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基于内含肽介导的蛋白质工程的细胞基生物传感器用于检测生物活性信号分子。

Cell-Based Biosensors Based on Intein-Mediated Protein Engineering for Detection of Biologically Active Signaling Molecules.

机构信息

Department of Biomedical Engineering (BK21 plus) , Dongguk University , Seoul 04620 , Korea.

出版信息

Anal Chem. 2018 Aug 21;90(16):9779-9786. doi: 10.1021/acs.analchem.8b01481. Epub 2018 Aug 3.

DOI:10.1021/acs.analchem.8b01481
PMID:30028129
Abstract

Live-cell-based biosensors have emerged as a useful tool for biotechnology and chemical biology. Genetically encoded sensor cells often use bimolecular fluorescence complementation or fluorescence resonance energy transfer to build a reporter unit that suffers from nonspecific signal activation at high concentrations. Here, we designed genetically encoded sensor cells that can report the presence of biologically active molecules via fluorescence-translocation based on split intein-mediated conditional protein trans-splicing (PTS) and conditional protein trans-cleavage (PTC) reactions. In this work, the target molecules or the external stimuli activated intein-mediated reactions, which resulted in activation of the fluorophore-conjugated signal peptide. This approach fully valued the bond-making and bond-breaking features of intein-mediated reactions in sensor construction and thus eliminated the interference of false-positive signals resulting from the mere binding of fragmented reporters. We could also avoid the necessity of designing split reporters to refold into active structures upon reconstitution. These live-cell-based sensors were able to detect biologically active signaling molecules, such as Ca and cortisol, as well as relevant biological stimuli, such as histamine-induced Ca stimuli and the glucocorticoid receptor agonist, dexamethasone. These live-cell-based sensing systems hold large potential for applications such as drug screening and toxicology studies, which require functional information about targets.

摘要

基于活细胞的生物传感器已成为生物技术和化学生物学的有用工具。遗传编码的传感器细胞通常使用双分子荧光互补或荧光共振能量转移来构建报告单元,但在高浓度下会受到非特异性信号激活的影响。在这里,我们设计了遗传编码的传感器细胞,它们可以通过基于分裂内含子介导的条件蛋白转剪接 (PTS) 和条件蛋白转裂解 (PTC) 反应的荧光易位来报告生物活性分子的存在。在这项工作中,目标分子或外部刺激激活内含子介导的反应,从而激活荧光标记的信号肽。这种方法充分利用了内含子介导反应在传感器构建中的成键和断键特性,从而消除了由于仅仅结合碎片化报告器而导致的假阳性信号的干扰。我们还可以避免设计分裂报告器以在重新组装时折叠成活性结构的必要性。这些基于活细胞的传感器能够检测生物活性信号分子,如 Ca 和皮质醇,以及相关的生物刺激物,如组胺诱导的 Ca 刺激物和糖皮质激素受体激动剂,地塞米松。这些基于活细胞的传感系统在药物筛选和毒理学研究等应用中具有很大的潜力,这些应用需要有关目标的功能信息。

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