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首页> 美国卫生研究院文献>Journal of Virology >Induction of human interferon gene expression is associated with a nuclear factor that interacts with the NF-kappa B site of the human immunodeficiency virus enhancer.
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Induction of human interferon gene expression is associated with a nuclear factor that interacts with the NF-kappa B site of the human immunodeficiency virus enhancer.

机译:人干扰素基因表达的诱导与与人免疫缺陷病毒增强剂的NF-κB位点相互作用的核因子有关。

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The relationship between transcription of alpha and beta interferon (IFN-alpha and IFN-beta) genes and the interaction of IFN promoter-binding transcription factors has been examined in monoblastoid U937 cells following priming with recombinant IFN-alpha 2 (rIFN-alpha 2) and Sendai virus induction. Pretreatment of U937 cells with rIFN-alpha 2 prior to Sendai virus infection increased the mRNA levels of IFN-alpha 1, IFN-alpha 2, and IFN-beta as well as the final yield of biologically active IFN. Analysis of nuclear protein-IFN promoter DNA interactions by electrophoretic mobility-shift assays demonstrated increased factor binding to IFN-alpha 1 and IFN-beta regulatory domains, although no new induction-specific complexes were identified. On the basis of competition electrophoretic mobility-shift assay results, factors interacting with the IFN-alpha 1 and IFN-beta promoters appear to be distinct DNA-binding proteins. U937 factor binding was localized to the P2 domain (-64 to -55) of the IFN-beta regulatory element, a sequence motif with 80% homology to the recognition site of transcription factor NF-kappa B. Protein-DNA interactions within the IFN-beta P2 domain were, in fact, specifically competed by either excess homologous P2 fragment or the human immunodeficiency virus enhancer element which contains two duplicated NF-kappa B recognition sites. Hybrid promoter-chloramphenicol acetyltransferase fusion plasmids, containing either the IFN-beta regulatory element or the human immunodeficiency virus enhancer element linked to the simian virus 40 promoter, were analyzed for virus and phorbol ester inducibility in epithelial and lymphoid cells, respectively. In the 293 cell line, both plasmids were constitutively expressed but not virus inducible, while in Jurkat cells, chloramphenicol acetyltransferase activity from these plasmids was induced by tumor-promoting agent treatment. These experiments suggest that induction of IFN gene expression may be controlled in part by transcription regulatory proteins binding to an NF-kappa B-like site within the IFN-beta promoter.
机译:用重组IFN-alpha 2(rIFN-alpha 2)引发后,已在单母细胞样U937细胞中检查了α和β干扰素(IFN-α和IFN-β)基因的转录与IFN启动子结合转录因子相互作用的关系。和仙台病毒诱导。在仙台病毒感染之前用rIFN-alpha 2预处理U937细胞可以提高IFN-alpha 1,IFN-alpha 2和IFN-beta的mRNA水平以及生物活性IFN的最终产量。通过电泳迁移率迁移分析对核蛋白-IFN启动子DNA相互作用的分析表明,尽管未发现新的诱导特异性复合物,但因子与IFN-α1和IFN-β调节域的结合增加。根据竞争电泳迁移率变动分析结果,与IFN-alpha 1和IFN-beta启动子相互作用的因子似乎是不同的DNA结合蛋白。 U937因子结合定位于IFN-β调节元件的P2域(-64至-55),该序列基序与转录因子NF-κB的识别位点具有80%的同源性。IFN中的蛋白质-DNA相互作用实际上,β-P2结构域被过量的同源P2片段或包含两个重复的NF-κB识别位点的人类免疫缺陷病毒增强子元件特异性竞争。分别分析了与猿猴病毒40启动子相连的,包含IFN-β调控元件或人免疫缺陷病毒增强子元件的杂种启动子-氯霉素乙酰转移酶融合质粒的病毒和佛波酯可诱导性。在293细胞系中,两个质粒都组成性表达,但不能被病毒诱导,而在Jurkat细胞中,这些质粒的氯霉素乙酰转移酶活性是通过肿瘤促进剂处理诱导的。这些实验表明,可以通过与IFN-β启动子内的NF-κB样位点结合的转录调节蛋白来部分控制IFN基因表达的诱导。

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