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结构起源与绿色荧光蛋白高亮非经典变体的理性发展。

Structural origin and rational development of bright red noncanonical variants of green fluorescent protein.

机构信息

Department of Chemistry, Oregon State University, 153 Gilbert Hall, Corvallis, Oregon 97331, USA.

Department of Chemistry, University of Virginia, Charlottesville, Virginia 22904, USA.

出版信息

Phys Chem Chem Phys. 2023 Jun 15;25(23):15624-15634. doi: 10.1039/d3cp01315d.

Abstract

The incorporation of noncanonical amino acids (ncAAs) into fluorescent proteins is promising for red-shifting their fluorescence and benefiting tissue imaging with deep penetration and low phototoxicity. However, ncAA-based red fluorescent proteins (RFPs) have been rare. The 3-aminotyrosine modified superfolder green fluorescent protein (aY-sfGFP) represents a recent advance, yet the molecular mechanism for its red-shifted fluorescence remains elusive while its dim fluorescence hinders applications. Herein, we implement femtosecond stimulated Raman spectroscopy to obtain structural fingerprints in the electronic ground state and reveal that aY-sfGFP possesses a GFP-like instead of RFP-like chromophore. Red color of aY-sfGFP intrinsically arises from a unique "double-donor" chromophore structure that raises ground-state energy and enhances charge transfer, notably differing from the conventional conjugation mechanism. We further developed two aY-sfGFP mutants (E222H and T203H) with significantly improved (∼12-fold higher) brightness by rationally restraining the chromophore's nonradiative decay through electronic and steric effects, aided by solvatochromic and fluorogenic studies of the model chromophore in solution. This study thus provides functional mechanisms and generalizable insights into ncAA-RFPs with an efficient route for engineering redder and brighter fluorescent proteins.

摘要

将非天然氨基酸 (ncAA) 掺入荧光蛋白中有望实现其荧光红移,从而有益于具有深穿透和低光毒性的组织成像。然而,基于 ncAA 的红色荧光蛋白 (RFPs) 却很少见。经过 3-氨基酪氨酸修饰的超折叠绿色荧光蛋白 (aY-sfGFP) 代表了最近的一项进展,但它的红色荧光的分子机制仍然难以捉摸,而其暗淡的荧光则阻碍了其应用。在此,我们采用飞秒受激拉曼光谱技术获得了电子基态的结构指纹图谱,结果表明 aY-sfGFP 具有 GFP 样而不是 RFP 样的生色团。aY-sfGFP 的红色本质上源于独特的“双供体”生色团结构,该结构提高了基态能量并增强了电荷转移,这与传统的共轭机制显著不同。我们进一步通过合理的电子和空间位阻效应,开发了两种 aY-sfGFP 突变体 (E222H 和 T203H),其亮度显著提高 (∼12 倍),这得益于模型生色团在溶液中的溶剂化变色和荧光研究。该研究因此为 ncAA-RFPs 提供了功能机制和可推广的见解,并为工程更红和更亮的荧光蛋白提供了一条有效途径。

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