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首页> 外文期刊>Analytica chimica acta >Increased sensitivity of the SOS-LUX-Test for the detection of hydrophobic genotoxic substances with Salmonella typhimurium TA 1535 as host strain
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Increased sensitivity of the SOS-LUX-Test for the detection of hydrophobic genotoxic substances with Salmonella typhimurium TA 1535 as host strain

机译:以鼠伤寒沙门氏菌TA 1535为宿主菌株的SOS-LUX-Test检测疏水性遗传毒性物质的灵敏度更高

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摘要

The SOS-LUX- Test is a simple and fast prokaryotic bioassay for the detection and quantification of genotoxic substances by the measurement of the DNA-damage proportional intensity of bioluminescence. This bioluminescence is produced by bacteria carrying the plasmid pPLS-I with a lux operon under the control of a SOS promoter. In previous experiments different Escherichia coli strains have been used as host bacteria. Depending on the degree of hydrophobicity of the genotoxic substances the sensitivity of the SOS-LUX- Test was lower than measured in other bacterial bioassays for genotoxicity. An initial improvement could be made by using the E. coli strain PB3 with a tolC mutation causing an increased cell membrane penneability for hydrophobic substances compared to a tol wild-type strain. The change of the bacterial species from E. coli to a Salmonella typhimurium strain with a defect in the synthesis of the outer cell membrane (rIa-, strain TA1535) has led to a further increase in sensitivity. After a minor adaptation and modification of the experimental procedure the results obtained with both strains were compared for the test substances NFO, ICR 191, MMC, NQO, NA, AA, 2-AF, B(a)P. With hydrophobic substances the sensitivity of TA1535(pPLS-1) is higher than that of PB3(pPLS-1). This is correlated in most cases with a higher toxicity, whereas the sensitivity for water-soluble substances is not significantly increased, as expected. From these results we decided to use the strain S. typhimurium (also called S. choleraesuis ssp. choleraesuis) TA1535(pPLS-I) in the SOS-LUX- Test in future genotoxicity tests.
机译:SOS-LUX-Test是一种简单快速的原核生物测定法,可通过测量生物发光的DNA损伤比例强度来检测和定量遗传毒性物质。这种生物发光是由在SOS启动子控制下携带带有lux操纵子的质粒pPLS-1的细菌产生的。在先前的实验中,已将不同的大肠杆菌菌株用作宿主细菌。根据遗传毒性物质的疏水性程度,SOS-LUX-Test的灵敏度低于遗传毒性其他细菌生物测定法中测得的灵敏度。与tol野生型菌株相比,使用具有tolC突变的大肠埃希氏菌PB3可以引起疏水性物质的细胞膜渗透性增加,从而初步改善。细菌种类从大肠杆菌到鼠伤寒沙门氏菌菌株的改变(在外细胞膜的合成中存在缺陷)(rIa-,菌株TA1535)导致敏感性进一步提高。在对实验程序进行较小的修改和修改后,比较了两种菌株获得的测试物NFO,ICR 191,MMC,NQO,NA,AA,2-AF,B(a)P的结果。对于疏水性物质,TA1535(pPLS-1)的灵敏度高于PB3(pPLS-1)。在大多数情况下,这与较高的毒性相关,而对水溶性物质的敏感性并未如预期的那样显着提高。根据这些结果,我们决定在未来的基因毒性测试中,将S. typhimurium(也称为霍乱沙门氏菌s。choleraesuis)TA1535(pPLS-1)用于SOS-LUX-Test中。

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