DNA-controlled protein fluorescence: Design of aptamer-split peptide hetero-modulator for GFP to respond to intracellular ATP levels

Author:

Park Ki Sung12ORCID,Cha Hanvit23,Niu Jia4,Soh Hyongsok Tom56ORCID,Lee Jin Hyup23,Pack Seung Pil12ORCID

Affiliation:

1. Department of Biotechnology and Bioinformatics, Korea University , Sejong  30019 , Republic of Korea

2. Biological Clock-based Anti-Aging Convergence RLRC, Korea University , Sejong  30019 , Republic of Korea

3. Department of Food and Biotechnology, Korea University , Sejong  30019 , Republic of Korea

4. Department of Chemistry , Boston College, Chestnut Hill, MA  02467 , USA

5. Department of Electrical Engineering, Stanford University , Stanford , CA  94305 , USA

6. Department of Radiology, Stanford University , Stanford , CA  94305 , USA

Abstract

Abstract Enabling the precise control of protein functions with artificially programmed reaction patterns is beneficial for investigating biological processes. Although several strategies have been established that employ the programmability of nucleic acid, they have been limited to DNA hybridization without external stimuli or target binding. Here, we report an approach for the DNA-mediated control of the tripartite split-GFP assembly via aptamers with responsiveness to intracellular small molecules as stimuli. We designed a novel structure-switching aptamer-peptide conjugate as a hetero modulator for split GFP in response to ATP. By conjugating two peptides (S10/11) derived from the tripartite split-GFP to ATP aptamer, we achieved GFP reassembly using only ATP as a trigger molecule. The response to ATP at ≥4 mM concentrations indicated that it can be applied to respond to intracellular ATP in live cells. Furthermore, our hetero-modulator exhibited high and long-term stability, with a half-life of approximately four days in a serum stability assay, demonstrating resistance to nuclease degradation. We validated that our aptamer-modulator split GFP was successfully reconstituted in the cell in response to intracellular ATP levels. Our aptamer-modulated split GFP platform can be utilized to monitor a wide range of intracellular metabolites by replacing the aptamer sequence.

Funder

National Research Foundation of Korea

Korean government

Ministry of Education

Korea University

Publisher

Oxford University Press (OUP)

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