Mapping information-rich genotype-phenotype landscapes with genome-scale Perturb-seq

Replogle, Joseph M.; Saunders, Reuben A.; Pogson, Angela N; Hussmann, Jeffrey A.; LeNail, Alexander; Guna, Alina; Mascibroda, Lauren G.; Wagner, Eric J.; Adelman, Karen; Lithwick‐Yanai, Gila; Iremadze, Nika; Oberstrass, Florian C.; Lipson, Doron; Bonnar, Jessica L.; Jost, Marco; Norman, Thomas M.; Weissman, Jonathan S.

doi:10.1016/j.cell.2022.05.013

Cited by 245 publications

(358 citation statements)

References 81 publications

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“…In the realm of CRISPRi effectors, our work points to a clear consensus: Zim3-dCas9 is the effector of choice, as it appears equal or superior to other effectors in every test we performed and had no downsides. We had previously measured by Perturb-seq that Zim3-dCas9 afforded median mRNA knockdown of 91.6% across 2,285 genes in RPE1 cells (Replogle et al, 2022), and here we further found that Zim3-dCas9 mediates robust knockdown across a range of cell types. Our work highlights the importance of using multiple assays to assess effector function including single-cell assays to assess cell-to-cell heterogeneity, of directly measuring knockdown instead of relying on proxies such as growth phenotypes that conflate multiple factors, and of evaluating effectors in stably transduced cells rather than in transiently transfected cells to evaluate longer-term consequences for cell viability.…”

Section: Discussionsupporting

confidence: 75%

“…Like other CRISPR approaches, CRISPRi has been paired with large-scale sgRNA libraries to conduct systematic genetic screens. Such screens have been deployed to identify essential protein-coding and non-coding genes (Gilbert et al, 2014; Haswell et al, 2021; Horlbeck et al, 2016a; Liu et al, 2017; Raffeiner et al, 2020), to map the targets of regulatory elements (Fulco et al, 2019, 2016; Gasperini et al, 2019; Kearns et al, 2015; Klann et al, 2017; Thakore et al, 2015), to identify regulators of cellular signaling and metabolism (Coukos et al, 2021; Liang et al, 2020; Luteijn et al, 2019; Semesta et al, 2020), to uncover stress response pathways in stem cell-derived neurons (Tian et al, 2021, 2019), to uncover regulators of disease-associated states in microglia and astrocytes (Dräger et al, 2022; Leng et al, 2022), to decode regulators of cytokine production in primary human T-cells (Schmidt et al, 2022), to define mechanisms of action of bioactive small molecules (Jost et al, 2017; Morgens et al, 2019; Sage et al, 2017), to identify synthetic-lethal genetic interactions in cancer cells (Du et al, 2017; Horlbeck et al, 2018), and to identify genetic determinants of complex transcriptional responses using RNA-seq readouts (Perturb-seq) (Adamson et al, 2016; Replogle et al, 2022, 2020; Tian et al, 2021, 2019), among others.…”

Section: Introductionmentioning

confidence: 99%

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Maximizing CRISPRi efficacy and accessibility with dual-sgRNA libraries and optimal effectors

Replogle¹,

Bonnar²,

Pogson³

et al. 2022

Preprint

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CRISPR interference (CRISPRi) enables programmable, reversible, and titratable repression of gene expression (knockdown) in mammalian cells. Initial CRISPRi-mediated genetic screens have showcased the potential to address basic questions in cell biology, genetics, and biotechnology, but wider deployment of CRISPRi screening has been constrained by the large size of single guide RNA (sgRNA) libraries and challenges in generating cell models with consistent CRISPRi-mediated knockdown. Here, we present next-generation CRISPRi sgRNA libraries and effector expression constructs that enable strong and consistent knockdown across mammalian cell models. First, we combine empirical sgRNA selection with a dual-sgRNA library design to generate an ultra-compact (1-3 elements per gene), highly active CRISPRi sgRNA library. Next, we rigorously compare CRISPRi effectors to show that the recently published Zim3-dCas9 provides the best balance between strong on-target knockdown and minimal nonspecific effects on cell growth or the transcriptome. Finally, we engineer a suite of cell lines with stable expression of Zim3-dCas9 and robust on-target knockdown. Our results and publicly available reagents establish best practices for CRISPRi genetic screening.

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Section: Discussionsupporting

confidence: 75%

Section: Introductionmentioning

confidence: 99%

Maximizing CRISPRi efficacy and accessibility with dual-sgRNA libraries and optimal effectors

Replogle¹,

Bonnar²,

Pogson³

et al. 2022

Preprint

Self Cite

View full text Add to dashboard Cite

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“…A multivariate distance measure between sets of cells resulting from different perturbations is needed to perform effective statistics comparing perturbations. With such a distance measure, one can describe the difference or similarity between sets of cells treated with distinct perturbations to infer difference or similarity in terms of mechanism or perturbation target; shared mechanisms tend to produce similar shifts in molecular profiles (Replogle et al, 2022;Tian et al, 2021). A number of distance measures for scRNA-seq have been explored by the single-cell community in recent years, including Wasserstein distances (Chen et al, 2020), maximum mean discrepancy (Kimmel et al, 2021), neighborhood-based measures (Burkhardt et al, 2021;Dann et al, 2022), E-distance (Replogle et al, 2022), and distances in learnt autoencoder latent spaces (Lotfollahi et al, 2019).…”

Section: Motivation For a Distance Measure For High-dimensional Expre...mentioning

confidence: 99%

scPerturb: Harmonized Single-Cell Perturbation Data

Peidli

Green

Shen

et al. 2022

Preprint

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Recent biotechnological advances led to growing numbers of single-cell studies, which reveal molecular and phenotypic responses to large numbers of perturbations. However, analysis across diverse datasets is typically hampered by differences in format, naming conventions, data filtering and normalization. In order to facilitate development and benchmarking of computational methods in systems biology, we collect a set of 44 publicly available single-cell perturbation-response datasets with molecular readouts, including transcriptomics, proteomics and epigenomics. We apply uniform pre-processing and quality control pipelines and harmonize feature annotations. The resulting information resource enables efficient development and testing of computational analysis methods, and facilitates direct comparison and integration across datasets. Using these datasets, we demonstrate the application of E-distance for quantifying perturbation similarity and strength. This work provides an information resource and guide for researchers working with single-cell perturbation data and highlights conceptual considerations for new experiments. The data collection, scPerturb, is publicly available at scperturb.org.

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“…These single-cell CRISPR screen technologies can provide rich phenotypes for massive numbers of perturbations. A recent effort has expanded Perturb-seq to the genome-wide level for the first time [ 84 ]. Besides CRISPR-based gene perturbations, scRNA-seq can also be combined with the pooled ORF overexpression to enable screening for cell reprogramming [ 85 , 86 ] or coding variants of oncogenes [ 87 ].…”

Section: Emerging Single-cell Technologies and Future Perspectivesmentioning

confidence: 99%

Transcriptional Regulation of the Hippo Pathway: Current Understanding and Insights from Single-Cell Technologies

Paul¹,

Xie²,

Yao³

et al. 2022

Cells

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The Hippo pathway regulates tissue homeostasis in normal development and drives oncogenic processes. In this review, we extensively discuss how YAP/TAZ/TEAD cooperate with other master transcription factors and epigenetic cofactors to orchestrate a broad spectrum of transcriptional responses. Even though these responses are often context- and lineage-specific, we do not have a good understanding of how such precise and specific transcriptional control is achieved—whether they are driven by differences in TEAD paralogs, or recruitment of cofactors to tissue-specific enhancers. We believe that emerging single-cell technologies would enable a granular understanding of how the Hippo pathway influences cell fate and drives oncogenic processes, ultimately allowing us to design better pharmacological agents against TEADs and identify robust pharmacodynamics markers of Hippo pathway inhibition.

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Mapping information-rich genotype-phenotype landscapes with genome-scale Perturb-seq

Cited by 245 publications

References 81 publications

Maximizing CRISPRi efficacy and accessibility with dual-sgRNA libraries and optimal effectors

Maximizing CRISPRi efficacy and accessibility with dual-sgRNA libraries and optimal effectors

scPerturb: Harmonized Single-Cell Perturbation Data

Transcriptional Regulation of the Hippo Pathway: Current Understanding and Insights from Single-Cell Technologies

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