Detection of Hg2+ Using a Dual-Mode Biosensing Probe Constructed Using Ratiometric Fluorescent Copper Nanoclusters@Zirconia Metal-Organic Framework/N-Methyl Mesoporphyrin IX and Colorimetry G-Quadruplex/Hemin Peroxidase-Mimicking G-Quadruplex DNAzyme.

IF 5 Q1 ENGINEERING, BIOMEDICAL
BME frontiers Pub Date : 2024-12-17 eCollection Date: 2024-01-01 DOI:10.34133/bmef.0078
Shikha Jain, Monika Nehra, Neeraj Dilbaghi, Ganga Ram Chaudhary, Sandeep Kumar
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引用次数: 0

Abstract

Mercury (Hg2+) has been recognized as a global pollutant with a toxic, mobile, and persistent nature. It adversely affects the ecosystem and human health. Already developed biosensors for Hg2+ detection majorly suffer from poor sensitivity and specificity. Herein, a colorimetric/fluorimetric dual-mode sensing approach is designed for the quantitative detection of Hg2+. This novel sensing approach utilizes nanofluorophores, i.e., fluorescent copper nanoclusters-doped zirconia metal-organic framework (CuNCs@Zr-MOF) nanoconjugate (blue color) and N-methyl mesoporphyrin IX (NMM) (red color) in combination with peroxidase-mimicking G-quadruplex DNAzyme (PMDNAzyme). In the presence of Hg2+, dabcyl conjugated complementary DNA with T-T mismatches form the stable duplex with the CuNCs@Zr-MOF@G-quadruplex structure through T-Hg2+-T base pairing. It causes the quenching of fluorescence of CuNCs@Zr-MOF (463 nm) due to the Förster resonance energy transfer (FRET) system. Moreover, the G-quadruplex (G4) structure of the aptamer enhances the fluorescence emission of NMM (610 nm). Besides this, the peroxidase-like activity of G4/hemin DNAzyme offers the colorimetric detection of Hg2+. The formation of duplex with PMDNAzyme increases the catalytic activity. This novel biosensing probe quantitatively detected Hg2+ using both fluorimetry and colorimetry approaches with a low detection limit of 0.59 and 36.3 nM, respectively. It was also observed that the presence of interfering metal ions in case of real aqueous samples does not affect the performance of this novel biosensing probe. These findings confirm the considerable potential of the proposed biosensing probe to screen the concentration of Hg2+ in aquatic products.

利用比率荧光铜纳米簇@氧化锆金属有机框架/N-甲基中卟啉 IX 和比色法 G-四链/海明过氧化物酶模拟 G-四链 DNA 酶构建的双模式生物传感探针检测 Hg2+。
汞(Hg2+)是公认的具有毒性、流动性和持久性的全球性污染物。它对生态系统和人类健康产生不利影响。已经开发的用于Hg2+检测的生物传感器主要存在灵敏度和特异性较差的问题。本文设计了一种比色/荧光双模传感方法,用于Hg2+的定量检测。这种新型传感方法利用纳米荧光团,即荧光铜纳米团簇掺杂氧化锆金属有机框架(CuNCs@Zr-MOF)纳米偶联物(蓝色)和n -甲基间卟啉IX (NMM)(红色)与模拟过氧化物酶的g -四联DNAzyme (PMDNAzyme)结合。在Hg2+存在下,dabcyl偶联T-T错配的互补DNA通过T-Hg2+-T碱基配对形成稳定的CuNCs@Zr-MOF@ g -四联体结构。由于Förster共振能量转移(FRET)系统,导致CuNCs@Zr-MOF (463 nm)的荧光猝灭。此外,适体的g -四重体(G4)结构增强了NMM (610 nm)的荧光发射。此外,G4/hemin DNAzyme的过氧化物酶样活性提供了Hg2+的比色检测。与PMDNAzyme形成双相,提高了催化活性。该新型生物传感探针采用荧光法和比色法对Hg2+进行定量检测,检测限分别为0.59 nM和36.3 nM。还观察到,在实际水样品中存在干扰金属离子并不影响这种新型生物传感探针的性能。这些发现证实了所提出的生物传感探针在筛选水产品中Hg2+浓度方面的巨大潜力。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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CiteScore
7.10
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