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Ratiometric fluorescence and colorimetry dual-mode assay based on manganese dioxide nanosheets for visual detection of alkaline phosphatase activity

机译:基于二氧化锰纳米片的比例荧光和比色法双模式测定法用于碱性磷酸酶活性的可视检测

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摘要

Alkaline phosphatase (ALP) activity plays a crucial role in foods and varies greatly in livestock and dairy products; it is quite difficult to compatibly monitor the different activities in various complicated foods. Herein, we proposed a ratiometric fluorescence and colorimetry dual-mode assay based on manganese dioxide (MnO2) nanosheets for the visualization of ALP activity in livestock serum and pasteurized milk samples compatibly. MnO2 nanosheets could oxidize dopamine into green fluorescent polydopamine (PDA) nanoparticles, so to quench the red fluorescent quantum dots (QDs), or oxidize colorless 3,3',5,5'-tetramethylbenzidine (TMB) into yellow TMBox. In the coexistence of ALP and 2-phospho-L-ascorbic acid, MnO2 nanosheets were reduced into Mn2+ ions by the catalysate of ascorbic acid, failing to generate PDA nanoparticles, and therefore, recovering the fluorescence of QDs for ratiometric fluorescence detection of high-activity ALP, or weakening the oxidization of TMB for colorimetric detection of ultralow-activity ALP. The ratiometric fluorescence-colorimetry combination extended the linear range over three orders of magnitude (0.04-80 mU/mL), and lowered the detection limit down to 0.015 mU/mL, along with profuse ALP-dependent (fluorescence) color changes for visual detection of ALP activity. Excellent recognition selectivity for ALP was attained over possibly coexistent reducing substances. Furthermore, the endogenous ALP were detected ranging from 17.32 to 269.54 mU/mL in seven typical livestock sera, consistent with that measured by commercial ALP assay kit; the detection results for ALP in four pasteurized milks matched well with that by test paper. The developed dual-mode assay held great potential for rapid on-site visual determination of reductant-related analytes in complicated matrices.
机译:碱性磷酸酶(ALP)的活性在食品中起着至关重要的作用,在牲畜和奶制品中差异很大。很难兼容地监视各种复杂食品中的不同活动。在此,我们提出了一种基于二氧化锰(MnO2)纳米片的比例荧光和比色法双模式测定法,以可视化地观察家畜血清和巴氏灭菌牛奶样品中的ALP活性。 MnO2纳米片可以将多巴胺氧化为绿色荧光聚多巴胺(PDA)纳米颗粒,从而猝灭红色荧光量子点(QD),或将无色的3,3',5,5'-四甲基联苯胺(TMB)氧化为黄色TMBox。在ALP和2-磷酸-L-抗坏血酸共存的情况下,MnO2纳米片被抗坏血酸的催化还原为Mn2 +离子,无法生成PDA纳米颗粒,因此,回收了QDs的荧光,用于高比例荧光检测。活性ALP,或减弱TMB的氧化,用于比色检测超低活性ALP。比率荧光比色法组合将线性范围扩展了三个数量级(0.04-80 mU / mL),并将检出限降低至0.015 mU / mL,并进行了可视化检测的大量依赖于ALP的(荧光)颜色变化ALP活动。相对于可能共存的还原物质,ALP具有出色的识别选择性。此外,在七个典型的牲畜血清中检测到的内源性ALP范围为17.32至269.54 mU / mL,与通过商业ALP分析试剂盒测得的值一致;四种巴氏灭菌牛奶中ALP的检测结果与试纸相符。所开发的双模式测定法具有用于快速现场目测确定复杂基质中还原剂相关分析物的巨大潜力。

著录项

  • 来源
    《Sensors and Actuators》 |2020年第1期|127176.1-127176.10|共10页
  • 作者单位

    Nanchang Univ State Key Lab Food Sci & Technol Nanchang 330047 Jiangxi Peoples R China|Chinese Acad Sci Yantai Inst Coastal Zone Res Res Ctr Coastal Environm Engn & Technol CAS Key Lab Coastal Environm Proc & Ecol Remediat Yantai 264003 Peoples R China;

    Chinese Acad Sci Yantai Inst Coastal Zone Res Res Ctr Coastal Environm Engn & Technol CAS Key Lab Coastal Environm Proc & Ecol Remediat Yantai 264003 Peoples R China|Binshou Med Univ Sch Pharm Yantai 264003 Peoples R China;

    Nanchang Univ State Key Lab Food Sci & Technol Nanchang 330047 Jiangxi Peoples R China;

    Chinese Acad Sci Yantai Inst Coastal Zone Res Res Ctr Coastal Environm Engn & Technol CAS Key Lab Coastal Environm Proc & Ecol Remediat Yantai 264003 Peoples R China;

    Chung Ang Univ Dept Chem Seoul 06974 South Korea;

    Chinese Acad Sci Yantai Inst Coastal Zone Res Res Ctr Coastal Environm Engn & Technol CAS Key Lab Coastal Environm Proc & Ecol Remediat Yantai 264003 Peoples R China|Chinese Acad Sci Ctr Ocean Megasci Qingdao 266071 Shandong Peoples R China;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    Alkaline phosphatase; Visual detection; Ratiometric fluorescence; Colorimetry; Dual-mode assay;

    机译:碱性磷酸酶;视觉检测;比例荧光;比色法双模式测定;

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