ial target for JNK1 regulation. The role of JNK1 within T cells is an active area of investigation. JNK1 has previously been shown to play a role in TH1/TH2 polarization and cytokine production, although its role in differentiation of TH17 cells is unknown. The impact of JNK1 deficiency with regards to IL-17A and airway epithelial cells was previously unclear. Our data show that JNK1 is required for induction of IFNc, MCP-1, G-CSF and antimicrobial peptides. These data define a clear role for an IL-17A/JNK1 signaling axis in lung primary epithelial cells relevant to lung infection and in whole lung tissue. The findings presented in this study indicate a diverse role for JNK1 in host defense in the lung. The potential role for JNK1 in regulation of macrophage responses in vivo is intriguing and JNK1 and Host Defense requires further investigation. In addition, the role of JNK1 in regulating antimicrobial peptide production may have broad consequences in immunity against numerous extracellular pathogens. Finally, the impact of JNK1 on viral clearance and pathogenesis is intriguing and remains to be elucidated. Since JNK1 modulates some of the functional effects of IL-17A, it is likely that JNK1 is required for host defense in a number of TH17 mediated diseases. These data identify the JNK1 pathway as “2049105 an important target in understanding lung immunity. Targeting JNK1 may provide a novel therapeutic approach for treating pneumonia. Materials and Methods Animals Heterozygous JNK1 /2 mice on a N5 generation C57BL/6 background were purchased from Jackson Laboratories and were maintained as a breeding colony under pathogen free conditions. All experiments were conducted with age and sex “2413012 matched JNK1 2/2 and wild-type littermate controls. All animal studies were approved by the University of Pittsburgh Institutional Animal Care and Use Committee, protocol 0903113. 9 JNK1 and Host Defense Bacterial Infection Models JNK1 2/2 and WT mice were inoculated with Escherichia coli or AMI-1 Staphylococcus aureus by oropharyngeal aspiration in 50 ml of sterile PBS. Bacteria were grown for 18 hours to stationary phase prior to inoculation. Twenty-four hours following infection, mice were lavaged with 1 ml sterile PBS for differential cell counts by cytospin. The right lung was then homogenized in 1 ml sterile PBS for bacterial colony counting, cytokine analysis by multiplex assay or by ELISA for IL-23p19, and real-time PCR for gene expression. The left lung was fixed in 10% neutral buffered formalin for histologic processing and H&E staining. Lung parenchymal and peribronchial inflammation were scored on double-blinded sections using a 0, least inflamed to 3, most inflamed. Each slide was scored twice and data reflect the cumulative inflammation score. JNK1 Kinase Assay JNK1 activity in protein homogenates from MTEC was determined as previously described. Briefly, JNK1 was immunoprecipitated from homogenates using anti-JNK1 antibody. JNK1 was then incubated with P32ATP and a GST-c-Jun substrate for 30 minutes at 30uC. Phosphorylation of GST-c-Jun was then visualized by SDS-PAGE and autoradiography imaging. Exogenous IL-17A Models Adenovirus expressing IL-17A was generated as previously described . WT and JNK1 2/2 mice were instilled with 56108 pfu of adenovirus expressing IL-17A by oropharyngeal aspiration. Mice were then incubated for 3 days prior to harvest. Mouse lungs were lavaged and processed as described above. Additionally, WT and JNK1 2/2 mice were insti
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