Fluorogenic CRISPR for genomic DNA imaging.
Zhongxuan ZhangXiaoxiao RongTianjin XieZehao LiHaozhi SongShujun ZhenHaifeng WangJiahui WuSamie R JaffreyXing LiPublished in: Nature communications (2024)
Genomic DNA exhibits high heterogeneity in terms of its dynamic within the nucleus, its structure and functional roles. CRISPR-based imaging approaches can image genomic loci in living cells. However, conventional CRISPR-based tools involve expressing constitutively fluorescent proteins, resulting in high background and nonspecific nucleolar signal. Here, we construct fluorogenic CRISPR (fCRISPR) to overcome these issues. fCRISPR is designed with dCas9, an engineered sgRNA, and a fluorogenic protein. Fluorogenic proteins are degraded unless they are bound to specific RNA hairpins. These hairpins are inserted into sgRNA, resulting in dCas9: sgRNA: fluorogenic protein ternary complexes that enable fluorogenic DNA imaging. With fCRISPR, we image various genomic DNA in different human cells with high signal-to-noise ratio and sensitivity. Furthermore, fCRISPR tracks chromosomes dynamics and length. fCRISPR also allows DNA double-strand breaks (DSBs) and repair to be tracked in real time. Taken together, fCRISPR offers a high-contrast and sensitive platform for imaging genomic loci.
Keyphrases
- genome wide
- circulating tumor
- single molecule
- living cells
- high resolution
- copy number
- cell free
- crispr cas
- genome editing
- nucleic acid
- dna methylation
- fluorescent probe
- gene expression
- magnetic resonance imaging
- magnetic resonance
- machine learning
- air pollution
- high throughput
- small molecule
- amino acid
- quantum dots
- protein protein
- mass spectrometry
- gold nanoparticles
- contrast enhanced