalization. TGF-β2 protein level
was measured by enzyme-linked immunosorbent assay selleckchem as compared with mock. Each point on the graph respresents the mean fold-changes. The experimental mean fold-changes of mRNA and protein levels were compared to that of mock controls ± SD (p* < 0.05), (p#< 0.05), respectively. Discussion In this study we examined the connection between influenza A virus infection and the global patterns of cellular miRNA expression. The major observations from this work were that influenza A virus infection resulted in the altered regulation of cellular miRNAs. Avian influenza A virus can alter cellular miRNAs to a greater extent than that of seasonal human influenza A virus. Influenza A virus affects the regulation of many cellular processes. In some Reverse transcriptase cases, these changes are directed by the virus for its advantage and others are cellular defense responses to infection. Here, we found that influenza A virus infection led to altered regulation of cellular miRNAs. Given the number of genes that can be regulated by individual miRNAs and the number of miRNAs expressed
in cells, this greatly expands the range of possible virus-host regulatory interactions. The complexity is underscored by there being no uniform global pattern of regulation; rather, it appears that individual (or Y-27632 clinical trial groups of) miRNA are independently regulated, some positively and some negatively. Persistent and transient effects were seen, and changes in miRNA expression profiles were linked to the time course of infection. As a summary, miR-1246, miR-663 and miR-574-3p were up-regulated (>3-fold, p<0.05) at 24-hour post-infection with subtype H5 as compared with non-infected control cells. Moreover, miR-100*, miR-21*, miR-141, miR-1274a and miR1274b were found to be down-regulated (>3-fold, p<0.05) in infection with subtype H5, particularly at 18 or 24 hours post-infection as compared with non-infected control cells.