DNA fingerprint analysis in chemically mutagenized Chinese hamster lung cells

Tsukasa Kikuno , Masamitsu Honma , Syozo Ogura , Hiroshi Mizusawa , Makoto Hayashi , Toshio Sofuni
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引用次数: 6

Abstract

Using a multi locus minisatellite Per-6 DNA probe, we performed DNA fingerprint analysis. Chinese hamster lung (CHL) cells were treated with six model chemicals: N-methyl-N′-nitro-N-nitrosoguanidine, mitomycin C, methyl methanesulfonate, furylfuramide, 2-acetylamino-fluorene, and cyclophosphamide, with or without S9 mix. 771 hypoxanthine phosphoribosyltransferase deficient clones (749 from mutagen-treated cells and 22 from untreated cells) and 90 unselected clones from untreated cells were isolated and analyzed. The spontaneous mutation frequency at CHL cell minisatellite loci was 0.31–0.63%. All the chemicals increased mutation frequencies. Almost all mutations localized to the three specific minisatellite loci corresponding to 4.2, 3.8, and 2.4 kb bands, suggesting that these regions are more unstable and susceptible to mutation. DNA fingerprint analysis is a promising technique for detecting mutations at neutral DNA regions, especially recombinational mutations, and may be useful for surveying genetic instability related to heritable defects or aging.

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化学诱变中国仓鼠肺细胞DNA指纹图谱分析
使用多位点微型卫星Per-6 DNA探针,我们进行了DNA指纹分析。采用六种模型化学物质:n -甲基-n ' -硝基-n -亚硝基胍、丝裂霉素C、甲磺酸甲酯、呋喃呋喃酰胺、2-乙酰氨基芴和环磷酰胺,加或不加S9混合物处理中国仓鼠肺(CHL)细胞。共分离并分析了771个次黄嘌呤磷酸核糖基转移酶缺陷克隆(749个来自诱变剂处理的细胞,22个来自未处理的细胞)和90个来自未处理细胞的未选择克隆。CHL细胞微卫星位点的自发突变频率为0.31 ~ 0.63%。所有的化学物质都增加了突变的频率。几乎所有的突变都集中在对应于4.2、3.8和2.4 kb波段的三个特定的小卫星位点上,这表明这些区域更不稳定,更容易发生突变。DNA指纹分析是一种很有前途的技术,用于检测中性DNA区域的突变,特别是重组突变,并可用于研究与遗传缺陷或衰老相关的遗传不稳定性。
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