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Homogeneous Electrochemiluminescence Biosensor for the Detection of RNase A Activity and Its Inhibitor

机译:均匀电化学发光生物传感器,用于检测RNase A活性及其抑制剂

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摘要

Ribonuclease A (RNase A) is increasingly considered as a biomarker for tumor diagnosis, and it is of great significance to develop an ultrasensitive, cost-effective assay for RNase A detection. Electrochemiluminescence (ECL) technology has distinctive advantages in the development of biosensors for diverse targets. However, most of the ECL biosensors require the complex process of electrode modification, which is laborious and time consuming. In this work, an immobilization-free homogeneous ECL assay was developed for the highly sensitive detection of RNase A activity for the first time. On the basis of the fact that RNase A can specifically hydrolyze RNA at the site of ribonucleotide uracil (rU), a rU-containing chimeric DNA probe is designed and labeled with Ru(bpy)(3)(2+) (act as ECL indicator). The chimeric DNA probe hardly diffuses to the surface of negatively charged indium tin oxide (ITO) electrode due to the strong electrostatic repulsion between the negatively charged DNA and ITO electrode, resulting in a weak ECL signal detected. When the RNase A is present, the chimeric DNA probe is hydrolyzed into small fragments, which contains little negative charge and can diffuse easily to the ITO electrode surface due to the decreased electrostatic repulsion. In this case, an enhanced ECL signal can be detected. Under the optimal conditions, there is a linear relationship between the ECL signal and the concentration of RNase A in the range of 0.001-0.10 ng/mL, and the detection limit is 0.2 pg/mL. In addition, the proposed ECL sensing system is also applied to detect the RNase A inhibitor, taking As3+ as an example. The proposed homogeneous ECL sensing system provides a new approach for the highly sensitive and convenient detection of RNase A as well as other ribonucleases only by redesigning a responding chimeric DNA probe.
机译:核糖核酸酶A(RNaseA)越来越多地被认为是用于肿瘤诊断的生物标志物,并且对于RNase A检测产生超细化,经济高效的测定具有重要意义。电化学发光(ECL)技术在为不同目标的生物传感器开发方面具有独特的优势。然而,大多数ECL生物传感器需要复杂的电极改性过程,这是费力和耗时的。在这项工作中,首次开发了无致密的均质ECL测定,用于首次对RNase A活性的高敏感性检测。在rnase a可以在核糖核苷酸尿嘧啶(Ru)位点的特异性水解RNA的基础上,设计并用Ru(bpy)(3)(2+)设计并标记了含Ru的嵌合DNA探针(作为ECL指标)。由于带负电荷的DNA和ITO电极之间的强烈的静电排斥,嵌合DNA探针几乎不扩散到带负电铟锡(ITO)电极的表面,导致检测到弱ECL信号。当存在RNase A时,将嵌合DNA探针水解成小片段,其含有少量的负电荷,并且由于静电排斥减小而容易扩散到ITO电极表面上。在这种情况下,可以检测到增强的ECL信号。在最佳条件下,ECL信号与RNase A的浓度之间存在线性关系,在0.001-0.10ng / ml的范围内,检测限为0.2pg / ml。此外,还应用了所提出的ECL传感系统以检测RNase抑制剂,以AS3 +为例。所提出的均匀ECL传感系统仅通过重新设计响应的嵌合DNA探针来提供高度敏感和方便地检测RNase A以及其他Ribonucl释放的新方法。

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  • 来源
    《Analytical chemistry》 |2019年第22期|共6页
  • 作者单位

    Minnan Normal Univ Fujian Prov Key Lab Modern Analyt Sci &

    Separat T Coll Chem Chem Engn &

    Environm Zhangzhou 363000 Peoples R China;

    Minnan Normal Univ Fujian Prov Key Lab Modern Analyt Sci &

    Separat T Coll Chem Chem Engn &

    Environm Zhangzhou 363000 Peoples R China;

    Minnan Normal Univ Fujian Prov Key Lab Modern Analyt Sci &

    Separat T Coll Chem Chem Engn &

    Environm Zhangzhou 363000 Peoples R China;

    Southern Med Univ Dermatol Hosp Mol Diag &

    Treatment Ctr Infect Dis Guangzhou 510631 Guangdong Peoples R China;

    Minnan Normal Univ Fujian Prov Key Lab Modern Analyt Sci &

    Separat T Coll Chem Chem Engn &

    Environm Zhangzhou 363000 Peoples R China;

    Fuzhou Univ MOE Key Lab Analyt Sci Food Safety &

    Biol Fujian Prov Key Lab Anal &

    Detect Technol Food Sa Coll Chem Fuzhou 350116 Fujian Peoples R China;

    Fuzhou Univ MOE Key Lab Analyt Sci Food Safety &

    Biol Fujian Prov Key Lab Anal &

    Detect Technol Food Sa Coll Chem Fuzhou 350116 Fujian Peoples R China;

    Fuzhou Univ MOE Key Lab Analyt Sci Food Safety &

    Biol Fujian Prov Key Lab Anal &

    Detect Technol Food Sa Coll Chem Fuzhou 350116 Fujian Peoples R China;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 分析化学;
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