调节白细胞介素-1受体相关激酶4作为对抗尿酸钠和黄嘌呤诱导的巨噬细胞和肝癌细胞系炎症的治疗策略

Modulation of IRAK4 as a Therapeutic Strategy Against Monosodium Urate- and Xanthine-Induced Inflammation in Macrophages and HepG2 Cells.

作者信息

Umar Sadiq, Chang Huan T, Maienschein-Cline Mark, Ravindran Sriram

机构信息

University of Illinois Chicago.

Jesse Brown VA Medical Center.

出版信息

Res Sq. 2025 Jul 16:rs.3.rs-6908346. doi: 10.21203/rs.3.rs-6908346/v1.

DOI:10.21203/rs.3.rs-6908346/v1

PMID:40709261

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12288545/

Abstract

BACKGROUND

Interleukin-1 receptor-associated kinase 4 (IRAK4) is a pivotal mediator of toll-like receptor (TLR) and interleukin-1 receptor (IL-1R) signaling, critically involved in innate immune activation and pro-inflammatory cytokine production. Dysregulated IRAK4 activity contributes to chronic inflammation in both immune and non-immune cells. In this study, we evaluated the immunomodulatory potential of a selective IRAK4 inhibitor on monosodium urate (MSU) crystals-stimulated macrophages and xanthine-challenged HepG2 cells to assess its therapeutic potential.

METHODS

Human PBMCs were pretreated with 1 μM IRAK4 inhibitor (IRAK4i) overnight, followed by stimulation with 100 μg/ml MSU for either 30 minutes or 24 hours. Conditioned medium was collected for ELISA and RNA for qPCR to quantify pro- and anti-inflammatory factors. Cell lysates were prepared to analyze various TLR/IL-1β signaling proteins, including phosphorylated IRAK4, P38, ERK, and JNK. Phagocytosis was assessed using a Vybrant phagocytosis assay kit in PBMCs. We also utilize HepG2 cells and pretreated with 1 μM IRAK4 inhibitor (IRAK4i) overnight, followed by stimulation with 2.5mM of xanthine for 24 hours to assess the expression of cytokine and xanthine oxidoreductase.

RESULTS

Primary macrophages and HepG2 cells were treated with a potent IRAK4 inhibitor in the presence and absence of MSU or xanthine. In macrophages, IRAK4 inhibition significantly reduced the expression of TNF-α, IL-6, and IL-1β at both mRNA and protein levels, while promoting polarization toward an anti-inflammatory (M2-like) phenotype alongside reduced activation of NF-κB and MAPK pathways. In HepG2 cells, IRAK4 blockade attenuated xanthine-induced expression of xanthine dehydrogenase and inflammatory cytokines.

CONCLUSION

These findings demonstrate the dual anti-inflammatory effect of IRAK4 inhibition in both immune and hepatic cells and suggest a promising strategy to mitigate inflammation in gout.

摘要

背景

白细胞介素-1受体相关激酶4（IRAK4）是Toll样受体（TLR）和白细胞介素-1受体（IL-1R）信号传导的关键介质，在先天免疫激活和促炎细胞因子产生中起关键作用。IRAK4活性失调会导致免疫细胞和非免疫细胞的慢性炎症。在本研究中，我们评估了一种选择性IRAK4抑制剂对尿酸钠（MSU）晶体刺激的巨噬细胞和黄嘌呤刺激的HepG2细胞的免疫调节潜力，以评估其治疗潜力。

方法

人外周血单核细胞（PBMC）用1μM IRAK4抑制剂（IRAK4i）预处理过夜，然后用100μg/ml MSU刺激30分钟或24小时。收集条件培养基用于ELISA检测，收集RNA用于qPCR以定量促炎和抗炎因子。制备细胞裂解物以分析各种TLR/IL-1β信号蛋白，包括磷酸化的IRAK4、P38、ERK和JNK。使用Vybrant吞噬分析试剂盒评估PBMC中的吞噬作用。我们还使用HepG2细胞，用1μM IRAK4抑制剂（IRAK4i）预处理过夜，然后用2.5mM黄嘌呤刺激24小时，以评估细胞因子和黄嘌呤氧化还原酶的表达。

结果

在有和没有MSU或黄嘌呤的情况下，用强效IRAK4抑制剂处理原代巨噬细胞和HepG2细胞。在巨噬细胞中，IRAK4抑制在mRNA和蛋白质水平上均显著降低TNF-α、IL-6和IL-1β的表达，同时促进向抗炎（M2样）表型的极化，同时降低NF-κB和MAPK途径的激活。在HepG2细胞中，IRAK4阻断减弱了黄嘌呤诱导的黄嘌呤脱氢酶和炎性细胞因子的表达。