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基于有序多孔层干涉测量法的不溶性底物酶活性测定及其在溶栓药物评价中的应用。

Measurement of enzyme activity of insoluble substrates based on ordered porous layer interferometry and the application in evaluation of thrombolytic drugs.

机构信息

Pharmacy School, Jiangsu Ocean University, Lianyungang 222005, China.

Jiangsu Key Laboratory of Marine Drug Screening, Lianyungang 222005, China.

出版信息

Analyst. 2024 Feb 26;149(5):1537-1547. doi: 10.1039/d3an02054a.

DOI:10.1039/d3an02054a
PMID:38284466
Abstract

The development of innovative methods for real-time surveillance of enzymatic activity determination processes is essential, particularly for insoluble substrate enzymatic assessments. In this work, a novel method for enzymatic activity determination was devised by assembling a 190 nm silica colloidal crystal (SCC) film onto a glass slide, coupled with Ordered Porous Layer Interferometry (OPLI) technology. By fixing the substrate of the enzyme on the surface of the silica sphere, a solid-liquid interface can be formed for monitoring enzymatic activity. The enzymatic activity is gauged by the change in the SCC film's thickness caused by the digestion of the loaded substrate. The procedure of chymotrypsin-mediated casein digestion was documented in real time, facilitating the examination of chymotrypsin's activity and kinetics. The newly-developed enzymatic activity determination method demonstrated exceptional sensitivity towards chymotrypsin activity, with a linear range spanning 0.0505-2.02 units per mg. Additionally, the method was extended to the assessment of fibrinolysis enzyme activity and kinetic analysis, yielding promising results. Therefore, this technique can serve as a real-time, user-friendly, cost-effective novel approach for enzymatic activity determination, providing fresh perspectives for enzymatic activity determination studies.

摘要

开发用于实时监测酶活性测定过程的创新方法至关重要,特别是对于不溶性底物的酶评估。在这项工作中,通过将 190nm 二氧化硅胶体晶体 (SCC) 薄膜组装到载玻片上,并结合有序多孔层干涉测量 (OPLI) 技术,设计了一种用于酶活性测定的新方法。通过将酶的底物固定在二氧化硅球的表面上,可以形成固液界面以监测酶活性。通过负载的底物的消化引起的 SCC 膜厚度的变化来测量酶活性。实时记录了胰凝乳蛋白酶介导的酪蛋白消化过程,便于检查胰凝乳蛋白酶的活性和动力学。新开发的酶活性测定方法对胰凝乳蛋白酶活性具有出色的灵敏度,线性范围为 0.0505-2.02 单位/毫克。此外,该方法还扩展到纤溶酶活性的评估和动力学分析,取得了有前景的结果。因此,该技术可以作为一种实时、用户友好、具有成本效益的新型酶活性测定方法,为酶活性测定研究提供了新的视角。

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