H Takano, T Ise, M Nomoto, K Kato, T Murakami, H Ohmori, T Imamura, G Nagatani, T Okamoto, R Ohta, M Furukawa, K Shibao, H Izumi, M Kuwano, K Kohno
{"title":"耐药细胞中人类DNA拓扑异构酶ⅱα基因控制区的结构和功能分析。","authors":"H Takano, T Ise, M Nomoto, K Kato, T Murakami, H Ohmori, T Imamura, G Nagatani, T Okamoto, R Ohta, M Furukawa, K Shibao, H Izumi, M Kuwano, K Kohno","doi":"","DOIUrl":null,"url":null,"abstract":"<p><p>We have previously shown that the DNA topoisomerase II alpha (topo II alpha) gene is down-regulated in VP16/VM26-resistant cells at the transcriptional level. To determine the DNA elements responsible for down-regulation, the transcriptional activities of luciferase reporter constructs containing various lengths of the promoter sequences were investigated by transient transfection of two resistant cell lines, KB/VP2 and KB/VM4. The transcriptional activities of the full-length promoter (-295 to +85) and of three deletion constructs (-197, -154 and -74 to +85) were significantly down-regulated in resistant cells. In contrast, the transcriptional activity of the minimal promoter (-20 to +85) in resistant cells was similar to that in parental KB cells. Furthermore, introduction of a mutation in ICE1 abolished the down-regulation of the topo II alpha promoter activity in drug-resistant cells. In vivo footprinting analysis of topo II alpha gene promoter revealed several specific protein-binding sites, a GC box, ICE1, ICE2 and ICE3. In vivo footprinting analysis also identified a cluster of hypersensitive sites. However, there was no marked difference in protein-binding sites between parental and resistant cells. To confirm our previous results, we have established the VP16-resistant cell lines T12-VP1 and T12-VP2 from T12 cells derived from human bladder cancer T24 cells stably transfected with the chloramphenicol acetyltransferase reporter gene driven by the topo II alpha gene promoter. The expression to topo II alpha was down-regulated in both cell lines. We also found that CAT gene expression was significantly decreased to one-fifth of that in T12 parental cells. These results suggest that the expression of the topo II alpha gene requires the binding of multiple factors to the core promoter and is down-regulated at the transcriptional level, probably through binding of a negative factor to ICE1 in drug-resistant cells.</p>","PeriodicalId":7927,"journal":{"name":"Anti-cancer drug design","volume":"14 2","pages":"87-92"},"PeriodicalIF":0.0000,"publicationDate":"1999-04-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":"{\"title\":\"Structural and functional analysis of the control region of the human DNA topoisomerase II alpha gene in drug-resistant cells.\",\"authors\":\"H Takano, T Ise, M Nomoto, K Kato, T Murakami, H Ohmori, T Imamura, G Nagatani, T Okamoto, R Ohta, M Furukawa, K Shibao, H Izumi, M Kuwano, K Kohno\",\"doi\":\"\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><p>We have previously shown that the DNA topoisomerase II alpha (topo II alpha) gene is down-regulated in VP16/VM26-resistant cells at the transcriptional level. To determine the DNA elements responsible for down-regulation, the transcriptional activities of luciferase reporter constructs containing various lengths of the promoter sequences were investigated by transient transfection of two resistant cell lines, KB/VP2 and KB/VM4. The transcriptional activities of the full-length promoter (-295 to +85) and of three deletion constructs (-197, -154 and -74 to +85) were significantly down-regulated in resistant cells. In contrast, the transcriptional activity of the minimal promoter (-20 to +85) in resistant cells was similar to that in parental KB cells. Furthermore, introduction of a mutation in ICE1 abolished the down-regulation of the topo II alpha promoter activity in drug-resistant cells. In vivo footprinting analysis of topo II alpha gene promoter revealed several specific protein-binding sites, a GC box, ICE1, ICE2 and ICE3. In vivo footprinting analysis also identified a cluster of hypersensitive sites. However, there was no marked difference in protein-binding sites between parental and resistant cells. To confirm our previous results, we have established the VP16-resistant cell lines T12-VP1 and T12-VP2 from T12 cells derived from human bladder cancer T24 cells stably transfected with the chloramphenicol acetyltransferase reporter gene driven by the topo II alpha gene promoter. The expression to topo II alpha was down-regulated in both cell lines. We also found that CAT gene expression was significantly decreased to one-fifth of that in T12 parental cells. 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引用次数: 0
摘要
我们之前已经证明,在VP16/ vm26抗性细胞中,DNA拓扑异构酶II α (topo II α)基因在转录水平上下调。为了确定负责下调的DNA元件,通过瞬时转染两种抗性细胞系KB/VP2和KB/VM4,研究了含有不同长度启动子序列的荧光素酶报告结构的转录活性。全长启动子(-295至+85)和三个缺失结构(-197、-154和-74至+85)的转录活性在抗性细胞中显著下调。相比之下,抗性细胞中最小启动子(-20至+85)的转录活性与亲本KB细胞相似。此外,ICE1突变的引入消除了耐药细胞中topo II α启动子活性的下调。topo II α基因启动子的体内足迹分析显示了几个特定的蛋白质结合位点,一个GC盒,ICE1, ICE2和ICE3。体内足迹分析也发现了一组超敏感部位。然而,亲本和抗性细胞之间的蛋白结合位点没有显著差异。为了证实我们之前的结果,我们从人类膀胱癌T24细胞中提取的T12细胞中稳定转染了topo II α基因启动子驱动的氯霉素乙酰转移酶报告基因,建立了抗vp16细胞系T12- vp1和T12- vp2。topo II α的表达在两种细胞系中均下调。我们还发现,CAT基因表达量显著降低至T12亲本细胞的五分之一。这些结果表明,topo II α基因的表达需要多个因子与核心启动子结合,并且在转录水平上下调,可能是通过在耐药细胞中将一个负因子与ICE1结合。
Structural and functional analysis of the control region of the human DNA topoisomerase II alpha gene in drug-resistant cells.
We have previously shown that the DNA topoisomerase II alpha (topo II alpha) gene is down-regulated in VP16/VM26-resistant cells at the transcriptional level. To determine the DNA elements responsible for down-regulation, the transcriptional activities of luciferase reporter constructs containing various lengths of the promoter sequences were investigated by transient transfection of two resistant cell lines, KB/VP2 and KB/VM4. The transcriptional activities of the full-length promoter (-295 to +85) and of three deletion constructs (-197, -154 and -74 to +85) were significantly down-regulated in resistant cells. In contrast, the transcriptional activity of the minimal promoter (-20 to +85) in resistant cells was similar to that in parental KB cells. Furthermore, introduction of a mutation in ICE1 abolished the down-regulation of the topo II alpha promoter activity in drug-resistant cells. In vivo footprinting analysis of topo II alpha gene promoter revealed several specific protein-binding sites, a GC box, ICE1, ICE2 and ICE3. In vivo footprinting analysis also identified a cluster of hypersensitive sites. However, there was no marked difference in protein-binding sites between parental and resistant cells. To confirm our previous results, we have established the VP16-resistant cell lines T12-VP1 and T12-VP2 from T12 cells derived from human bladder cancer T24 cells stably transfected with the chloramphenicol acetyltransferase reporter gene driven by the topo II alpha gene promoter. The expression to topo II alpha was down-regulated in both cell lines. We also found that CAT gene expression was significantly decreased to one-fifth of that in T12 parental cells. These results suggest that the expression of the topo II alpha gene requires the binding of multiple factors to the core promoter and is down-regulated at the transcriptional level, probably through binding of a negative factor to ICE1 in drug-resistant cells.
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