Directed evolution of the genetically encoded zinc(II) FRET sensor ZapCY1

Zinc(II) ions (Zn2+) play an essential role in living systems, with their delicate concentration balance differing among the various intracellular organelles. The spatiotemporal distribution and homeostasis of Zn2+ can be monitored through photoluminescence imaging using zinc sensors. Among such bio...

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Published inBiochimica et biophysica acta. General subjects Vol. 1866; no. 10; p. 130201
Main Authors Wei, Tianbiao, Huang, Shanqing, Hu, Qingyuan, Wang, Jue, Huo, Zhongzhong, Liu, Chunhong, Lu, Shuyu, Chen, Hao
Format Journal Article
LanguageEnglish
Published Elsevier B.V 01.10.2022
Subjects
biocompatibility
biosensors
Directed evolution
energy transfer
fluorescence
FRET
Genetically encoded fluorescent sensor
homeostasis
mutants
organelles
photoluminescence
signal-to-noise ratio
zinc
Zinc sensor
FRET
Directed evolution
Genetically encoded fluorescent sensor
Zinc sensor
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Summary:Zinc(II) ions (Zn2+) play an essential role in living systems, with their delicate concentration balance differing among the various intracellular organelles. The spatiotemporal distribution and homeostasis of Zn2+ can be monitored through photoluminescence imaging using zinc sensors. Among such biosensors, genetically encoded fluorescent sensor proteins are attractive tools owing to their subcellular localization advantage and high biocompatibility. However, the limited fluorescent properties of these proteins, such as their insufficient quantum yield and dynamic range, restrict their practical use. In this study, we developed an expression–screening–directed evolution system and used it to improve ZapCY1, a genetically encoded fluorescence resonance energy transfer (FRET) sensor. After four rounds of directed evolution, the FRET dynamic range of the modified sensor (designated ZapTV-EH) was increased by 1.5–1.7-fold. With its enhanced signal-to-noise ratio and ability to detect a wide Zn2+ concentration range, ZapTV-EH proves to be a better visualization tool for monitoring Zn2+ at the subcellular level. Combined with the simplified subcloning and expression steps and sufficient mutant libraries, this directed evolution system may provide a more simple and efficient way to develop and optimize genetically encoded FRET sensors through high-throughput screening. •A self-induced expression and batch-screening system with simpler processes•Combines a mutation library and screening system to evolve the sensor properties•An improved genetically encoded zinc sensor with a broader FRET dynamic range
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ISSN:0304-4165
1872-8006
1872-8006
DOI:10.1016/j.bbagen.2022.130201