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艾姆斯试验从微量滴定板转移至平面检测形式。

Ames Assay Transferred from the Microtiter Plate to the Planar Assay Format.

作者信息

Schmidtmann Katharina, Lemme Johanna, Morlock Gertrud E

机构信息

Chair of Food Science, Institute of Nutritional Science, Justus Liebig University Giessen, Heinrich-Buff-Ring 26-32, 35392 Giessen, Germany.

出版信息

J Xenobiot. 2025 May 7;15(3):67. doi: 10.3390/jox15030067.

Abstract

The International Agency for Research on Cancer has studied and classified 1045 potential substances. It is therefore important to develop rapid screening methods to identify the mutagenicity of compounds and, further on, the intensity and number of individual mutagenic substances in complex sample mixtures. The current in vitro Ames assay in the microtiter plate format (MPF) uses a pH-sensitive detection as endpoint, however, acidic substances in complex mixtures may interfere the mutagenicity result. Hence, it was transferred to the planar assay format to be more selective for complex mixture testing. The co-culture of Typhimurium strains TA98 and TA100 with an optical density of 0.4 at 600 nm was applied on a high-performance thin-layer chromatography silica gel 60 chromatogram and on-surface incubated for 5 h, which period was limited due to zone diffusion. Various positive controls were tested, and 4-nitrochinolin--oxide with a limit of detection of 100 ng was established as a positive control. However, due to the shorter incubation time, no mutagenic compounds were detectable or differentiable in the tested perfumes, herbal teas, margarines, and hand creams. This does not mean that the samples are mutagen-free, but it suggests that further improvements to the bioassay are urgently needed to increase the sensitivity and selectivity of the response. Compared to conventional sum value assays, a planar Ames assay performed on the separated and adsorbed sample components advances toxicology research because mutagenic compounds are separated from interfering molecules due to the integrated separation. It thus would provide a more selective detection of mutagens in complex mixtures and allow testing of large sample volumes or concentrated samples without matrix interference.

摘要

国际癌症研究机构已对1045种潜在物质进行了研究和分类。因此,开发快速筛选方法以鉴定化合物的致突变性,并进一步确定复杂样品混合物中单个诱变物质的强度和数量非常重要。当前微孔板形式(MPF)的体外艾姆斯试验使用pH敏感检测作为终点,然而,复杂混合物中的酸性物质可能会干扰致突变性结果。因此,将其转换为平面试验形式,以便对复杂混合物测试更具选择性。将在600nm处光密度为0.4的鼠伤寒沙门氏菌TA98和TA100菌株共培养物应用于高效薄层色谱硅胶60色谱图上,并在表面孵育5小时,由于区域扩散,该时间段受到限制。测试了各种阳性对照,并确定检测限为100ng的4-硝基喹啉-N-氧化物作为阳性对照。然而,由于孵育时间较短,在所测试的香水、花草茶、人造黄油和护手霜中未检测到或区分出诱变化合物。这并不意味着样品无诱变作用,但表明迫切需要对生物测定进行进一步改进,以提高响应的灵敏度和选择性。与传统的总和值测定相比,对分离和吸附的样品成分进行的平面艾姆斯试验推动了毒理学研究,因为由于集成分离,诱变化合物与干扰分子分离。因此,它将对复杂混合物中的诱变剂进行更具选择性的检测,并允许在无基质干扰的情况下测试大量样品或浓缩样品。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5378/12101383/86c82c8b8f5f/jox-15-00067-g001.jpg

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