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通过F145Y取代实现Green2向光稳定性和量子产率增强的结构导向进化。

Structure-guided evolution of Green2 toward photostability and quantum yield enhancement by F145Y substitution.

作者信息

Sun Tingting, Li Tianpeng, Yi Ke, Gao Xiaolian

机构信息

College of Food Science and Pharmaceutical Engineering, Zaozhuang University, Zaozhuang, Shandong, China.

College of City and Architecture Engineering, Zaozhuang University, Zaozhuang, Shandong, China.

出版信息

Protein Sci. 2020 Sep;29(9):1964-1974. doi: 10.1002/pro.3917.

Abstract

Quantum yield is a determinant for fluorescent protein (FP) applications and enhancing FP brightness through gene engineering is still a challenge. Green2, our de novo FP synthesized by microfluidic picoarray and cloning, has a significantly lower quantum yield than enhanced green FP, though they have high homology and share the same chromophore. To increase its quantum yield, we introduced an F145Y substitution into Green2 based on rational structural analysis. Y145 significantly increased the quantum yield (0.22 vs. 0.18) and improved the photostability (t , 73.0 s vs. 46.0 s), but did not affect the excitation and emission spectra. Further structural analysis showed that the F145Y substitution resulted in a significant electrical field change in the immediate environment of the chromophore. The perturbation of electrostatic charge around the chromophore lead to energy barrier changes between the ground and excited states, which resulted in the enhancement of quantum yield and photostability. Our results illustrate a typical example of engineering an FP based solely on fluorescence efficiency optimization and provide novel insights into the rational evolution of FPs.

摘要

量子产率是荧光蛋白(FP)应用的一个决定因素,通过基因工程提高FP的亮度仍然是一个挑战。我们通过微流控皮升阵列和克隆合成的新型FP Green2,尽管与增强型绿色FP具有高度同源性且共享相同的发色团,但其量子产率仍显著低于增强型绿色FP。为了提高其量子产率,我们基于合理的结构分析在Green2中引入了F145Y替换。Y145显著提高了量子产率(从0.18提高到0.22)并改善了光稳定性(半衰期从46.0秒提高到73.0秒),但不影响激发和发射光谱。进一步的结构分析表明,F145Y替换导致发色团紧邻环境中的电场发生显著变化。发色团周围静电荷的扰动导致基态和激发态之间的能垒变化,从而提高了量子产率和光稳定性。我们的结果展示了一个仅基于荧光效率优化来改造FP的典型例子,并为FP的合理进化提供了新的见解。

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