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Relationships among ergot alkaloids cytochrome P450 activity and beef steer growth

机译:麦角生物碱细胞色素P450活性和牛ste生长之间的关系

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摘要

Determining a grazing animal's susceptibility to ergot alkaloids has been a research topic for decades. Our objective was to determine if the Promega™ P450-Glo assay could be used to indirectly detect ergot alkaloids or their metabolites in urine of steers. The first experiment validated the effects of ergot alkaloids [0, 20, and 40 μM of ergotamine (ET), dihydroergotamine (DHET), and ergonovine (EN)] on human CYP3A4 using the P450-Glo assay (Promega™ V9800). With this assay, luminescence is directly proportional to CYP450 activity. Relative inhibition of in vitro cytochrome P450 activity was affected (P < 0.001) by an interaction between alkaloids and concentration. That interaction resulted in no concentration effect of EN, but within ET and DHET 20 and 40 μM concentrations inhibited CYP450 activity when compared with controls. In experiment 2, urine was collected from Angus-sired crossbred steers (n = 39; 216 ± 2.6 days of age; 203 ± 1.7 kg) after grazing tall fescue pastures for 105 days. Non-diluted urine was added to the Promega™ P450-Glo assay, and observed inhibition (3.7 % ± 2.7 of control). Urine content of total ergot alkaloids (331.1 ng/mg of creatinine ± 325.7) was determined using enzyme linked immunosorbent assay. Urine inhibition of CYP450 activity and total alkaloids were correlated (r = −0.31; P < 0.05). Steers were genotyped at CYP450 single nucleotide polymorphism, C994G. Steer genotype affected (P < 0.03) inhibition of CYP450 activity by urine; heterozygous steers had the least amount of CYP450 inhibition suggesting that genotyping cattle may be a method of identifying animals that are susceptible to ergot alkaloids. Although, additional research is needed, we demonstrate that the Promega™ P450-Glo assay is sensitive to ergot alkaloids and urine from steers grazing tall fescue. With some refinement the P450-Glo assay has potential as a tool for screening cattle for their exposure to fescue toxins.
机译:数十年来,确定放牧动物对麦角生物碱的敏感性一直是研究的主题。我们的目标是确定Promega™P450-Glo检测法是否可用于间接检测ste牛尿中的麦角生物碱或其代谢产物。第一个实验使用P450-Glo分析(Promega™V9800)验证了麦角生物碱[0、20和40μM麦角胺(ET),二氢麦角胺(DHET)和麦角新碱(EN)]对人CYP3A4的作用。通过该测定,发光与CYP450活性成正比。生物碱和浓度之间的相互作用会影响体外抑制细胞色素P450的活性(P <0.001)。这种相互作用不会引起EN的浓度升高,但是在ET和DHET范围内,与对照组相比,浓度为20和40μM的CYP450酶活性受到抑制。在实验2中,放牧高羊茅草牧场105天后,从安格斯杂交杂种公牛(n = 39; 216±2.6天龄; 203±1.7 kg)中收集尿液。将未稀释的尿液添加到Promega™P450-Glo分析中,并观察到抑制作用(对照组的3.7%±2.7)。使用酶联免疫吸附法测定麦角总生物碱的尿液含量(331.1 ng / mg肌酐±325.7)。尿中CYP450活性的抑制与总生物碱的相关性(r = -0.31; P <0.05)。对牛进行CYP450单核苷酸多态性C994G的基因分型。转向基因型影响尿液对CYP450活性的抑制(P <0.03);杂合性ste牛对CYP450的抑制作用最小,这表明对牛进行基因分型可能是鉴定对麦角生物碱敏感的动物的一种方法。尽管还需要进一步的研究,但我们证明Promega™P450-Glo分析法对麦草生物碱和放牧高羊茅的ste牛尿敏感。经过一些改进,P450-Glo分析法有潜力作为筛选牛是否暴露于羊茅毒素的工具。

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