| Literature DB >> 32142663 |
Till Ringel1, Nina Frey2, Femke Ringnalda2, Sharan Janjuha1, Sarah Cherkaoui3, Stefan Butz4, Sumana Srivatsa5, Martin Pirkl5, Giancarlo Russo6, Lukas Villiger2, Gerhard Rogler7, Hans Clevers8, Niko Beerenwinkel5, Nicola Zamboni3, Tuncay Baubec4, Gerald Schwank9.
Abstract
Forward genetic screens with genome-wide CRISPR libraries are powerful tools for resolving cellular circuits and signaling pathways. Applying this technology to organoids, however, has been hampered by technical limitations. Here we report improved accuracy and robustness for pooled-library CRISPR screens by capturing sgRNA integrations in single organoids, substantially reducing required cell numbers for genome-scale screening. We applied our approach to wild-type and APC mutant human intestinal organoids to identify genes involved in resistance to TGF-β-mediated growth restriction, a key process during colorectal cancer progression, and validated hits including multiple subunits of the tumor-suppressive SWI/SNF chromatin remodeling complex. Mutations within these genes require concurrent inactivation of APC to promote TGF-β resistance and attenuate TGF-β target gene transcription. Our approach can be applied to a variety of assays and organoid types to facilitate biological discovery in primary 3D tissue models.Entities:
Keywords: APC; ATAC; CRISPR screen; Cut and Run; SWI/SNF; TGFb; colorectal cancer; organoids
Mesh:
Substances:
Year: 2020 PMID: 32142663 DOI: 10.1016/j.stem.2020.02.007
Source DB: PubMed Journal: Cell Stem Cell ISSN: 1875-9777 Impact factor: 24.633