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首页> 外文期刊>Toxicological sciences: An official journal of the Society of Toxicology >Development of an exonuclease protection mediated PCR bioassay for sensitive detection of ah receptor agonists.
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Development of an exonuclease protection mediated PCR bioassay for sensitive detection of ah receptor agonists.

机译:核酸外切酶保护介导的PCR生物测定法的开发,用于ah受体激动剂的灵敏检测。

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The aromatic hydrocarbon receptor (AhR) is a ligand-activated transcription factor that mediates many of the biological and toxicological effects of 2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD, dioxin) and related chemicals. Here we developed a novel method to detect the presence of AhR ligands using Exonuclease Protection Mediated PCR bioassay (EPM-PCR). This assay measures the ability of a chemical to activate AhR DNA binding in vitro. In the presence of AhR ligand, an expected length PCR product was observed on electrophoresis, but no signal was detected in the absence of ligand. Real-time quantitative PCR was performed to quantify DNA bound to ligand:AhR complex. We obtained a standard curve with TCDD concentration to bound DNA copies in the range of 0.01 pM-10 nM of TCDD. Minimal detection limit of the assay was below 0.01 pM TCDD, and the whole detection time was less than 5 h. In comparison to the chemical-activated luciferase gene expression (CALUX) bioassay, EPM-PCR bioassay is more sensitive and easier to perform. These results suggest that this assay is useful for detection and quantification of TCDD and related AhR ligands in a cell-free system without the use of radioactivity.
机译:芳香烃受体(AhR)是一种配体激活的转录因子,可介导2,3,7,8-四氯二苯并-对二恶英(TCDD,二恶英)和相关化学物质的许多生物学和毒理作用。在这里,我们开发了一种新颖的方法,可以使用核酸外切酶保护介导的PCR生物测定法(EPM-PCR)检测AhR配体的存在。该测定法测量化学物质在体外激活AhR DNA结合的能力。在AhR配体存在下,电泳时观察到预期长度的PCR产物,但在没有配体的情况下未检测到信号。进行实时定量PCR以定量结合至配体:AhR复合物的DNA。我们获得了在TCDD浓度为0.01 pM-10 nM的范围内与TCDNA结合的标准曲线。该测定法的最小检出限低于0.01 pM TCDD,整个检出时间少于5 h。与化学激活的萤光素酶基因表达(CALUX)生物测定法相比,EPM-PCR生物测定法更加灵敏且易于执行。这些结果表明,该测定法可用于无细胞系统中不使用放射性检测和定量TCDD和相关的AhR配体。

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