单核细胞黏附过程中IκBα的非转录依赖性周转：对调节IκBα/MAD-3 mRNA水平的翻译成分的影响。

Transcription-independent turnover of I kappa B alpha during monocyte adherence: implications for a translational component regulating I kappa B alpha/MAD-3 mRNA levels.

作者信息

Lofquist A K, Mondal K, Morris J S, Haskill J S

机构信息

UNC Lineberger Comprehensive Cancer Center, University of North Carolina at Chapel Hill 27599-7295.

出版信息

Mol Cell Biol. 1995 Mar;15(3):1737-46. doi: 10.1128/MCB.15.3.1737.

DOI:10.1128/MCB.15.3.1737

PMID:7532282

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC230398/

Abstract

We identified I kappa B alpha/MAD-3 as an immediate-early gene in human monocytes that is expressed in response to a variety of signals, including adhesion, lipopolysaccharide, and phorbol myristate acetate. Within 5 min of monocyte adhesion, the level of the I kappa B alpha protein is markedly diminished but is rapidly replaced in a cycloheximide-sensitive manner within 20 min. Accompanying the rapid turnover of the I kappa B alpha protein is simultaneous translocation of NF-kappa B-related transcription factors to nuclei of adhered monocytes. The demonstration that NF-kappa B can regulate I kappa B alpha/MAD-3 gene transcription in other cell types suggested that the rapid increase in steady-state I kappa B alpha/MAD-3 mRNA levels we observed within 30 min of monocyte adherence would result from NF-kappa B-dependent transcriptional stimulation of the I kappa B alpha/MAD-3 gene. Nuclear run-on analyses indicated that, instead, while several immediate-early cytokine genes, such as the interleukin 1 beta (IL-1 beta) gene, were transcriptionally activated during monocyte adhesion, the rate of I kappa B alpha/MAD-3 gene transcription remained constant. The adherence-dependent increase in I kappa B alpha/MAD-3 mRNA levels was also not a consequence of mRNA stabilization events. Interestingly, while increases in both IL-1 beta and I kappa B alpha/MAD-3 mRNA levels were detected in nuclei of adherent monocytes, cytoplasmic levels of IL-1 beta mRNA increased during adherence whereas those of I kappa B alpha/MAD-3 mRNA did not. Taken together, our data suggest that two interactive mechanisms regulate monocytic I kappa B alpha/MAD-3 mRNA levels. We propose that adherent monocytes regulate nuclear processing (or decay) of I kappa B alpha/MAD-3 mRNA, thereby increasing mRNA levels without stimulating I kappa B alpha/MAD-3 gene transcription. Moreover, since inhibition of protein synthesis leads to accumulation of I kappa B alpha/MAD-3 mRNA without stimulating I kappa B alpha/MAD-3 gene transcription, we suggest that low cytoplasmic levels of I kappa B alpha/MAD-3 mRNA are maintained by a translation-dependent degradation mechanism.

摘要

我们确定IκBα/MAD-3是人类单核细胞中的一个即早基因，其表达受多种信号的诱导，包括黏附、脂多糖和佛波酯。单核细胞黏附5分钟内，IκBα蛋白水平显著降低，但在20分钟内以对放线菌酮敏感的方式迅速恢复。伴随着IκBα蛋白的快速周转，NF-κB相关转录因子同时转位至黏附单核细胞的细胞核。在其他细胞类型中，NF-κB可调节IκBα/MAD-3基因转录，这表明我们在单核细胞黏附30分钟内观察到的稳态IκBα/MAD-3 mRNA水平的快速增加是由NF-κB依赖的IκBα/MAD-3基因转录刺激所致。然而，细胞核连续分析表明，在单核细胞黏附过程中，虽然一些即早细胞因子基因（如白细胞介素1β（IL-1β）基因）被转录激活，但IκBα/MAD-3基因的转录速率保持不变。IκBα/MAD-3 mRNA水平的黏附依赖性增加也不是mRNA稳定化事件的结果。有趣的是，虽然在黏附单核细胞的细胞核中检测到IL-1β和IκBα/MAD-3 mRNA水平均升高，但在黏附过程中，IL-1β mRNA的细胞质水平升高，而IκBα/MAD-3 mRNA的细胞质水平则没有升高。综上所述，我们的数据表明，两种相互作用的机制调节单核细胞IκBα/MAD-3 mRNA水平。我们提出，黏附的单核细胞调节IκBα/MAD-3 mRNA的核加工（或降解），从而在不刺激IκBα/MAD-3基因转录的情况下增加mRNA水平。此外，由于蛋白质合成抑制导致IκBα/MAD-3 mRNA积累而不刺激IκBα/MAD-3基因转录，我们认为IκBα/MAD-3 mRNA的低细胞质水平是由翻译依赖性降解机制维持的。