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用于α-葡萄糖苷酶活性测定和抑制剂筛选的荧光非共轭聚合物点的原位形成

In situ formation of fluorescent non-conjugated polymer dots for α-glucosidase activity assay and inhibitor screening.

作者信息

Wang Feifei, Wang Xinling, Wang Yu, Zhang Yin, Liu Tianxiang, Sun Jian

机构信息

College of Pharmacy, Xinjiang Key Laboratory of Biopharmaceuticals and Medical Devices, Xinjiang Medical University, Urumqi, 830017, China.

出版信息

Mikrochim Acta. 2025 Aug 8;192(9):569. doi: 10.1007/s00604-025-07417-1.

Abstract

A novel and facile fluorescence turn-on assay for detecting α-glucosidase (α-Glu) activity and screening inhibitors is reported. This assay exploits α-Glu-catalyzed hydrolysis of L-ascorbic acid-2-O-α-D-glucopyranosyl (AA2G) to release ascorbic acid (AA), triggering an in situ fluorogenic reaction with N-methylethylenediamine (N-MEDA) that generates non-conjugated polymer dots (NCPDs). These NCPDs emit blue fluorescence at 425 nm upon excitation at 350 nm, and the fluorescence intensity increases proportionally with the concentration of α-Glu, enabling quantitative detection of enzymatic activity. The fluorescent assay demonstrates a linear response ranging from 0.01 to 10 U/mL and achieves a low detection limit of 0.0034 U/mL, surpassing most existing methods in sensitivity and width of linear range. In addition, the proposed method has been successfully applied to screen α-Glu inhibitors (AGIs) and determine α-Glu activity in real samples, yielding satisfying results. This work introduces a robust analytical framework and promising approach for clinical diagnosis and anti-diabetic drug discovery.

摘要

报道了一种用于检测α-葡萄糖苷酶(α-Glu)活性和筛选抑制剂的新型简便的荧光开启检测方法。该检测方法利用α-Glu催化L-抗坏血酸-2-O-α-D-吡喃葡萄糖苷(AA2G)水解以释放抗坏血酸(AA),引发与N-甲基乙二胺(N-MEDA)的原位荧光反应,生成非共轭聚合物点(NCPD)。这些NCPD在350 nm激发下于425 nm处发射蓝色荧光,并且荧光强度与α-Glu的浓度成比例增加,从而能够定量检测酶活性。该荧光检测方法的线性响应范围为0.01至10 U/mL,检测限低至0.0034 U/mL,在灵敏度和线性范围宽度方面超过了大多数现有方法。此外,所提出的方法已成功应用于筛选α-Glu抑制剂(AGI)并测定实际样品中的α-Glu活性,产生了令人满意的结果。这项工作为临床诊断和抗糖尿病药物发现引入了一个强大的分析框架和有前景的方法。

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