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A biosensor for environmental genotoxin screening based on an SOS lux assay in recombinant Escherichia coli cells.

机译:基于SOS lux检测重组大肠杆菌细胞中环境遗传毒素的生物传感器。

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A genetically controlled luminescent bacterial reporter assay, the SOS lux test, was developed for rapid detection of environmental genotoxins. The bioassay is based on the recombinant plasmid pPLS-1, which was constructed as a derivative of pBR322, carrying the promoterless luxCDABFE genes of Photobacterium leiognathi downstream of a truncated cda gene from ColD with a strong SOS promoter. E. coli recA+ strains containing this construction are inducible to high levels of light production in the presence of substances or agents that cause damage to the DNA of the cells. The light signal, reflecting the SOS-inducing potency, is recorded from the growing culture within 1 s, and the test results are available within 1 to 2 h. Induction of bioluminescence was demonstrated by treatment of E. coli C600(pPLS-1) with 6 genotoxic chemicals (mitomycin C, N-methyl-N'-nitro-N-nitrosoguanidine, nalidixic acid, dimethylsulfate, hydrogen peroxide, and formaldehyde) and with UV and gamma radiation. A clear dose-response relationship was established for all eight genotoxins. The sensitivity of the SOS lux test is similar to that of other bioassays for genotoxicity or mutagenicity, such as the SOS chromotest, umu test, and Ames mutatest. These results indicate that the SOS lux test is potentially useful for the in situ and continuous detection of genotoxins.
机译:开发了一种遗传控制的发光细菌报告基因测定法(SOS lux试验),用于快速检测环境基因毒素。该生物测定法基于重组质粒pPLS-1,该质粒被构建为pBR322的衍生物,在来自ColD的截短cda基因下游的携带强SOS启动子的下游截短的cda基因中携带了无尾细菌的luxCDABFE基因。含有这种结构的大肠杆菌recA +菌株在存在会损坏细胞DNA的物质或试剂的情况下,可诱导大量发光。反映SOS诱导潜能的光信号在1 s内从生长的培养物中记录下来,测试结果在1-2 h内可用。用6种遗传毒性化学物质(丝裂霉素C,N-甲基-N'-硝基-N-亚硝基胍,萘啶酸,二甲基硫酸盐,过氧化氢和甲醛)处理大肠杆菌C600(pPLS-1)证明了生物发光的诱导。具有紫外线和伽玛射线。对于所有八种基因毒素,建立了明确的剂量反应关系。 SOS lux检测的灵敏度与其他生物测定的遗传毒性或诱变灵敏度相似,例如SOS色度测试,umu测试和Ames突变测试。这些结果表明,SOS lux检测对于基因毒素的原位和连续检测潜在有用。

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