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首页> 外文期刊>Journal of biomolecular screening: The official journal of the Society for Biomolecular Screening >An efficient method for quantitative determination of cellular ATP synthetic activity
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An efficient method for quantitative determination of cellular ATP synthetic activity

机译:一种定量测定细胞ATP合成活性的有效方法

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摘要

The authors have developed an efficient method to measure cellular activity of ATP synthesis. Although ATP is a major energy source of biological reactions, it has been difficult to measure cellular ATP synthetic activity quantitatively. In this report, bioluminescence from the luciferin-luciferase reaction was used for the quantitative measurement. Under the used condition, bioluminescence from standard ATP solution showed no attenuation within several minutes, and the intensity corresponded proportionally to ATP concentrations of the standards. To measure dynamic cellular ATP synthetic activity, combination of osmotic shock and detergent treatment was used to make Escherichia coli cells permeable. ATP was discharged from permeable cells and reacted with externally added luciferase. Because permeable cells used glucose to synthesize and accumulate ATP without further growth, intensity of bioluminescence was increasing during the cellular consumption of glucose. Cellular ATP biosynthetic activity was calculated form the slope of linearly increasing bioluminescence. This permeable cell assay Could be applied to high-throughput measuring for dynamic cellular activity of glycolytic ATP synthesis.
机译:作者已经开发出一种有效的方法来测量ATP合成的细胞活性。尽管ATP是生物反应的主要能源,但很难定量测量细胞ATP的合成活性。在此报告中,荧光素-荧光素酶反应产生的生物发光用于定量测量。在使用条件下,标准ATP溶液的生物发光在几分钟内没有衰减,并且强度与标准ATP浓度成正比。为了测量动态细胞ATP合成活性,渗透压休克和去污剂处理的组合用于使大肠杆菌细胞具有渗透性。 ATP从可渗透细胞中释放出来,并与外部添加的荧光素酶反应。因为渗透性细胞使用葡萄糖来合成和积累ATP而没有进一步的增长,所以在细胞消耗葡萄糖的过程中,生物发光的强度正在增加。从线性增加的生物发光的斜率计算出细胞ATP的生物合成活性。此渗透性细胞测定法可用于高通量测量糖酵解ATP合成的动态细胞活性。

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