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首页> 外文期刊>Mutation Research: International Journal on Mutagenesis, Chromosome Breakage and Related Subjects >Tandemly repeated DNA sequence instabilities induced by two promoters of morphological transformation in vitro: a short-term response to non-mutagenic agents in C3H/10T1/2 cells.
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Tandemly repeated DNA sequence instabilities induced by two promoters of morphological transformation in vitro: a short-term response to non-mutagenic agents in C3H/10T1/2 cells.

机译:由体外形态转化的两个启动子诱导的串联重复DNA序列不稳定性:对C3H / 10T1 / 2细胞中非诱变剂的短期响应。

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The ability of tumour promoters to alter DNA stability within regions that contain tandemly repeated sequences (TRSs), was studied in a cell culture model of multi-stage carcinogenesis. Non-cytotoxic concentrations of TPA (12-O-tetradecanoyl-phorbol-13-acetate) and xanthine oxidase with xanthine substrate, sufficient to promote morphological transformation in C3H/10T1/2 cultures, were tested for their effects on mutation frequencies in TRSs by a DNA fingerprinting approach. Specifically, restriction digests of genomic DNA samples from randomly selected, non-transformed clones, isolated from cultures after several days exposure to promoters, were visualized by Southern hybridizations with the multi-locus pentamer repeat sequence probe, Ms6-Hm (Pc-1). Basal and promoter-induced frequencies of sub-clone TRS fingerprint polymorphisms were estimated in five cell populations: an uncloned stock culture, three populations established from normal-appearing sub-clones, and one clonal population established from a 3-methylcholanthrene (MCA)-transformed focus. Basal variant fingerprint frequencies spanned a range from 0.0 to 0.43% mutants/band among cells from the four untransformed populations. Both TPA and xanthine oxidase treatments significantly increased recorded mutation frequencies, 2.3- and 2.7-fold, respectively, using combined data from the progenitor population and three untransformed clones. The untreated MCA-transformed clonal population appeared to contain a single, pre-existing mutant restriction fragment, but additional mutations were induced thereafter, in response to the promoting treatments. Taken together, the measured increases in mutations were highly significant and suggest that promoters of cell transformation in the C3H/10T1/2 cell line might induce a genome-wide instability targeted to regions containing Ms6-Hm sequence motifs.
机译:在多阶段致癌的细胞培养模型中研究了肿瘤启动子改变含有串联重复序列(TRS)的区域内DNA稳定性的能力。测试了TPA(12-O-十四烷酰基-phorbol-13-乙酸盐)和黄嘌呤氧化酶与黄嘌呤底物的无细胞毒性浓度,足以促进C3H / 10T1 / 2培养物中的形态转化,通过以下方法测试了它们对TRSs突变频率的影响: DNA指纹图谱方法。具体而言,通过与多位点五聚体重复序列探针Ms6-Hm(Pc-1)进行Southern杂交,可以观察到随机暴露于启动子后数天从培养物中分离而来的随机选择,未转化克隆的基因组DNA样品的限制性消化。 。在5个细胞群体中估计了基础和启动子诱导的亚克隆TRS指纹多态性的频率:未克隆的原种培养,从正常出现的亚克隆建立的3个群体和从3-甲基胆甾醇(MCA)建立的一个克隆群体-焦点转移。在四个未转化种群的细胞中,基础变异指纹频率范围为0.0-0.43%突变体/条带。使用祖细胞和三个未转化克隆的组合数据,TPA和黄嘌呤氧化酶处理均显着提高了记录的突变频率,分别为2.3倍和2.7倍。未经处理的MCA转化克隆种群似乎包含单个预先存在的突变限制片段,但此后,根据促进治疗,诱导了其他突变。综上所述,所测得的突变增加非常显着,表明C3H / 10T1 / 2细胞系中细胞转化的启动子可能诱导针对包含Ms6-Hm序列基序区域的全基因组不稳定性。

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