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首页> 外文期刊>Angewandte Chemie >Specific and Direct Amplified Detection of MicroRNA with MicroRNA:Argonaute-2 Cleavage (miRACle) Beacons
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Specific and Direct Amplified Detection of MicroRNA with MicroRNA:Argonaute-2 Cleavage (miRACle) Beacons

机译:MicroRNA的具体和直接扩增检测MicroRNA:Argonaute-2裂解(奇迹)信标

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摘要

MicroRNA detection is a valuable method for determining cell identity. Molecular beacons are elegant sensors that can transform intracellular microRNA concentration into a fluorescence intensity. While target binding enhances beacon fluorescence, the degree of enhancement is insufficient for demanding applications. The addition of specialty nucleases can enable target recycling and signal amplification, but this process complicates the assay. We have developed and characterized a class of beacons that are susceptible to the endogenous nuclease Argonaute-2 (Ago2). After purification of the complex by co-immunoprecipitation, microRNA: Ago2 cleavage (miRACle) beacons undergo site- and sequence-specific cleavage, and show a 13-fold fluorescence enhancement over traditional beacons. The system can be adapted to any microRNA sequence, and can cleave nuclease-resistant, non-RNA bases, potentially allowing miRACle beacons to be designed for cells without interference from non-specific nucleases.
机译:MicroRNA检测是用于确定细胞标识的有价值的方法。分子信标是优雅的传感器,可以将细胞内microRNA浓度转化为荧光强度。虽然靶结合增强了信标荧光,但增强程度不足以要求苛刻的应用。添加特种核酸酶可以实现目标回收和信号放大,但该过程使测定复杂化。我们已经开发并表征了一类易受内源性核酸酶Argonaute-2(前2)的信标。通过共免疫沉淀纯化复合物,MicroRNA:前2个裂解(奇迹)信标经过现场和序列的裂解,并在传统信标上显示13倍的荧光增强。该系统可以适应任何MicroRNA序列,并且可以切割耐核性的非RNA碱基,可能允许奇迹信标设计用于细胞而不会干扰非特异性核酸酶。

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