Nivard M J, Pastink A, Vogel E W
MGC-Department of Radiation Genetics and Chemical Mutagenesis, Leiden University, Sylvius Laboratories, Netherlands.
Mutat Res. 1996 Jun 10;352(1-2):97-115. doi: 10.1016/0027-5107(96)00011-5.
This paper describes the analysis of mutations induced at the vermilion locus in postmeiotic male germ cell stages of Drosophila exposed to 3 different N-methyl-N-nitroso compounds: N-methyl-N-nitrosourea (MNU); N-methyl-N'-nitro-N-nitrosoguanidine (MNNG); and N-nitrosodimethylamine (DMN). With MNU and DMN, the impact of DNA nucleotide excision repair (NER) on the spectra of mutations was studied. Mutants were isolated from F1 (mutations fixed before the first mitotic replication after fertilization) and F2 (mutations fixed following one or more mitotic replications; mosaics in F1) generations. The vermilion system enables the analysis of both intra- and inter-locus DNA changes for which several techniques have been adapted: (1) amplification of the vermilion gene by PCR, cloning of the fragment and sequence analysis of ssDNA; (2) Southern blot hybridization; and (3) cytological analysis of polytene chromosomes. In total, 49 MNU (26 from the exr+ genotype and 23 from the exr- genotype), 47 DMN (28 from the exr+ genotype and 19 from the exr- genotype) and 16 MNNG-induced mutations were characterized. The F1 spectra of all 3 agents contained base-pair changes and deletions (intra- and multi-locus) in a ratio of roughly 1 to 1, indicating a significant contribution of nitrogen DNA adducts to the spectra. In all F2 spectra the levels of base-pair changes were significantly higher compared to those in the F1 spectra, a finding also made for methyl methanesulfonate-induced mutations in earlier studies. There is an increase of mutations of, especially, the transversion types of mutations under exr- conditions in comparison to the exr+ situation. The induced transversions, clearly present in all spectra (exr+ and exr-), are presumably caused by N-methyl DNA adducts, which upon release from the DNA backbone lead to apurinic sites in a time-related process. Regarding the occurrence of transitions, it turned out for all 3 mutagens that the AT-->GC type strongly dominated the GC-->AT transitions. This suggest that O6-methylguanine is efficiently repaired, in contrast to O4-methylthymine. Based on the data obtained in the vermilion system with ENU, we propose, in addition, that the Drosophila alkyltransferase system repairs O6-methylguanine more efficiently than O6-ethylguanine.
本文描述了对暴露于3种不同的N-甲基-N-亚硝基化合物的果蝇减数分裂后雄性生殖细胞阶段朱砂位点诱导突变的分析:N-甲基-N-亚硝基脲(MNU);N-甲基-N'-硝基-N-亚硝基胍(MNNG);以及N-亚硝基二甲胺(DMN)。对于MNU和DMN,研究了DNA核苷酸切除修复(NER)对突变谱的影响。从F1代(受精后第一次有丝分裂复制前固定的突变)和F2代(一次或多次有丝分裂复制后固定的突变;F1代中的嵌合体)中分离出突变体。朱砂系统能够分析位点内和位点间的DNA变化,为此采用了几种技术:(1)通过PCR扩增朱砂基因,克隆片段并对单链DNA进行序列分析;(2)Southern印迹杂交;(3)多线染色体的细胞学分析。总共对49个MNU诱导的突变(26个来自exr+基因型,23个来自exr-基因型)、47个DMN诱导的突变(28个来自exr+基因型,19个来自exr-基因型)和16个MNNG诱导的突变进行了表征。所有3种试剂的F1突变谱中碱基对变化和缺失(位点内和多位点)的比例大致为1:1,表明氮DNA加合物对突变谱有显著贡献。在所有F2突变谱中,碱基对变化的水平与F1突变谱相比显著更高,这一发现也在早期研究中对甲磺酸甲酯诱导的突变中得到。与exr+情况相比,在exr-条件下,尤其是颠换类型的突变有所增加。所有谱(exr+和exr-)中明显存在的诱导颠换可能是由N-甲基DNA加合物引起的,这些加合物从DNA主链释放后会在一个与时间相关的过程中导致脱嘌呤位点。关于转换的发生,结果表明所有3种诱变剂中,AT→GC类型强烈主导GC→AT转换。这表明与O4-甲基胸腺嘧啶相反,O6-甲基鸟嘌呤能被有效修复。此外,基于在朱砂系统中用ENU获得的数据,我们提出果蝇烷基转移酶系统修复O6-甲基鸟嘌呤比修复O'6-乙基鸟嘌呤更有效。
