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首页> 外文期刊>Oncology reports >Curcumin alters gene expression-associated DNA damage, cell cycle, cell survival and cell migration and invasion in NCI-H460 human lung cancer cells in vitro
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Curcumin alters gene expression-associated DNA damage, cell cycle, cell survival and cell migration and invasion in NCI-H460 human lung cancer cells in vitro

机译:姜黄素在体外改变NCI-H460人肺癌细胞中与基因表达相关的DNA损伤,细胞周期,细胞存活以及细胞迁移和侵袭

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Lung cancer is the most common cause of cancer mortality and new cases are on the increase worldwide. However, the treatment of lung cancer remains unsatisfactory. Curcumin has been shown to induce cell death in many human cancer cells, including human lung cancer cells. However, the effects of curcumin on genetic mechanisms associated with these actions remain unclear. Curcumin (2 mu M) was added to NCI-H460 human lung cancer cells and the cells were incubated for 24 h. Total RNA was extracted from isolated cells for cDNA synthesis, labeling, microarray hybridization and flour-labeled cDNA hybridized on chip. Localized concentrations of fluorescent molecules were detected and quantified using Expression Console software (Affymetrix) with default RMA parameters. GeneGo software was used for the key genes involved and their possible interaction pathways. The results showed that similar to 170 genes were significantly upregulated and 577 genes were significantly downregulated in curcumin-treated cells. Specifically, the up- and downregulated genes included CCNE2, associated with DNA damage; ID3, associated with cell survival and 146 genes with a >2- to 3-fold change including the TP53INP1 gene, associated with DNA damage; CDC6, CDCA5,TAKMIP2, CDK14, CDK5,CDCA76, CDC25A, CDC5L and SKP2, associated with cell cycle; the CARD6, ID1 and ID2 genes, associated with cell survival and the BRMSIL, associated with cell migration and invasion. Additionally, 59 downregulated genes exhibited a >4-fold change, including the DDIT3 gene, associated with DNA damage; while 97 genes had a >3- to 4-fold change including the DDIT4 gene, associated with DNA damage; the CCPGI gene, associated with cell cycle and 321 genes with a >2- to 3-fold including the GADD45A and CGREFI genes, associated with DNA damage; the CCPGI gene, associated with cell cycle, the TNFRSFIOB, GASS, TSSCI and TNFRSF11B gene, associated with cell survival and the ARHAP29 and CADM2 genes, associated with cell migration and invasion. In conclusion, gene alterations provide information regarding the cytotoxic mechanism of curcumin at the genetic level and provide additional biomarkers or targets for the treatment of human lung cancer.
机译:肺癌是导致癌症死亡的最常见原因,全球范围内新病例的增加。但是,肺癌的治疗仍然不能令人满意。姜黄素已显示出在许多人类癌细胞(包括人类肺癌细胞)中诱导细胞死亡。然而,姜黄素对与这些作用有关的遗传机制的影响尚不清楚。将姜黄素(2μM)添加到NCI-H460人肺癌细胞中,并将细胞孵育24小时。从分离的细胞中提取总RNA,用于cDNA合成,标记,微阵列杂交和在面粉上杂交的面粉标记cDNA。使用Expression Console软件(Affymetrix)使用默认RMA参数检测并定量荧光分子的局部浓度。 GeneGo软件用于涉及的关键基因及其可能的相互作用途径。结果显示,在姜黄素处理的细胞中,大约有170个基因被显着上调,而577个基因被显着下调。具体而言,上调和下调的基因包括CCNE2,与DNA损伤相关;与细胞存活有关的ID3和146种具有> 2至3倍变化的基因,包括TP53INP1基因,与DNA损伤有关;与细胞周期有关的CDC6,CDCA5,TAKMIP2,CDK14,CDK5,CDCA76,CDC25A,CDC5L和SKP2;与细胞存活相关的CARD6,ID1和ID2基因以及与细胞迁移和侵袭相关的BRMSIL。此外,59个下调的基因表现出> 4倍的变化,其中包括DDIT3基因,与DNA损伤有关。而97个基因(包括DDIT4基因)的变化是3到4倍,与DNA损伤有关;与细胞周期有关的CCPGI基因和与DNA损伤有关的321个基因,其中GADD45A和CGREFI基因的影响是2-3倍,其中包括GADD45A和CGREFI。与细胞周期有关的CCPGI基因,与细胞存活有关的TNFRSFIOB,GASS,TSSCI和TNFRSF11B基因以及与细胞迁移和侵袭有关的ARHAP29和CADM2基因。总之,基因改变在遗传水平上提供了有关姜黄素细胞毒性机制的信息,并为治疗人类肺癌提供了其他生物标志物或靶标。

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