Rewiring Multidomain Protein Switches: Transforming a Fluorescent Zn2+ Sensor into a Light-Responsive Zn2+ Binding Protein

被引:9
|
作者
Aper, Stijn J. A.
Merkx, Maarten [1 ]
机构
[1] Eindhoven Univ Technol, Dept Biomed Engn, Biol Chem Lab, POB 513, NL-5600 MB Eindhoven, Netherlands
来源
ACS SYNTHETIC BIOLOGY | 2016年 / 5卷 / 07期
关键词
optogenetics; protein engineering; light switching; metal binding; fluorescent sensor; Vivid; ENERGY-TRANSFER; OPTICAL CONTROL; SPATIOTEMPORAL CONTROL; OPTOGENETIC CONTROL; FRET SENSORS; ZINC; DESIGN; ACTIVATION; INDUCTION; MECHANISM;
D O I
10.1021/acssynbio.6b00027
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Protein-based sensors and switches provide attractive tools for the real-time monitoring and control of molecular processes in complex biological environments. Fluorescent sensor proteins have been developed for a wide variety of small molecules, but the construction of genetically encoded light-responsive ligand binding proteins remains mostly unexplored. Here we present a generic approach to reengineer a previously developed FRET-based Zn2+ sensor into a light-activatable Zn2+ binding protein using a design strategy based on mutually exclusive domain interactions. These so-called VividZn proteins consist of two light-responsive Vivid domains that homodimerize upon illumination with blue light, thus preventing the binding of Zn2+ between two Zn2+ binding domains, Atoxl and WD4. Following optimization of the linker between WD4 and the N-terminus of one of the Vivid domains, VividZn variants were obtained that show a 9- to SS-fold decrease in Zn2+ affinity upon illumination, which is fully reversible following dark adaptation. The Zn2+ affinities of the switch could be rationally tuned between 1 pM and 2 nM by systematic variation of linker length and mutation of one of the Zn2+ binding residues. Similarly, introduction of mutations in the Vivid domains allowed tuning of the switching kinetics between 10 min and 7 h. Low expression levels in mammalian cells precluded the demonstration of light-induced perturbation of cytosolic Zn2+ levels. Nonetheless, our results firmly establish the use of intramolecular Vivid dimerization as an attractive light-sensitive input module to rationally engineer light-responsive protein switches based on mutually exclusive domain interactions.
引用
收藏
页码:698 / 709
页数:12
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