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Rapid interrogation of cancer cell of origin through CRISPR editing.


ABSTRACT: The increasing complexity of different cell types revealed by single-cell analysis of tissues presents challenges in efficiently elucidating their functions. Here we show, using prostate as a model tissue, that primary organoids and freshly isolated epithelial cells can be CRISPR edited ex vivo using Cas9-sgRNA (guide RNA) ribotnucleoprotein complex technology, then orthotopically transferred in vivo into immunocompetent or immunodeficient mice to generate cancer models with phenotypes resembling those seen in traditional genetically engineered mouse models. Large intrachromosomal (∼2 Mb) or multigenic deletions can be engineered efficiently without the need for selection, including in isolated subpopulations to address cell-of-origin questions.

SUBMITTER: Feng W 

PROVIDER: S-EPMC8364185 | biostudies-literature | 2021 Aug

REPOSITORIES: biostudies-literature

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Rapid interrogation of cancer cell of origin through CRISPR editing.

Feng Weiran W   Cao Zhen Z   Lim Pei Xin PX   Zhao Huiyong H   Luo Hanzhi H   Mao Ninghui N   Lee Young Sun YS   Rivera Aura Agudelo AA   Choi Danielle D   Wu Chao C   Han Teng T   Romero Rodrigo R   de Stanchina Elisa E   Carver Brett S BS   Wang Qiao Q   Jasin Maria M   Sawyers Charles L CL  

Proceedings of the National Academy of Sciences of the United States of America 20210801 32


The increasing complexity of different cell types revealed by single-cell analysis of tissues presents challenges in efficiently elucidating their functions. Here we show, using prostate as a model tissue, that primary organoids and freshly isolated epithelial cells can be CRISPR edited ex vivo using Cas9-sgRNA (guide RNA) ribotnucleoprotein complex technology, then orthotopically transferred in vivo into immunocompetent or immunodeficient mice to generate cancer models with phenotypes resemblin  ...[more]

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