Pooled Genome-Scale CRISPR Screens in Single Cells

Author:

Schraivogel Daniel1,Steinmetz Lars M.123,Parts Leopold4

Affiliation:

1. Genome Biology Unit, European Molecular Biology Laboratory (EMBL), Heidelberg, Germany;

2. Department of Genetics, Stanford University School of Medicine, Stanford, California, USA;

3. Stanford Genome Technology Center, Stanford University School of Medicine, Palo Alto, California, USA

4. Wellcome Sanger Institute, Hinxton, United Kingdom;

Abstract

Assigning functions to genes and learning how to control their expression are part of the foundation of cell biology and therapeutic development. An efficient and unbiased method to accomplish this is genetic screening, which historically required laborious clone generation and phenotyping and is still limited by scale today. The rapid technological progress on modulating gene function with CRISPR-Cas and measuring it in individual cells has now relaxed the major experimental constraints and enabled pooled screening with complex readouts from single cells. Here, we review the principles and practical considerations for pooled single-cell CRISPR screening. We discuss perturbation strategies, experimental model systems, matching the perturbation to the individual cells, reading out cell phenotypes, and data analysis. Our focus is on single-cell RNA sequencing and cell sorting–based readouts, including image-enabled cell sorting. We expect this transformative approach to fuel biomedical research for the next several decades.

Publisher

Annual Reviews

Subject

Genetics

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