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5,5-二烃基荧光素是用于基于生物发光的检测系统的热稳定底物。

5,5-Dialkylluciferins are thermal stable substrates for bioluminescence-based detection systems.

机构信息

Promega Biosciences, Inc., San Luis Obispo, California, United States of America.

Promega Corporation, Madison, Wisconsin, United States of America.

出版信息

PLoS One. 2020 Dec 14;15(12):e0243747. doi: 10.1371/journal.pone.0243747. eCollection 2020.

Abstract

Firefly luciferase-based ATP detection assays are frequently used as a sensitive, cost-efficient method for monitoring hygiene in many industrial settings. Solutions of detection reagent, containing a mixture of a substrate and luciferase enzyme that produces photons in the presence of ATP, are relatively unstable and maintain only a limited shelf life even under refrigerated conditions. It is therefore common for the individual performing a hygiene test to manually prepare fresh reagent at the time of monitoring. To simplify sample processing, a liquid detection reagent with improved thermal stability is needed. The engineered firefly luciferase, Ultra-Glo™, fulfills one aspect of this need and has been valuable for hygiene monitoring because of its high resistance to chemical and thermal inactivation. However, solutions containing both Ultra-Glo™ luciferase and its substrate luciferin gradually lose the ability to effectively detect ATP over time. We demonstrate here that dehydroluciferin, a prevalent oxidative breakdown product of luciferin, is a potent inhibitor of Ultra-Glo™ luciferase and that its formation in the detection reagent is responsible for the decreased ability to detect ATP. We subsequently found that dialkylation at the 5-position of luciferin (e.g., 5,5-dimethylluciferin) prevents degradation to dehydroluciferin and improves substrate thermostability in solution. However, since 5,5-dialkylluciferins are poorly utilized by Ultra-Glo™ luciferase as substrates, we used structural optimization of the luciferin dialkyl modification and protein engineering of Ultra-Glo™ to develop a luciferase/luciferin pair that shows improved total reagent stability in solution at ambient temperature. The results of our studies outline a novel luciferase/luciferin system that could serve as foundations for the next generation of bioluminescence ATP detection assays with desirable reagent stability.

摘要

萤火虫荧光素酶 ATP 检测法常被用于许多工业环境中,作为一种监测卫生情况的灵敏、经济有效的方法。检测试剂溶液包含一种底物和荧光素酶的混合物,在存在 ATP 的情况下会产生光子。然而,即使在冷藏条件下,检测试剂溶液也相对不稳定,保质期有限。因此,进行卫生测试的人员通常需要在监测时手动制备新鲜的试剂。为了简化样品处理过程,需要一种具有改进热稳定性的液体检测试剂。经过工程改造的萤火虫荧光素酶 Ultra-Glo™ 满足了这一需求的一个方面,由于其对化学和热失活的高抗性,它在卫生监测方面非常有价值。然而,含有 Ultra-Glo™ 荧光素酶及其底物荧光素的溶液会随着时间的推移逐渐丧失有效检测 ATP 的能力。我们在这里证明,脱荧光素是荧光素的一种常见氧化分解产物,是 Ultra-Glo™ 荧光素酶的一种有效抑制剂,它在检测试剂中的形成是导致检测 ATP 能力下降的原因。随后我们发现,荧光素在 5 位的二烷基化(例如 5,5-二甲基荧光素)可以防止其降解为脱荧光素,并提高溶液中底物的热稳定性。然而,由于 Ultra-Glo™ 荧光素酶对 5,5-二烷基荧光素的利用效率较低,因此我们使用荧光素二烷基修饰的结构优化和 Ultra-Glo™ 的蛋白工程,开发了一种在室温下具有更好的溶液总试剂稳定性的荧光素酶/荧光素对。我们的研究结果概述了一种新的荧光素酶/荧光素系统,可为具有理想试剂稳定性的下一代生物发光 ATP 检测法奠定基础。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c41d/7735563/e3347723e418/pone.0243747.g001.jpg

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