Efficient combinatorial targeting of RNA transcripts in single cells with Cas13 RNA Perturb-seq.
Hans-Hermann WesselsAlejandro Méndez-MancillaYuhan HaoEfthymia PapalexiWilliam M MauckLu LuJohn A MorrisEleni P MimitouPeter SmibertNeville E SanjanaRahul SatijaPublished in: Nature methods (2022)
Pooled CRISPR screens coupled with single-cell RNA-sequencing have enabled systematic interrogation of gene function and regulatory networks. Here, we introduce Cas13 RNA Perturb-seq (CaRPool-seq), which leverages the RNA-targeting CRISPR-Cas13d system and enables efficient combinatorial perturbations alongside multimodal single-cell profiling. CaRPool-seq encodes multiple perturbations on a cleavable CRISPR array that is associated with a detectable barcode sequence, allowing for the simultaneous targeting of multiple genes. We compared CaRPool-seq to existing Cas9-based methods, highlighting its unique strength to efficiently profile combinatorially perturbed cells. Finally, we apply CaRPool-seq to perform multiplexed combinatorial perturbations of myeloid differentiation regulators in an acute myeloid leukemia (AML) model system and identify extensive interactions between different chromatin regulators that can enhance or suppress AML differentiation phenotypes.
Keyphrases
- single cell
- crispr cas
- genome editing
- genome wide
- rna seq
- acute myeloid leukemia
- high throughput
- induced apoptosis
- transcription factor
- dna methylation
- cell cycle arrest
- cancer therapy
- allogeneic hematopoietic stem cell transplantation
- copy number
- dendritic cells
- gene expression
- bone marrow
- pain management
- signaling pathway
- nucleic acid
- dna damage
- randomized controlled trial
- cell death
- clinical trial
- open label
- high density