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用于检测半胱胺的用户友好型且超稳定的全包金片。

User-friendly and ultra-stable all-inclusive gold tablets for cysteamine detection.

作者信息

Al-Kassawneh Muna, Sadiq Zubi, Jahanshahi-Anbuhi Sana

机构信息

Department of Chemical and Materials Engineering, Gina Cody School of Engineering, Concordia University Montréal Québec Canada

出版信息

RSC Adv. 2023 Jun 29;13(28):19638-19650. doi: 10.1039/d3ra03073c. eCollection 2023 Jun 22.

Abstract

To date, a range of nanozymes has been reported for their enzyme-mimicking catalytic activity such as solution-based sensors. However, in remote areas, the need for portable, cost-effective, and one-pot prepared sensors is obvious. In this study, we report the development of a highly stable and sensitive gold tablet-based sensor for cysteamine quantification in human serum samples. The sensor is produced in two steps: synthesis of a pullulan-stabilized gold nanoparticle solution (pAuNP-Solution) using a pullulan polymer as a reducing, stabilizing, and encapsulating agent and then, casting the pAuNP-Solution into a pullulan gold nanoparticle tablet (pAuNP-Tablet) by a pipetting method. The tablet was characterized by UV-vis, DLS, FTIR, TEM, and AFM analyses. The pAuNP-tablet exhibited a high peroxidase-mimetic activity a TMB-HO system. The presence of cysteamine in the system introduced two types of inhibition which were dependent on the cysteamine concentration. By determining Michaelis-Menten's kinetic parameters, we gained mechanistic insights into the catalytic inhibition process. Based on the catalytic inhibition capability of cysteamine, the limit of detection (LoD) was calculated to be 69.04 and 82.9 μM in buffer and human serum samples, respectively. Finally, real human serum samples were tested, demonstrating the applicability of the pAuNP-Tablet for real-world applications. The % R values in human serum samples were in the range of 91-105% with % RSD less than 2% for all replicas. The stability tests over 16 months revealed the ultra-stable properties of the pAuNP-Tablet. Overall, with a simple fabrication method and a novel employed technique, this study contributes to the advancement of tablet-based sensors and helps in cysteamine detection in clinical settings.

摘要

迄今为止,已经报道了一系列具有模拟酶催化活性的纳米酶,例如基于溶液的传感器。然而,在偏远地区,对便携式、经济高效且能一锅制备的传感器的需求显而易见。在本研究中,我们报告了一种用于定量检测人血清样品中半胱胺的高稳定性和高灵敏度的金片基传感器的研制。该传感器分两步制备:使用支链淀粉聚合物作为还原剂、稳定剂和包封剂合成支链淀粉稳定的金纳米颗粒溶液(pAuNP溶液),然后通过移液法将pAuNP溶液浇铸成支链淀粉金纳米颗粒片(pAuNP片)。通过紫外可见光谱、动态光散射、傅里叶变换红外光谱、透射电子显微镜和原子力显微镜分析对该片剂进行了表征。pAuNP片在TMB-H₂O₂体系中表现出高过氧化物酶模拟活性。体系中半胱胺的存在引入了两种类型的抑制作用,这两种抑制作用取决于半胱胺的浓度。通过测定米氏动力学参数,我们对催化抑制过程有了机理上的认识。基于半胱胺的催化抑制能力,计算出缓冲液和人血清样品中的检测限(LoD)分别为69.04 μM和82.9 μM。最后,对实际人血清样品进行了测试,证明了pAuNP片在实际应用中的适用性。人血清样品中的%R值在91-105%范围内,所有复制品的%RSD均小于2%。超过16个月的稳定性测试揭示了pAuNP片的超稳定性能。总体而言,通过简单的制备方法和新颖的技术应用,本研究推动了片基传感器的发展,并有助于临床环境中半胱胺的检测。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0804/10308203/3799bdd48950/d3ra03073c-f6.jpg

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