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调控红/绿藻胆色素蛋白荧光发射的关键残基的计算鉴定

Computational identification of key residues regulating fluorescence emission in a red/green cyanobacteriochrome.

作者信息

Kannan Priyadharshini, Oh Jisung, Yeon Young Joo, Park Youn-Il, Seo Moon-Hyeong, Park Keunwan

机构信息

Natural Product Informatics Research Center, Korea Institute of Science and Technology, Gangneung, Republic of Korea.

Department of Biochemical Engineering, Gangneung-Wonju National University, Gangneung, Republic of Korea.

出版信息

Proteins. 2024 Jan;92(1):106-116. doi: 10.1002/prot.26586. Epub 2023 Aug 30.

DOI:10.1002/prot.26586
PMID:37646483
Abstract

Cyanobacteriochromes (CBCRs) are linear tetrapyrrole bilin-binding photoreceptors of cyanobacteria that exhibit high spectral diversity, gaining attention in optogenetics and bioimaging applications. Several engineering studies on CBCRs were attempted, especially for designing near-infrared (NIR) fluorescent proteins with longer fluorescence wavelengths. However, despite continuous efforts, a key component regulating fluorescence emission property in CBCRs is still poorly understood. As a model system, we focused on red/green CBCR Slr1393g3, from the unicellular cyanobacterium Synechocystis sp. PCC 6803 to engineer Pr to get far-red light-emitting property. Energy profiling and pairwise structural comparison of Slr1393g3 variants effectively reveal the mutations that are critical to the fluorescence changes. H497 seems to play a key role in stabilizing the chromophore environment, especially the α3 helix, while H495, T499, and Q502 are potential key residues determining fluorescence emission peak wavelength. We also found that mutations of α2 and α4 helical regions are closely related to the chromophore binding stability and likely affect fluorescence properties. Taken together, our computational analysis suggests that the fluorescence of Slr1393g3 is mainly controlled by the stabilization of the chromophore binding pocket. The predicted key residues potentially regulating the fluorescence emission property of a red/green CBCR will be advantageous for designing improved NIR fluorescent protein when combined with in vitro molecular evolution approaches.

摘要

蓝细菌视色素(CBCRs)是蓝细菌中的线性四吡咯胆色素结合光感受器,具有高度的光谱多样性,在光遗传学和生物成像应用中受到关注。人们尝试了多项关于CBCRs的工程研究,特别是设计具有更长荧光波长的近红外(NIR)荧光蛋白。然而,尽管不断努力,CBCRs中调节荧光发射特性的关键成分仍未得到很好的理解。作为一个模型系统,我们聚焦于单细胞蓝细菌集胞藻6803中的红/绿CBCR Slr1393g3,对其进行工程改造以获得远红光发射特性。对Slr1393g3变体进行能量分析和成对结构比较,有效地揭示了对荧光变化至关重要的突变。H497似乎在稳定发色团环境,特别是α3螺旋方面起关键作用,而H495、T499和Q502是决定荧光发射峰值波长的潜在关键残基。我们还发现α2和α4螺旋区域的突变与发色团结合稳定性密切相关,可能影响荧光特性。综上所述,我们的计算分析表明,Slr1393g3的荧光主要受发色团结合口袋稳定性的控制。预测的潜在调节红/绿CBCR荧光发射特性的关键残基,与体外分子进化方法相结合时,将有利于设计改进的近红外荧光蛋白。

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