Destabilized reporters for background-subtracted, chemically-gated, and multiplexed deep-tissue imaging.
Jason YunYimeng HuangAustin D C MillerBrandon L ChangLogan BaldiniKaamini M DhanabalanEugene LiHonghao LiArnab MukherjeePublished in: Chemical science (2024)
Tracking gene expression in deep tissues requires genetic reporters that can be unambiguously detected using tissue penetrant techniques. Magnetic resonance imaging (MRI) is uniquely suited for this purpose; however, there is a dearth of reporters that can be reliably linked to gene expression with minimal interference from background tissue signals. Here, we present a conceptually new method for generating background-subtracted, drug-gated, multiplex images of gene expression using MRI. Specifically, we engineered chemically erasable reporters consisting of a water channel, aquaporin-1, fused to destabilizing domains, which are stabilized by binding to cell-permeable small-molecule ligands. We showed that this approach allows for highly specific detection of gene expression through differential imaging. In addition, by engineering destabilized aquaporin-1 variants with orthogonal ligand requirements, it is possible to distinguish distinct subpopulations of cells in mixed cultures. Finally, we demonstrated this approach in a mouse tumor model through differential imaging of gene expression with minimal background.
Keyphrases
- gene expression
- magnetic resonance imaging
- dna methylation
- high resolution
- small molecule
- contrast enhanced
- copy number
- stem cells
- high throughput
- deep learning
- magnetic resonance
- diffusion weighted imaging
- mass spectrometry
- fluorescence imaging
- cell death
- cell proliferation
- optical coherence tomography
- cell cycle arrest
- photodynamic therapy
- drug induced
- real time pcr
- quantum dots
- loop mediated isothermal amplification