Airway Disease, National Heart and Lung Institute, Imperial College London, London, UK.
Respir Res. 2010 Jun 2;11(1):68. doi: 10.1186/1465-9921-11-68.
Despite the widespread induction of miR-146a during the innate immune response little is known regarding its biogenesis, function and mechanism. We have therefore examined the role of miR-146a during the interleukin (IL)-1beta-stimulated IL-6 and IL-8 release and proliferation in primary human airway smooth muscle (HASM) cells.
HASM cells were isolated from human lung re-section, cultured to a maximum of 3 - 6 passages and then exposed to IL-1beta. miR-146a expression were determined by qRT-PCR, IL-6 and IL-8 release by ELISA and proliferation using bromodeoxyuridine incorporation. The role of NF-kappaB and the MAP kinase pathways was assessed using pharmacological inhibitors of IKK2 (TPCA-1), JNK (SP600125), p38 MAP kinase (SB203580) and MEK-1/2 (PD98059). miR-146a function was determined following transfection of HASM with inhibitors and mimics using Amaxa electroporation.
IL-1beta induced a time-dependent and prolonged 100-fold induction in miR-146a expression, which correlated with release of IL-6 and IL-8. Exposure to IL-1beta had no effect upon HASM proliferation. Pharmacological studies showed that expression of primary miR-146a was regulated at the transcriptional levels by NF-kappaB whilst post-transcriptional processing to mature miR-146a was regulated by MEK-1/2 and JNK-1/2. Functional studies indicated that IL-1beta-induced miR-146a expression does not negatively regulate IL-6 and IL-8 release or basal proliferation. However, inhibition of IL-1beta-induced IL-6 and IL-8 release was observed at the super-maximal intracellular miR-146a levels obtained by transfection with miR-146a mimics and indicates that studies using miRNA mimics can produce false positive results. Mechanistic studies showed that in the presence of super-maximal levels, the action of miR-146a mimics was mediated at a step following IL-6 and IL-8 mRNA transcription and not through down-regulation of IL-1 receptor associated kinase 1 (IRAK-1) and TNF receptor-associated factor 6 (TRAF6) protein expression, two predicted miR-146a targets involved in IL-1beta signalling.
We have shown that IL-1beta-induced miR-146a expression in HASM and that this was regulated at the transcriptional level by NF-kappaB and at the post-transcriptional level by the MEK-1/2 and JNK-1/2. Unlike previous reports, studies using miRNA inhibitors showed that miR-146a expression did not regulate IL-6 and IL-8 release or proliferation and suggest miR-146a function and mechanism is cell-type dependent.
尽管在先天免疫反应中广泛诱导了 miR-146a,但关于其生物发生、功能和机制知之甚少。因此,我们研究了 miR-146a 在白细胞介素 (IL)-1β刺激的人原代气道平滑肌 (HASM) 细胞中 IL-6 和 IL-8 释放和增殖中的作用。
从人肺切除术中分离 HASM 细胞,培养至最大 3-6 代,然后用 IL-1β 处理。通过 qRT-PCR 测定 miR-146a 的表达,通过 ELISA 测定 IL-6 和 IL-8 的释放,通过溴脱氧尿苷掺入测定增殖。使用 IKK2(TPCA-1)、JNK(SP600125)、p38 MAP 激酶(SB203580)和 MEK-1/2(PD98059)的药理学抑制剂评估 NF-κB 和 MAP 激酶途径的作用。使用 Amaxa 电穿孔转染 HASM 中的抑制剂和模拟物来确定 miR-146a 的功能。
IL-1β诱导 miR-146a 表达呈时间依赖性和延长 100 倍诱导,与 IL-6 和 IL-8 的释放相关。IL-1β 对 HASM 增殖没有影响。药理研究表明,初级 miR-146a 的表达在转录水平上受 NF-κB 调节,而成熟 miR-146a 的转录后加工受 MEK-1/2 和 JNK-1/2 调节。功能研究表明,IL-1β 诱导的 miR-146a 表达不会负调控 IL-6 和 IL-8 的释放或基础增殖。然而,在用 miR-146a 模拟物转染获得的最大细胞内 miR-146a 水平下观察到抑制 IL-1β 诱导的 IL-6 和 IL-8 释放,表明使用 miRNA 模拟物的研究可能产生假阳性结果。机制研究表明,在存在超最大水平的情况下,miR-146a 模拟物的作用是在 IL-6 和 IL-8 mRNA 转录之后的步骤介导的,而不是通过下调 IL-1 受体相关激酶 1 (IRAK-1) 和肿瘤坏死因子受体相关因子 6 (TRAF6) 蛋白表达,这两种预测的 miR-146a 靶点参与了 IL-1β 信号转导。
我们已经表明,IL-1β 在 HASM 中诱导 miR-146a 表达,并且这是由 NF-κB 在转录水平和 MEK-1/2 和 JNK-1/2 在转录后水平调节的。与先前的报道不同,使用 miRNA 抑制剂的研究表明,miR-146a 表达不会调节 IL-6 和 IL-8 的释放或增殖,并表明 miR-146a 的功能和机制依赖于细胞类型。
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