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首页> 外文期刊>Brazilian Journal of Medical and Biological Research >Protection of plasmid DNA by a Ginkgo biloba extract from the effects of stannous chloride and the action on the labeling of blood elements with technetium-99m
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Protection of plasmid DNA by a Ginkgo biloba extract from the effects of stannous chloride and the action on the labeling of blood elements with technetium-99m

机译:银杏提取物对氯化亚锡作用和and元素对血元素标记作用的作用保护银杏叶提取物对质粒DNA的保护

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Ginkgo biloba extract (EGb) is a phytotherapeutic agent used for the treatment of ischemic and neurological disorders. Because the action of this important extract is not fully known, assays using different biological systems need to be performed. Red blood cells (RBC) are labeled with technetium-99m (Tc-99m) and used in nuclear medicine. The labeling depends on a reducing agent, usually stannous chloride (SnCl2). We assessed the effect of different concentrations of EGb on the labeling of blood constituents with Tc-99m, as sodium pertechnetate (3.7 MBq), and on the mobility of a plasmid DNA treated with SnCl2 (1.2 μg/ml) at room temperature. Blood was incubated with EGb before the addition of SnCl2 and Tc-99m. Plasma (P) and RBC were separated and precipitated with trichloroacetic acid, and soluble (SF-P and SF-RBC) and insoluble (IF-P and IF-RBC) fractions were isolated. The plasmid was incubated with Egb, SnCl2 or EGb plus SnCl2 and agarose gel electrophoresis was performed. The gel was stained with ethidium bromide and the DNA bands were visualized by fluorescence in an ultraviolet transilluminator system. EGb decreased the labeling of RBC, IF-P and IF-RBC. The supercoiled form of the plasmid was modified by treatment with SnCl2 and protected by 40 mg/ml EGb. The effect of EGb on the tested systems may be due to its chelating action with the stannous ions and/or pertechnetate or to the capability to generate reactive oxygen species that could oxidize the stannous ion.
机译:银杏叶提取物(EGb)是一种用于治疗缺血性和神经性疾病的植物治疗剂。由于这种重要提取物的作用尚不完全清楚,因此需要使用不同的生物系统进行测定。红血球(RBC)用tech 99m(Tc-99m)标记,并用于核医学。标记取决于还原剂,通常是氯化亚锡(SnCl2)。我们评估了不同浓度的EGb对Tc-99m血液成分标记的高tech酸钠(3.7 MBq),以及室温下经SnCl2(1.2μg/ ml)处理的质粒DNA迁移率的影响。在添加SnCl2和Tc-99m之前,将血液与EGb孵育。分离血浆(P)和RBC,并用三氯乙酸沉淀,分离出可溶性(SF-P和SF-RBC)和不溶性(IF-P和IF-RBC)馏分。将质粒与Egb,SnCl2或EGb加SnCl2一起孵育,并进行琼脂糖凝胶电泳。凝胶用溴化乙锭染色,并在紫外透照仪系统中通过荧光使DNA条带可视化。 EGb减少了RBC,IF-P和IF-RBC的标记。通过用SnCl2处理修饰质粒的超螺旋形式,并用40mg / ml EGb保护。 EGb对被测系统的影响可能是由于其与亚锡离子和/或高tech酸盐的螯合作用,或者是由于生成了可以氧化亚锡离子的活性氧的能力。

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