摘要
本研究用电穿孔法将带有邻苯二酚氧化酶基因(xY1E基因)的质粒pESnx转染至5种哺乳动物细胞(FL,HT,LTR,PA317和Wg3-h)。结果表明,质粒pESnx在5种细胞中均可形成抗性克隆。但是,仅pESnx/FL克隆可获得每皿50个以上的转化子和低于10-4的自发突变率,符合穿梭质粒测试系统的要求。为进一步验证可用于检测致突变性,用已知可诱发点突变的致癌物亚硝基胍(MNNG)处理pESnx/FL克隆细胞。结果表明,MNNG的诱发突变率高于自发突变率27.8倍,并有剂量-效应关系。突变子快速鉴定结果显示,质粒稳定地存在于突变子中,并无大片段缺失和分子量改变,证实MNNG诱变的是点突变。
In this study, plasmid pESnx with xY1E gene(catecholgene)were transfected into 5 kinds of mammalian cells(FL, HT, LTR, PA317,and Wg3-h)by electroporation. Results showed that plasmid pESnx could form resistant colonies in all of the five mammalian cells, but transformants could be produced more than 50/amp plate in pESnx/FL only when it was transfected into MC1061F'Kan. The spontaneous mutation frequency was less than 10-4 in pESnx/FL. Therefore, pESnx/FL accord with the requirements of shuttle vector plasmid mutation test system. In order to further confirm that pESnx/FL could be utilized for detection of mutagenicity, a known mutagen MNNG which could induce point mutation was used to treat pESnx/FL colonies. Results showed that the mutation frequency induced by MNNG was 27.8 folds higher than that of the spontaneous mutation frequency and had dose-effect dependent. The mutants were identified by Cracking gel rapid extraction. Results revealed that the shuttle vector was stable, there was no large deletion of DNA and change of molecular weight, and it was verified that mutation induced by MNNG was a point mutation.
出处
《第二军医大学学报》
CAS
CSCD
北大核心
1994年第4期318-322,共5页
Academic Journal of Second Military Medical University
基金
国家自然科学基金
关键词
邻苯二酚
氧化酶
基因
致突变
质粒
xY1E gene
shuttle vector plasmid
mutation
test system
