p38 MAP 激酶和 MAP 激酶激酶 6 对抗炎基因的差异调节。
Differential regulation of anti-inflammatory genes by p38 MAP kinase and MAP kinase kinase 6.
机构信息
University of California San Diego School of Medicine, La Jolla, CA, USA.
出版信息
J Inflamm (Lond). 2014 May 16;11:14. doi: 10.1186/1476-9255-11-14. eCollection 2014.
BACKGROUND
Conventional p38α inhibitors have limited efficacy in rheumatoid arthritis, possibly because p38 blockade suppresses the counter-regulatory mechanisms that limit inflammation. In contrast, targeting the upstream MAP kinase kinases, MKK3 and MKK6, partially maintains p38-mediated anti-inflammatory responses in bone marrow-derived macrophages (BMDM). In this study, we explored the mechanisms that preserve anti-inflammatory gene expression by evaluating differential regulation of IL-10 and p38-dependent anti-inflammatory genes in MKK3-/-, MKK6-/-, and p38 inhibitor-treated wildtype cells.
METHODS
BMDM from wild type (WT), MKK3-/-, and MKK6-/- mice were pre-treated with p38 inhibitor SB203580 (SB), JNK inhibitor SP600125 (SP), and/or ERK inhibitor PD98059 (PD) and stimulated with LPS. Supernatant protein levels were measured by multiplex bead immunoassay. mRNA expression was determined by qPCR and protein expression by Western blot analysis. De novo IL-10 mRNA synthesis was quantified in cells treated with ethynyl-uridine and LPS followed by reverse transcription and qPCR. mRNA half-life was measured in LPS-treated cells that were then incubated with actinomycin D ± SB203580.
RESULTS
Pre-treatment of WT BMDM with p38 inhibitor significantly reduced IL-10 production in the three groups, while ERK and JNK inhibitors had minimal effects. IL-10 production was significantly decreased in MKK3-/- BMDM compared with either WT or MKK6-/- cells. IL-10 mRNA expression was modestly reduced in MKK3-/- BMDM but was preserved in MKK6-/- cells compared with WT. De novo IL-10 mRNA synthesis was inhibited in MKK3-/- and p38 inhibitor pre-treated cells, but not MKK6-/- cells compared with WT. IL-10 mRNA half-life was markedly reduced in p38 inhibitor-treated WT cells while MKK-deficiency had minimal effect. DUSP1 mRNA levels were preserved in MKK-deficient cells but not in p38 inhibitor-treated WT cells. Tristetraprolin mRNA and protein levels were reduced in p38 inhibitor-treated WT cells compared with MKK6-/- cells.
CONCLUSION
Unlike p38-inhibition, the absence of MKK6 mostly preserves IL-10 and TTP protein expression in BMDM. MKK6-deficiency also spares DUSP1 and IL-1RA, which are key negative regulators of the inflammatory response. Together, these data suggest that MKK6 is a potential therapeutic target in RA.
背景
传统的 p38α 抑制剂在类风湿关节炎中的疗效有限,这可能是因为 p38 阻断会抑制限制炎症的代偿机制。相比之下,靶向上游 MAP 激酶激酶 MKK3 和 MKK6,部分维持了骨髓来源的巨噬细胞(BMDM)中 p38 介导的抗炎反应。在这项研究中,我们通过评估 MKK3-/-, MKK6-/-, 和 p38 抑制剂处理的野生型细胞中 IL-10 和 p38 依赖性抗炎基因的差异调控,来探讨保留抗炎基因表达的机制。
方法
用 p38 抑制剂 SB203580(SB)、JNK 抑制剂 SP600125(SP)和/或 ERK 抑制剂 PD98059(PD)预处理野生型(WT)、MKK3-/-和 MKK6-/-小鼠的 BMDM,并用 LPS 刺激。通过多重珠免疫测定法测量上清液蛋白水平。通过 qPCR 确定 mRNA 表达,通过 Western blot 分析确定蛋白表达。用 LPS 处理后,用 ethynyl-uridine 和 LPS 处理细胞,然后进行反转录和 qPCR 来定量新合成的 IL-10 mRNA。在 LPS 处理的细胞中测量 mRNA 半衰期,然后用 actinomycin D ± SB203580 孵育。
结果
WT BMDM 用 p38 抑制剂预处理显著降低了三组中的 IL-10 产生,而 ERK 和 JNK 抑制剂的影响较小。与 WT 或 MKK6-/-细胞相比,MKK3-/-BMDM 的 IL-10 产生明显减少。与 WT 相比,MKK3-/-BMDM 的 IL-10 mRNA 表达略有降低,但在 MKK6-/-细胞中得以保留。与 WT 相比,新合成的 IL-10 mRNA 在 MKK3-/-和 p38 抑制剂预处理的细胞中被抑制,但在 MKK6-/-细胞中未被抑制。与 MKK 缺陷细胞相比,用 p38 抑制剂处理的 WT 细胞中的 IL-10 mRNA 半衰期明显降低。DUSP1 mRNA 水平在 MKK 缺陷细胞中得以保留,但在 p38 抑制剂处理的 WT 细胞中未保留。与 MKK6-/-细胞相比,p38 抑制剂处理的 WT 细胞中的 tristetraprolin mRNA 和蛋白水平降低。
结论
与 p38 抑制不同,MKK6 的缺失在 BMDM 中主要保留了 IL-10 和 TTP 蛋白的表达。MKK6 缺失还可节省 DUSP1 和 IL-1RA,它们是炎症反应的关键负调节剂。这些数据表明,MKK6 是 RA 的一个潜在治疗靶点。
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