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Novel transcriptional regulation of the schlafen-2 gene in macrophages in response to TLR-triggered stimulation.

机译:响应TLR触发的刺激,巨噬细胞中schlafen-2基因的新型转录调控。

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Schlafen-2 (slfn-2) is a member of slfn family, regulators of T cell development and its expression is altered during infection by microbial pathogens. However, the molecular mechanism involved in slfn expression is still to be determined. In this study, we isolated slfn-2 as a LPS-induced differentially expressed genes (DEGs) in RAW 264.7 cells and examined expression and regulation of slfn-2 in CpG-DNA-treated and LPS-treated macrophages. We defined a transcriptional start site in the slfn-2 gene. To examine the promoter organization of the slfn-2 gene, we cloned a approximately 1.8 kb region upstream of the transcription start site. Sequence analysis indicates consensus sites for AP-1 and NF-kappaB. Comprehensive mutant analyses, ELISA-based transcription factor activation assay, and ChIP assays reveal that functional interaction of AP-1 and NF-kappaB with the promoter element is necessary for the Toll-like receptor (TLR)-mediated slfn-2 gene expression by CpG-DNA and LPS treatment in macrophages. In summary, we identified a slfn-2 promoter for the first time and demonstrated that CpG-DNA and LPS triggers slfn-2 gene expression by activating NF-kappaB and AP-1 pathways in macrophages.
机译:Schlafen-2(slfn-2)是slfn家族的成员,是T细胞发育的调节剂,其表达在微生物病原体感染期间会发生改变。但是,涉及slfn表达的分子机制尚待确定。在这项研究中,我们分离了slfn-2作为LPS诱导的RAW 264.7细胞中的差异表达基因(DEG),并检查了slfn-2在CpG-DNA处理和LPS处理的巨噬细胞中的表达和调控。我们在slfn-2基因中定义了一个转录起始位点。为了检查slfn-2基因的启动子组织,我们在转录起始位点上游克隆了一个大约1.8 kb的区域。序列分析表明AP-1和NF-κB的共有位点。全面的突变分析,基于ELISA的转录因子激活分析和ChIP分析表明,AP-1和NF-κB与启动子的功能相互作用对于Toll样受体(TLR)介导的slfn-2基因表达是必需的。巨噬细胞中的CpG-DNA和LPS处理。总之,我们首次鉴定了slfn-2启动子,并证明CpG-DNA和LPS通过激活巨噬细胞中的NF-κB和AP-1途径触发slfn-2基因表达。

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