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Detection of gentoxicity of benzidine and its derivatives with the Escherichia coli DJ 702 lacZ reversion mutagenicity assay

机译:用大肠杆菌DJ 702 lacZ反向诱变试验检测联苯胺及其衍生物的遗传毒性

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AIMS: The feasibility of Escherichia coli DJ 702 lacZ mutagenicity assay to detect genotoxicity of benzidine and its derivatives was evaluated. METHODS AND RESULTS: DJ 702 strain was grown overnight at 30 degrees C in Luria-Bertani (LB) medium containing some components, such as chloramphenicol, ampicillin, delta-aminolevulinic acid, isopropyl-beta-d-thiogalactoside, and trace element mix. The mixtures of a bacterial culture and tested chemical at indicated doses were incubated at 30 degrees C for 30 min. Subsequently, 2 ml of molten top agar was added and the resulting mixtures were immediately poured onto a minimal lactose (ML) plate. Plates were incubated at 30 degrees C for 48 h. The number of colonies was determined by visual scoring. In this study, results showed that all the tested chemicals were mutagenic to DJ 702 strain. CONCLUSIONS: E. coli lac mutagenicity assay using DJ 702 strain can detect the mutagenicity of benzidine and its derivatives. SIGNIFICANCE AND IMPACT OF THE STUDY: We detected the mutagenicity of benzidine and its derivatives in E. coli lac mutagenicity assay using DJ 702, indicating that this assay may be used to detect benzidine and its derivatives in a powerful, sensitive, and convenient mutagenesis assay.
机译:目的:评价了大肠杆菌DJ 702 lacZ诱变试验检测联苯胺及其衍生物的遗传毒性的可行性。方法和结果:DJ 702菌株在30摄氏度的Luria-Bertani(LB)培养基中生长过夜,该培养基含有一些成分,例如氯霉素,氨苄青霉素,δ-氨基乙酰丙酸,异丙基-β-d-硫代半乳糖苷和微量元素混合物。将指示剂量的细菌培养物和受试化学品的混合物在30摄氏度下孵育30分钟。随后,加入2 ml熔融的顶部琼脂,并将所得混合物立即倒入最小乳糖(ML)板上。将板在30℃下孵育48小时。通过视觉评分确定菌落数。在这项研究中,结果表明所有测试的化学品均对DJ 702菌株具有致突变性。结论:使用DJ 702菌株进行大肠杆菌lac致突变性测定可检测联苯胺及其衍生物的致突变性。研究的意义和影响:我们使用DJ 702在大肠杆菌lac致突变性检测中检测到联苯胺及其衍生物的致突变性,表明该检测法可用于在功能强大,灵敏且方便的诱变检测中检测联苯胺及其衍生物。

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