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Intramolecular substitution uncages fluorogenic probes for detection of metallo-carbapenemase-expressing bacteria

机译:分子内取代解笼荧光探针用于检测表达金属碳卡宾酶的细菌

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摘要

This work reports a novel caging strategy for designing fluorogenic probes to detect the activity of β-lactamases. The caging strategy uses a thiophenyl linker connected to a fluorophore caged by a good leaving group—dinitrophenyl. The uncaging proceeds in two steps through the sulfa-releasing and subsequent intramolecular substitution. The length of the linker has been examined and optimized to maximize the rate of intramolecular reaction and thus the rate of fluorescence activation. Finally based on this strategy, we prepared a green fluorogenic probe >CAT-7 and validated its selectivity for detecting metallo-carbapenemases (VIM-27, IMP-1, NDM-1) in carbapenem-resistant Enterobacteriaceae (CRE) lysates.
机译:这项工作报告了一种新颖的笼养策略,用于设计检测β-内酰胺酶活性的荧光探针。笼养策略使用与被良好离去基团-二硝基苯基笼罩的荧光团连接的硫代苯基接头。通过磺胺释放和随后的分子内取代,分两步进行解封。已检查并优化了连接子的长度,以使分子内反应的速率最大化,从而使荧光激活的速率最大化。最终,基于此策略,我们制备了绿色荧光探针> CAT-7 ,并验证了其在耐碳青霉烯肠杆菌科细菌( CRE)裂解液。

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