Kohler S W, Provost G S, Fieck A, Kretz P L, Bullock W O, Sorge J A, Putman D L, Short J M
Stratagene, La Jolla, CA 92037.
Proc Natl Acad Sci U S A. 1991 Sep 15;88(18):7958-62. doi: 10.1073/pnas.88.18.7958.
Transgenic mice with a lambda shuttle vector containing a lacI target gene were generated for use as a short-term, in vivo mutagenesis assay. The gene is recovered from the treated mice by exposing mouse genomic DNA to in vitro packaging extracts and plating the rescued phage on agar plates containing 5-bromo-4-chloro-3-indolyl beta-D-galactopyranoside (X-Gal). Phage with mutations in the lacI gene form blue plaques, whereas phage with a nonmutated lacI form colorless plaques. Spontaneous background mutant rates using this system range from 0.6 x 10(-5) to 1.7 x 10(-5), depending upon tissue analyzed, with germ cells exhibiting less than one-third the background rate of somatic tissue. Treatment of the mice with N-ethyl-N-nitrosourea (EtNU), benzo[a]pyrene (B[a]P), or cyclophosphamide caused an induction of mutations over background. Recovery of the lacI target for sequence analysis was performed by genetic excision of a plasmid from the phage using partial filamentous phage origins. The predominant mutations identified from untreated and treated populations were base substitutions. Although it has been shown by others that 70% of all spontaneous mutations within the lacI gene, when replicated in Escherichia coli, occur at a hot spot located at bases 620-632, only 1 of 21 spontaneous mutations has been identified in this region in the transgenic mouse system. In addition, 5 of 9 spontaneous transitions analyzed occur at CpG dinucleotides, whereas no transition mutations were identified at the prokaryotic deamination hot spots occurring at dcm sites (CCA/TGG) within the lacI gene. For EtNU, approximately equal amounts of transitions and transversions were observed, contrasting with B[a]P-induced mutations, in which only transversions were obtained. In addition, B[a]P mutagenesis showed a predominance of mutations (81%) involving cytosines and/or guanines, consistent with its known mode of action. The discovery of a spontaneous mutation spectrum different from that of bacterial assays, coupled with the concordance of EtNU and B[a]P base mutations with the known mechanisms of activity for these mutagens, suggests that this transgenic system will be useful as a short-term, in vivo system for mutagen assessment and analysis of mechanisms leading to mutations.
构建了带有含lacl靶基因的λ穿梭载体的转基因小鼠,用于短期体内诱变分析。通过将小鼠基因组DNA暴露于体外包装提取物,并将拯救的噬菌体接种在含有5-溴-4-氯-3-吲哚基-β-D-吡喃半乳糖苷(X-Gal)的琼脂平板上,从处理过的小鼠中回收该基因。lacl基因发生突变的噬菌体形成蓝色噬菌斑,而lacl基因未发生突变的噬菌体形成无色噬菌斑。使用该系统的自发背景突变率在0.6×10⁻⁵至1.7×10⁻⁵之间,具体取决于所分析的组织,生殖细胞的背景率不到体细胞组织的三分之一。用N-乙基-N-亚硝基脲(EtNU)、苯并[a]芘(B[a]P)或环磷酰胺处理小鼠会导致在背景基础上诱导突变。通过使用部分丝状噬菌体起源从噬菌体中对质粒进行基因切除,来回收用于序列分析的lacl靶标。从未处理和处理群体中鉴定出的主要突变是碱基替换。尽管其他人已经表明,lacl基因内所有自发突变的70%在大肠杆菌中复制时发生在位于620-632位碱基的热点处,但在转基因小鼠系统的该区域中仅鉴定出21个自发突变中的1个。此外,所分析的9个自发转换中有5个发生在CpG二核苷酸处,而在lacl基因内dcm位点(CCA/TGG)处的原核脱氨热点未鉴定到转换突变。对于EtNU,观察到转换和颠换的数量大致相等,这与B[a]P诱导的突变形成对比,在B[a]P诱导的突变中仅获得了颠换。此外,B[a]P诱变显示涉及胞嘧啶和/或鸟嘌呤的突变占主导(81%),与其已知的作用模式一致。自发突变谱与细菌分析不同,再加上EtNU和B[a]P碱基突变与这些诱变剂已知的活性机制一致,这表明该转基因系统将作为一种短期体内系统,用于诱变评估和导致突变的机制分析。
