1. FIP200 is Involved in Murine Pseudomonas Infection by Regulating HMGB1 Intracellular Translocation
- Author
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Jin-liang Yang, Changpei Gan, Xuefeng Li, Xikun Zhou, Shuang Zhang, Min Wu, Yuquan Wei, and Yi Li
- Subjects
Gene knockdown ,Physiology ,Autophagy ,chemical and pharmacologic phenomena ,Chromosomal translocation ,Transfection ,Biology ,Molecular biology ,3. Good health ,Cell biology ,Cell culture ,Alveolar macrophage ,Gene silencing ,Signal transduction - Abstract
c The first two authors contributed equally to this work Abstract Background: FIP200, a critical autophagy initiating protein, can participate in numerous cellular functions including cancer development; however, its functional role in P. aeruginosa infection of alveolar macrophages is unknown. Methods: To investigate the role of FIP200 in host defense, we transfected murine alveolar macrophage MH-S cells with FIP200 siRNA. Having confirmed that FIP200 knockdown inhibited PAO1-induced autophagosme formation, we sought to characterize the underlying signaling pathways by immunoblotting. Further, we used fip200 KO mice to study the effects of fip200 deficiency on HMGB1 translocation. Results: We showed that Pseudomonas PAO1 strain infection facilitated autophagosome formation, whereas knockdown of FIP200 inhibited autophagosome formation and HMGB1 expression in MH-S cells. Silencing FIP200 impaired the translocation of HMGB1 to cytosol of MH-S cells and almost abolished acetylation of HMGB1 during PAO1 infection. In contrast, FIP200 overexpression facilitated the cytosol translocation of HMGB1 from nuclei and increased acetylation of HMGB1 in PAO1-infected MH-S cells. Importantly, expression and acetylation of HMGB1 were also significantly down-regulated in fip200 KO mice following PAO1 infection. Conclusions: Collectively, these findings elucidate that FIP200 may regulate expression and translocation of HMGB1 during PAO1 infection, which may indicate novel therapeutic targets to control pulmonary infection.
- Published
- 2014