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首页> 外文期刊>The Analyst: The Analytical Journal of the Royal Society of Chemistry: A Monthly International Publication Dealing with All Branches of Analytical Chemistry >Cerium oxide-triggered 'one-to-many' catalytic cycling strategy for in situ amplified electronic signal of low-abundance protein
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Cerium oxide-triggered 'one-to-many' catalytic cycling strategy for in situ amplified electronic signal of low-abundance protein

机译:氧化铈触发的“一对多”催化循环策略用于低丰度蛋白的原位扩增电子信号

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摘要

Multifunctionalized thionine-modified cerium oxide (Thi-CeO_2) nanostructures with redox ability and catalytic activity were designed as the bionanolabels for in situ amplified electronic signal of low-abundance protein (carcinoembryonic antigen, CEA, used as a model) based on a cerium oxide-triggered 'one-to-many' catalytic cycling strategy. Initially, the carried CeO_2 nanoparticles autocatalytically hydrolyzed the phosphate ester bond of l-ascorbic acid 2-phosphate (AAP) to produce a new reactant (l-ascorbic acid, AA), then the generated AA was electrochemically oxidized by the assembled thionine on the Thi-CeO_2, and the resultant product was then reduced back to AA by the added tris(2-carboxyethy)phosphine (TCEP). The catalytic cycling could be re-triggered by the thionine and TCEP, resulting in amplification of the electrochemical signal. Under the optimized conditions, the electrochemical immunosensor exhibited a wide linear range of 0.1 pg mL ~(-1) to 80 ng mL~(-1) with a low detection limit of 0.08 pg mL~(-1) CEA at the 3σblank level. In addition, the methodology was evaluated for the analysis of clinical serum samples, and was in good accordance with values obtained using the commercialized enzyme-linked immunosorbent assay (ELISA) method.
机译:设计具有氧化还原能力和催化活性的多功能化的硫氨酸修饰的氧化铈(Thi-CeO_2)纳米结构,作为基于氧化铈原位扩增低丰度蛋白(癌胚抗原,CEA,作为模型)的电子信号的生物标记。触发的“一对多”催化循环策略。最初,携带的CeO_2纳米粒子自催化水解1-抗坏血酸2-磷酸酯(AAP)的磷酸酯键以产生新的反应物(1-抗坏血酸,AA),然后将生成的AA用组装的亚硫氨酸电化学氧化。 Thi-CeO_2,然后通过添加三(2-羧基乙基)膦(TCEP)将生成的产物还原为AA。硫氨酸和TCEP可以重新触发催化循环,从而放大电化学信号。在最佳条件下,电化学免疫传感器的线性范围为0.1 pg mL〜(-1)至80 ng mL〜(-1),在3σ空白水平下的检测限为0.08 pg mL〜(-1)CEA。 。此外,评估了该方法用于临床血清样品的分析,并与使用商业化酶联免疫吸附测定(ELISA)方法获得的值完全一致。

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