Design and preparation of a fluorescent molecularly imprinted membrane for the selective detection of pepsin enzyme as a biomarker for gastroesophageal reflux disease

IF 4.1 Q1 CHEMISTRY, ANALYTICAL Talanta Open Pub Date : 2024-08-26 DOI:10.1016/j.talo.2024.100351
Aya M. Mostafa , Stephen J. Barton , Stephen P. Wren , James Barker
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Abstract

A novel fluorescent molecularly imprinted polymer membrane (FMIM) has been developed for the selective binding and qualitative detection of pepsin enzyme, a biomarker indicative of gastroesophageal reflux disease (GERD). This study utilises the high selectivity offered by molecular imprinting techniques to capture pepsin enzyme within complex biological matrices, such as human saliva. Additionally, fluorescent carbon dots integrated into the membrane matrix provide instant visual detection of pepsin. Various combinations of functional monomers and cross-linkers were systematically evaluated to investigate their impact on the binding capacity and mechanical stability of the resultant FMIMs. The optimum performance was achieved with a mixture of two hydrophilic monomers, namely N-(hydroxymethyl)acrylamide and acrylamide, in conjunction with N,N-methylenebis(acrylamide) as the cross-linking agent. The developed FMIM demonstrated a binding capacity of 21.56 mg g-1, surpassing that of the fluorescent non-imprinted membrane (FNIM) at 8.49 mg g-1. Moreover, the binding of FMIM to pepsin was tested against other competitor enzymes to verify its selectivity. Furthermore, comprehensive characterisation of both FMIM and FNIM was conducted using various analytical techniques to ensure their structural integrity and functionality. Ultimately, the developed FMIM exhibited effective binding of pepsin in standard solutions and samples, enabling enrichment and visual detection of the biomarker enzyme.

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设计和制备用于选择性检测胃蛋白酶的荧光分子印迹膜,作为胃食管反流病的生物标记物
我们开发了一种新型荧光分子印迹聚合物膜(FMIM),用于选择性结合和定性检测胃蛋白酶,胃蛋白酶是胃食管反流病(GERD)的一种生物标志物。这项研究利用分子印迹技术提供的高选择性,在复杂的生物基质(如人类唾液)中捕获胃蛋白酶。此外,集成到膜基质中的荧光碳点可提供胃蛋白酶的即时视觉检测。我们系统地评估了功能单体和交联剂的各种组合,以研究它们对最终 FMIMs 的结合能力和机械稳定性的影响。两种亲水性单体(即 N-(羟甲基)丙烯酰胺和丙烯酰胺)的混合物与 N,N-亚甲基双(丙烯酰胺)作为交联剂的组合达到了最佳性能。所开发的 FMIM 的结合能力为 21.56 mg g-1,超过了 8.49 mg g-1 的荧光非压印膜(FNIM)。此外,还测试了 FMIM 与胃蛋白酶和其他竞争酶的结合情况,以验证其选择性。此外,还使用各种分析技术对 FMIM 和 FNIM 进行了全面表征,以确保其结构完整性和功能性。最终,开发的 FMIM 在标准溶液和样品中显示出与胃蛋白酶的有效结合,实现了生物标记酶的富集和可视检测。
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来源期刊
Talanta Open
Talanta Open Chemistry-Analytical Chemistry
CiteScore
5.20
自引率
0.00%
发文量
86
审稿时长
49 days
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