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Genetically Modified Semisynthetic Bioluminescent Photoprotein Variants: Simultaneous Dual-Analyte Assay in a Single Well Employing Time Resolution of Decay Kinetics

机译:基因修饰的半合成生物发光光蛋白变体:在单井中同时进行衰变动力学的时间分辨的双重分析物测定。

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Progress in the miniaturization and automation of complex analytical processes depends largely on increasing the sensitivity, diversity, and robustness of current labels. Because of their ubiquity and ease of use, fluorescent, enzymatic, and bioluminescent labels are often employed in such miniaturized and multiplexed formats, with each type of label having its own unique advantages and drawbacks. The ultrasensitive detection limits of bioluminescent reporters are especially advantageous when dealing with very small sample volumes and biological fluids. However, bioluminescent reporters currently do not have the multiplexing capability that fluorescent labels do. In an effort to address this limitation, we have developed a method of discriminating two semisynthetic aequorin variants from one another using time resolution. In this work we paired two aequorin conjugates with different coelenterazine analogues and then resolved the two signals from one another using the difference in decay kinetics and half-life times. Utilizing this time-resolution, we then developed a simultaneous, dual-analyte, single well assay for 6-keto-prostaglandin-FI-alpha and angiotensin II, two important cardiovascular molecules.
机译:复杂分析过程的小型化和自动化的进展很大程度上取决于提高当前标签的灵敏度,多样性和耐用性。由于它们的普遍性和易用性,荧光,酶促和生物发光标签经常以这种小型化和多路复用的形式使用,每种类型的标签都有其独特的优点和缺点。当处理非常少量的样品和生物液体时,生物发光报告分子的超灵敏检测极限特别有利。但是,生物发光报道分子目前不具有荧光标记所具有的多路复用能力。为了解决这一局限性,我们开发了一种使用时间分辨率将两个半合成水母发光蛋白变体区分开的方法。在这项工作中,我们将两种水母发光蛋白缀合物与不同的腔肠素类似物配对,然后利用衰变动力学和半衰期的差异相互解析了这两种信号。利用这种时间分辨率,我们随后开发了一种同时进行的双重分析物单孔测定法,用于测定两个重要的心血管分子6-酮-前列腺素-FI-α和血管紧张素II。

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