Isolation of gene-edited cells via knock-in of short glycophosphatidylinositol-anchored epitope tags.
Anastasia ZotovaAlexey V PichuginAnastasia AtemasovaEkaterina KnyazhanskayaElena LopatukhinaNikita A MitkinEkhson HolmuhamedovMarina GottikhDmitry KuprashAlexander FilatovDmitriy MazurovPublished in: Scientific reports (2019)
We describe Surface Oligopeptide knock-in for Rapid Target Selection (SORTS), a novel method to select mammalian cells with precise genome modifications that does not rely on cell cloning. SORTS is designed to disrupt the target gene with an expression cassette encoding an epitope tag embedded into human glycophosphatidylinositol (GPI)-anchored protein CD52. The cassette is very short, usually less than 250 nucleotides, which simplifies donor DNA construction and facilitates transgene integration into the target locus. The chimeric protein is then expressed from the target promoter, processed and exposed on the plasma membrane where it serves as a marker for FACS sorting with tag-specific antibodies. Simultaneous use of two different epitope tags enables rapid isolation of cells with biallelic knock-ins. SORTS can be easily and reliably applied to a number of genome-editing problems such as knocking out genes encoding intracellular or secreted proteins, protein tagging and inactivation of HIV-1 provirus.
Keyphrases
- crispr cas
- genome editing
- induced apoptosis
- genome wide
- cell cycle arrest
- binding protein
- protein protein
- genome wide identification
- cell therapy
- dna methylation
- copy number
- endothelial cells
- mental health
- amino acid
- poor prognosis
- endoplasmic reticulum stress
- single cell
- gene expression
- transcription factor
- monoclonal antibody
- oxidative stress
- antiretroviral therapy
- hepatitis c virus
- hiv infected
- mesenchymal stem cells
- intellectual disability
- bone marrow
- cell proliferation
- loop mediated isothermal amplification
- south africa
- cell free
- genome wide analysis
- sensitive detection