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Tandem Dye Acceptor Used To Enhance Upconversion Fluorescence Resonance Energy Transfer in Homogeneous Assays

机译:串联染料受体用于均相测定中增强上转换荧光共振能量转移

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In fluorescence resonance energy transfer (FRET)-basedassays, spectral separation of acceptor emission from donor emission is a common problem affecting the assay sensitivity. The challenge derives from small Stokes shifts characteristic to conventional fluorescent dyes resulting in leakage of donor emission to the measurement window intended only to collect the acceptor emission. We have studied a FRET-based homogeneous bioaffinity assay utilizing a tandem dye acceptor with a large pseudo-Stokes shift (139 nm). The tandem dye was constructed using B-phycoerythrin as an absorber and multiple Alexa Fluor 680 dyes as emitters. As a donor, we employed upconverting phosphor particles, which uniquely emit at visible wavelengths under low-energy infrared excitation enabling the fluorescence measurements free from autofluorescence even without time-resolved detection. With the tandem dye, it was possible to achieve four times higher signal from a single binding event compared to the conventional Alexa Fluor 680 dye alone. Tandem dyes are widely used in cytometry and other multiplex purposes, but their applications can be expanded to fluorescence-based homogeneous assays. Both the optimal excitation and emission wavelengths of tandem dye can be tuned to a desired region by choosing appropriate fluorophores enabling specifically designed acceptor dyes with large Stokes shift.
机译:在基于荧光共振能量转移(FRET)的测定中,受体发射与供体发射的光谱分离是影响测定灵敏度的常见问题。挑战源于传统荧光染料的小斯托克斯位移特性,导致供体发射泄漏到仅用于收集受体发射的测量窗口中。我们已经研究了基于FRET的均质生物亲和力测定方法,该方法利用了具有大拟斯托克斯位移(139 nm)的串联染料受体。使用B-藻红蛋白作为吸收剂和多种Alexa Fluor 680染料作为发射体构建串联染料。作为供体,我们采用了上转换的荧光粉颗粒,该颗粒在低能红外激发下以可见波长唯一发射,即使没有时间分辨检测,也能实现无自发荧光的荧光测量。与传统的Alexa Fluor 680染料相比,使用串联染料的单次结合事件可获得的信号高四倍。串联染料广泛用于细胞计数和其他多重用途,但它们的应用可以扩展到基于荧光的均相测定。串联染料的最佳激发和发射波长都可以通过选择合适的荧光团调节到所需的区域,从而实现专门设计的具有大斯托克斯位移的受体染料。

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