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首页> 外文期刊>Journal of Materials Chemistry, B. materials for biology and medicine >Silver ion-stabilized DNA triplexes for completely enzyme-free and sensitive fluorescence detection of transcription factors via catalytic hairpin assembly amplification
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Silver ion-stabilized DNA triplexes for completely enzyme-free and sensitive fluorescence detection of transcription factors via catalytic hairpin assembly amplification

机译:银离子稳定的DNA通过催化发夹组装扩增进行完全酶无酶和敏感荧光检测转录因子

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摘要

Transcription factors play important roles in gene regulation and have been identified as promising biomarkers for disease diagnosis. On the basis of a new Ag+-stabilized DNA triplex probe and catalytic hairpin assembly (CHA) signal amplification, we have established a completely enzyme-free and sensitive method for simple fluorescence detection of NF-kappa B p50 (nuclear factor-kappa B), a transcription factor. We found that the employment of Ag+ to stabilize the DNA triplex structure could effectively reduce the background noise. The association of the target NF-kappa B p50 with the recognition hairpin in the Ag+-stabilized DNA triplex leads to the release of a single stranded DNA, which is used as the trigger to initiate subsequent CHA between a fluorescently quenched signal hairpin and the recognition hairpin in the triplex DNA structure, thereby resulting in drastically amplified fluorescence recovery for sensitive detection of NF-kappa B p50. This assay method shows a dynamic concentration range of 5 to 150 pM and a detection limit of 1.5 pM for the detection of NF-kappa B p50. Besides, the presence of the target molecules can also be selectively discriminated from other non-specific proteins. Moreover, the presence of low concentrations of NF-kappa B p50 in human serum samples could be monitored with this approach. With the successful demonstration for NF-kappa B p50, such a method can be potentially extended to detecting other transcription factors in a convenient and sensitive manner without using any enzymes for signal amplification.
机译:转录因子在基因调节中起重要作用,并已被确定为有前途的疾病诊断生物标志物。在新的Ag + -Stabilized DNA三重探针和催化发夹组件(CHA)信号放大的基础上,我们已经建立了一种完全无酶和敏感方法,用于NF-Kappa B P50的简单荧光检测(核因子-Kappa B) ,转录因子。我们发现AG +的就业稳定DNA三重结构可以有效地降低背景噪音。靶NF-Kappa B P50与Ag + -Stabilized DNA三链接中识别发夹的关联导致单链DNA的释放,其用作触发器,以在荧光淬火信号发夹和识别之间引发随后的CHA三醇DNA结构中的发夹,从而导致荧光恢复急剧放大,用于敏感检测NF-Kappa B P50。该测定方法显示5至150μm的动态浓度范围和用于检测NF-Kappa B P50的1.5μm的检测限。此外,还可以从其他非特异性蛋白选择性地区分靶分子的存在。此外,可以通过这种方法监测人血清样品中低浓度的NF-κBp50的存在。随着NF-Kappa B P50的成功演示,这种方法可以潜在地扩展到以方便和敏感的方式检测其他转录因子,而不使用任何酶进行信号放大。

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    Southwest Univ Sch Chem &

    Chem Engn Minist Educ Key Lab Luminescent &

    Real Time Analyt Chem Chongqing 400715 Peoples R China;

    Southwest Univ Sch Chem &

    Chem Engn Minist Educ Key Lab Luminescent &

    Real Time Analyt Chem Chongqing 400715 Peoples R China;

    Southwest Univ Sch Chem &

    Chem Engn Minist Educ Key Lab Luminescent &

    Real Time Analyt Chem Chongqing 400715 Peoples R China;

    Southwest Univ Sch Chem &

    Chem Engn Minist Educ Key Lab Luminescent &

    Real Time Analyt Chem Chongqing 400715 Peoples R China;

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  • 正文语种 eng
  • 中图分类 分析化学;
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