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Upconversion Fluorescence Resonance Energy Transfer in a Homogeneous Immunoassay for Estradiol

机译:雌二醇的均相免疫测定中的上转换荧光共振能量转移

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We recently described a novel homogeneous assay principle based on upconversion fluorescence resonance energy transfer (UC-FRET), where an upconverting phosphor (UCP) is utilized as a donor. The UC-FRET has now been applied to a competitive homogeneous immunoassay for 17beta-estradiol (E2) in serum, using a small-molecular dye as an acceptor. The assay was constructed by employing an UCP coated with an E2-specific recombinant antibody Fab fragment as a donor and an E2-conjugated small-molecular dye, Oyster-556, as an acceptor. Standard curves for the assay were produced both in buffer and in male serum. Sensitized acceptor emission was measured at 600 nm under continuous laser diode excitation at 980 nm. In buffer, the IC_(50) value of the assay was 1 nM and in serum 3 nM. The lower limits of detection (mean of zero calibrators, 3 SD) were 0.4 and 0.9 nM, respectively. The measurable concentration range extended up to 3 nM in buffer and 9 nM in serum. Equilibrium in the assay was reached in 30 min. The novel principle of UC-FRET has unique advantages compared to present homogeneous luminescence-based methods and can enable an attractive assay system platform for clinical diagnostics and for high-throughput screening approaches.
机译:我们最近描述了一种基于上转换荧光共振能量转移(UC-FRET)的新颖的均相测定原理,其中上转换荧光粉(UCP)被用作供体。 UC-FRET现在已被用于以小分子染料为受体的竞争性同质免疫分析法,用于血清中的17β-雌二醇(E2)。通过使用涂覆有E2特异性重组抗体Fab片段的UCP作为供体,并使用E2偶联的小分子染料Oyster-556作为受体来构建测定。在缓冲液和雄性血清中均产生测定的标准曲线。在980 nm的连续激光二极管激发下,在600 nm处测量了敏化的受体发射。在缓冲液中,测定的IC_(50)值为1 nM,在血清中为3 nM。检测的下限(零校准物的平均值,3 SD)分别为0.4和0.9 nM。可测量的浓度范围在缓冲液中扩展至3 nM,在血清中扩展至9 nM。在30分钟内达到测定平衡。与目前基于均相发光的方法相比,UC-FRET的新颖原理具有独特的优势,并且可以为临床诊断和高通量筛选方法提供有吸引力的分析系统平台。

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