Multiplexed single-cell profiling of post-perturbation transcriptional responses to define cancer vulnerabilities and therapeutic mechanism of action

Author:

McFarland James M.ORCID,Paolella Brenton R.,Warren Allison,Geiger-Schuller Kathryn,Shibue Tsukasa,Rothberg Michael,Kuksenko Olena,Jones Andrew,Chambers Emily,Dionne Danielle,Bender Samantha,Wolpin Brian M.,Ghandi Mahmoud,Tirosh Itay,Rozenblatt-Rosen Orit,Roth Jennifer A.,Golub Todd R.,Regev Aviv,Aguirre Andrew J.ORCID,Vazquez FranciscaORCID,Tsherniak AviadORCID

Abstract

AbstractAssays to study cancer cell responses to pharmacologic or genetic perturbations are typically restricted to using simple phenotypic readouts such as proliferation rate or the expression of a marker gene. Information-rich assays, such as gene-expression profiling, are generally not amenable to efficient profiling of a given perturbation across multiple cellular contexts. Here, we developed MIX-Seq, a method for multiplexed transcriptional profiling of post-perturbation responses across a mixture of samples with single-cell resolution, using SNP-based computational demultiplexing of single-cell RNA-sequencing data. We show that MIX-Seq can be used to profile responses to chemical or genetic perturbations across pools of 100 or more cancer cell lines, and combine it with Cell Hashing to further multiplex additional experimental conditions, such as multiple post-treatment time points or drug doses. Analyzing the high-content readout of scRNA-seq reveals both shared and context-specific transcriptional response components that can identify drug mechanism of action and can be used to predict long-term cell viability from short-term transcriptional responses to treatment.

Publisher

Cold Spring Harbor Laboratory

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