Stoeckle M Y
Division of Infectious Diseases, Cornell University Medical College, New York, NY 10021.
Nucleic Acids Res. 1991 Feb 25;19(4):917-20. doi: 10.1093/nar/19.4.917.
Expression of the cytokine gene gro, also known as melanoma growth stimulatory activity, is induced by inflammatory stimuli, including IL-1. To determine whether gro expression is regulated at a post-transcriptional level, the effect of IL-1 on gro mRNA stability was examined. Treatment of fibroblasts with IL-1 beta caused a dose-dependent induction of gro mRNA. When IL-1 was withdrawn, gro mRNA decayed rapidly with a half life of 1 hour. This decay occurred whether or not actinomycin D was added to block new transcription. In contrast, when IL-1 was present in the medium, the level of gro mRNA was stable over 8 hours following addition of actinomycin D. In addition, the stability of a related mRNA, IL-8, was found to be regulated by IL-1. To examine whether Northern results reflected expression of gro alpha, or of the closely related genes, gro beta and gro gamma, RNA samples were analyzed by PCR. All three genes were found to be induced by IL-1 and all mRNAs were stabilized in the presence of IL-1. Northern analysis revealed a minor species of gro mRNA which lacked poly(A). The pattern of expression of this RNA suggested that it was a decay intermediate of one or more of the gro mRNAs. The findings indicate that mRNA stabilization is an important component of IL-1 induced gene expression.
细胞因子基因gro(也称为黑素瘤生长刺激活性)的表达可由包括白细胞介素-1(IL-1)在内的炎症刺激诱导。为了确定gro的表达是否在转录后水平受到调控,研究了IL-1对gro mRNA稳定性的影响。用IL-1β处理成纤维细胞会导致gro mRNA呈剂量依赖性诱导。当去除IL-1时,gro mRNA迅速降解,半衰期为1小时。无论是否添加放线菌素D以阻断新的转录,这种降解都会发生。相反,当培养基中存在IL-1时,添加放线菌素D后8小时内gro mRNA水平保持稳定。此外,发现相关mRNA白细胞介素-8(IL-8)的稳定性也受IL-1调控。为了检查Northern印迹结果反映的是groα的表达,还是密切相关基因groβ和groγ的表达,通过聚合酶链反应(PCR)分析了RNA样本。发现所有三个基因均由IL-1诱导,并且在IL-1存在的情况下所有mRNA均得到稳定。Northern印迹分析揭示了一种缺少聚腺苷酸(poly(A))的gro mRNA小种。这种RNA的表达模式表明它是一种或多种gro mRNA的降解中间体。这些发现表明mRNA稳定化是IL-1诱导基因表达的一个重要组成部分。
Zotero 插件
