Kuwano Yuki, Rabinovic Ariel, Srikantan Subramanya, Gorospe Myriam, Demple Bruce
RNA Regulation Section, Laboratory of Cellular and Molecular Biology, National Institute on Aging-Intramural Research Program, National Institutes of Health, Baltimore, Maryland 21224, USA.
Mol Cell Biol. 2009 May;29(10):2622-35. doi: 10.1128/MCB.01495-08. Epub 2009 Mar 16.
We previously observed that nitric oxide (NO) exposure increases the stability of mRNAs encoding heme oxygenase 1 (HO-1) and TIEG-1 in human and mouse fibroblasts. Here, we have used microarrays to look broadly for changes in mRNA stability in response to NO treatment. Using human IMR-90 and mouse NIH 3T3 fibroblasts treated with actinomycin D to block de novo transcription, microarray analysis suggested that the stability of the majority of mRNAs was unaffected. Among the mRNAs that were stabilized by NO treatment, seven transcripts were found in both IMR-90 and NIH 3T3 cells (CHIC2, GADD45B, HO-1, PTGS2, RGS2, TIEG, and ID3) and were chosen for further analysis. All seven mRNAs showed at least one hit of a signature motif for the stabilizing RNA-binding protein (RBP) HuR; accordingly, ribonucleoprotein immunoprecipitation analysis revealed that all seven mRNAs associated with HuR. In keeping with a functional role of HuR in the response to NO, a measurable fraction of HuR increased in the cytoplasm following NO treatment. However, among the seven transcripts, only HO-1 mRNA showed a robust increase in the level of its association with HuR following NO treatment. In turn, HO-1 mRNA and protein levels were significantly reduced when HuR levels were silenced in IMR-90 cells, and they were elevated when HuR was overexpressed. In sum, our results indicate that NO stabilizes mRNA subsets in fibroblasts, identify HuR as an RBP implicated in the NO response, reveal that HuR alone is insufficient for stabilizing several mRNAs by NO, and show that HO-1 induction by NO is regulated by HuR.
我们之前观察到,在人和小鼠成纤维细胞中,一氧化氮(NO)暴露可增加编码血红素加氧酶1(HO-1)和TIEG-1的mRNA的稳定性。在此,我们使用微阵列来广泛寻找响应NO处理后mRNA稳定性的变化。在用放线菌素D处理以阻断从头转录的人IMR-90和小鼠NIH 3T3成纤维细胞中,微阵列分析表明大多数mRNA的稳定性未受影响。在经NO处理后被稳定的mRNA中,在IMR-90和NIH 3T3细胞中均发现了7种转录本(CHIC2、GADD45B、HO-1、PTGS2、RGS2、TIEG和ID3),并选择它们进行进一步分析。所有这7种mRNA均显示出至少一个稳定RNA结合蛋白(RBP)HuR的特征基序匹配;因此,核糖核蛋白免疫沉淀分析显示所有这7种mRNA均与HuR相关。与HuR在对NO的反应中的功能作用一致,经NO处理后,可测量的一部分HuR在细胞质中增加。然而,在这7种转录本中,只有HO-1 mRNA在经NO处理后与其与HuR的结合水平有显著增加。相应地,当在IMR-90细胞中沉默HuR水平时,HO-1 mRNA和蛋白水平显著降低,而当HuR过表达时则升高。总之,我们的结果表明NO可稳定成纤维细胞中的mRNA亚群,确定HuR为参与NO反应的RBP,揭示单独的HuR不足以通过NO稳定几种mRNA,并表明NO诱导的HO-1受HuR调节。