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Circularly Permuted Fluorescent Protein-Based Indicators: History Principles and Classification

机译:基于循环排列的荧光蛋白的指标:历史原理和分类

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摘要

Genetically encoded biosensors based on fluorescent proteins (FPs) are a reliable tool for studying the various biological processes in living systems. The circular permutation of single FPs led to the development of an extensive class of biosensors that allow the monitoring of many intracellular events. In circularly permuted FPs (cpFPs), the original N- and C-termini are fused using a peptide linker, while new termini are formed near the chromophore. Such a structure imparts greater mobility to the FP than that of the native variant, allowing greater lability of the spectral characteristics. One of the common principles of creating genetically encoded biosensors is based on the integration of a cpFP into a flexible region of a sensory domain or between two interacting domains, which are selected according to certain characteristics. Conformational rearrangements of the sensory domain associated with ligand interaction or changes in the cellular parameter are transferred to the cpFP, changing the chromophore environment. In this review, we highlight the basic principles of such sensors, the history of their creation, and a complete classification of the available biosensors.
机译:基于荧光蛋白(FP)的基因编码生物传感器是研究生命系统中各种生物过程的可靠工具。单个FP的循环排列导致了广泛的生物传感器的发展,该传感器可以监视许多细胞内事件。在圆形排列的FP(cpFP)中,使用肽接头将原始的N和C末端融合,而在发色团附近形成新的末端。与天然变体相比,这种结构使FP具有更大的迁移率,从而使光谱特性更加不稳定。创建遗传编码的生物传感器的常见原理之一是基于将cpFP整合到感觉域的柔性区域中或两个相互作用域之间的,该区域根据某些特征进行选择。与配体相互作用或细胞参数变化相关的感觉域的构象重排被转移至cpFP,从而改变了生色团环境。在本文中,我们重点介绍了此类传感器的基本原理,其创建历史以及可用生物传感器的完整分类。

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