The CRISPR-Cas13a Gemini System for noncontiguous target RNA activation.
Hongrui ZhaoYan ShengTenghua ZhangShujun ZhouYuqing ZhuFeiyang QianMeiru LiuWeixue XuDengsong ZhangJiaming HuPublished in: Nature communications (2024)
Simultaneous multi-target detection and multi-site gene editing are two key factors restricting the development of disease diagnostic and treatment technologies. Despite numerous explorations on the source, classification, functional features, crystal structure, applications and engineering of CRISPR-Cas13a, all reports use the contiguous target RNA activation paradigm that only enables single-target detection in vitro and one-site gene editing in vivo. Here we propose a noncontiguous target RNA activation paradigm of Cas13a and establish a CRISPR-Cas13a Gemini System composed of two Cas13a:crRNA binary complexes, which can provide rapid, simultaneous, highly specific and sensitive detection of two RNAs in a single readout, as well as parallel dual transgene knockdown. CRISPR-Cas13a Gemini System are demonstrated in the detection of two miRNAs (miR-155 and miR-375) for breast cancer diagnosis and two small RNAs (EBER-1 and EBER-2) for Epstein-Barr virus diagnosis using multiple diagnostic platforms, including fluorescence and colorimetric-based lateral flow systems. We also show that CRISPR-Cas13a Gemini System can knockdown two foreign genes (EGFP and mCherry transcripts) in mammalian cells simultaneously. These findings suggest the potential of highly effective and simultaneous detection of multiple biomarkers and gene editing of multiple sites.
Keyphrases
- crispr cas
- genome editing
- loop mediated isothermal amplification
- sensitive detection
- epstein barr virus
- cell proliferation
- label free
- crystal structure
- real time pcr
- long non coding rna
- quantum dots
- long noncoding rna
- gene expression
- diffuse large b cell lymphoma
- dna methylation
- single molecule
- nucleic acid
- transcription factor
- risk assessment
- fluorescent probe
- bioinformatics analysis