Identification and Analysis of Interacting Proteins Regulating IFNβ Expression in PPARγ Activated and Inhibited States
MA Zhuo-Yuan1,2, YANG Bin1,2, CHEN Yun-Long1,2, FAN Gang1,2, WU Xiao-Long1,2, WANG Xi-Yin1,2, HUA Jin-Lian1,2, WANG Yan1,2, ZHANG Yong-Qiang3,*, ZHANG Shi-Qiang1,2,*
1 College of Veterinary Medicine/Shaanxi Stem Cell Engineering Research Center, Northwest A&F University, Yangling 712100, China; 2 Key Laboratory of Livestock Biology, Northwest A&F University, Yangling 712100, China; 3 China Animal Health and Epidemiology Center, Qingdao 266032, China
Abstract:Peroxisome proliferator activated receptor γ (PPARγ) is specifically overexpressed in alveolar macrophages and has metabolic and immunoregulatory roles. It is not clear which interacting proteins of PPARγ are involved in the regulation of typeⅠinterferon production induced by innate immunity. In this study, wild boar (Sus scrofa) lung cell line (WSL) with stable overexpression of PPARγ-3×Flag was constructed using lentiviral vector system. Taking this cell strain as a model, fluorescence quantitative PCR assay revealed that the addition of the PPARγ agonist rosiglitazone significantly reduced the level of interferon β (IFNβ) expression induced by stimulating with the dsDNA mimic Poly (dA:dT); In contrast, addition of the PPARγ inhibitor T0070907 significantly increased the level of IFNβ expression induced by Poly (dA:dT) stimulation. Further, the PPARγ-3×Flag protein complex regulating the above process was precipitated by immunomagnetic beads of anti-FLAG protein. The PPARγ-3×Flag protein complexes enriched in cytoplasmic proteins and nuclear proteins were digested into peptides and analyzed by liquid chromatography and tandem mass spectrometry (LC-MS/MS), respectively. The results showed that there were 101 cytoplasmic proteins and 95 nucleoproteins interacting specifically with PPARγ when the PPARγ agonist rosiglitazone was added. Under the condition of adding PPARγ inhibitor T0070907, there were 24 cytoplasmic proteins and 14 nuclear proteins that specifically interacted with PPARγ. GO and KEGG analysis showed that specific PPARγ interactions of cytoplasmic proteins and nuclear proteins were related to translation regulation. This study provides a new clue to further study the mechanism of regulating of IFNβ expression by PPARγ.
[1] Akira S, Uematsu S, Takeuchi O.2006. Pathogen recognition and innate immunity[J]. Cell, 124(4): 783-801. [2] Arimoto K I, Miyauchi S, Stoner S A, et al.2018. Negative regulation of typeⅠIFN signaling[J]. Jourmal of Leukocyte Biology, 103(6): 1099-1116. [3] Chen C, Xu P L.2023. Cellular functions of cGAS-STING signaling[J]. Trends in Cell Biology, 33(8): 630-648. [4] Chen J, Baig E, Fish E N.2004. Diversity and relatedness among the typeⅠinterferons[J]. Journal of Interferon and Cytokine Research, 24(12): 687-698. [5] Dong H J, Zhang R, Kuang Y, et al.2021. Selective regulation in ribosome biogenesis and protein production for efficient viral translation[J]. Archives of Microbiology, 203(3): 1021-1032. [6] Dreyer C, Krey G, Keller H, et al.1992. Control of the peroxisomal beta-oxidation pathway by a novel family of nuclear hormone receptors[J]. Cell, 68(5): 879-887. [7] Garcia-Belmonte R, Perez-Nunez D, Pittau M, et al.2019. African swine fever virus Armenia/07 virulent strain controls interferon beta production through the cGAS-STING pathway[J]. Journal of Virology, 93(12): e02298. [8] Huang S, Zhu B, Cheon I S, et al.2019. PPAR-gamma in macrophages limits pulmonary inflammation and promotes host recovery following respiratory viral infection[J]. Journal of Virology, 93(9): e00030. [9] Issemann I, Green S.1990. Activation of a member of the steroid hormone receptor superfamily by peroxisome proliferators[J]. Nature, 347(6294): 645-650. [10] Janani C, Ranjitha Kumari B D.2015. PPAR gamma gene-a review[J]. Diabetes & Metabolic Syndrome, 9(1): 46-50. [11] Ju X, Li F, Li J, et al.2021. Genome-wide transcriptomic analysis of highly virulent African swine fever virus infection reveals complex and unique virus host interaction[J]. Veterinary Microbiology, 261: 109211. [12] Kawane K, Motani K, Nagata S.2014. DNA degradation and its defects[J]. Cold Spring Harbor Perspectives in Biology, 6(6): 176. [13] Orsi D L, Pook E, Brauer N, et al.2022. Discovery and structure-based design of potent covalent PPARgamma inverse-agonists BAY-4931 and BAY-0069[J]. Journal of Medicinal Chemistry, 65(21): 14843-14863. [14] Pestka S, Krause C D, Walter M R.2004. Interferons, interferon-like cytokines, and their receptors[J]. Immunological Reviews, 202: 8-32. [15] Schneider C, Nobs S P, Kurrer M, et al.2014. Induction of the nuclear receptor PPAR-gamma by the cytokine GM-CSF is critical for the differentiation of fetal monocytes into alveolar macrophages[J]. Nature Immunology, 15(11): 1026-1037. [16] Schoggins J W.2019. Interferon-stimulated genes: What do they all do[J]? Annual Review of Virology, 6(1): 567-584. [17] Umemoto T, Fujiki Y.2012. Ligand-dependent nucleo-cytoplasmic shuttling of peroxisome proliferator-activated receptors, PPARalpha and PPARgamma[J]. Genes Cells, 17(7): 576-596. [18] Woo Y D, Jeong D, Chung D H.2021. Development and functions of alveolar macrophages[J]. Molecules and Cells, 44(5): 292-300. [19] Wu Q, Leng X, Xu P.2023. Intercellular transmission of cGAS-STING signaling in cancer[J]. Cancer Biology & Medicine, 20(2): 93-97. [20] Yagi K, Huffnagle G B, Lukacs N W, et al.2021. The lung microbiome during health and disease[J]. International Journal of Molecular Sciences, 20(2): 93-97. [21] Zhang H, Alford T, Liu S, et al.2022. Influenza virus causes lung immunopathology through down-regulating PPARgamma activity in macrophages[J]. Frontiers in Immunology, 13: 958801.
