Scalable multimodal mapping of macrophage regulatory architecture by integrating optical and transcriptomic pooled screens

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Abstract

Understanding how genetic perturbations reshape cellular states requires measuring diverse phenotypic modalities at scale. Here, we present PerturbPair, a platform that combines parallel Perturb-Seq and optical pooled screening (OPS) in primary mouse bone marrow-derived macrophages stimulated with lipopolysaccharide. Profiling over 334,000 single-cell transcriptomes across ∼1,000 gene perturbations and 7.8 million imaging-phenotyped cells across ∼3,000 gene perturbations, we reveal high concordance between transcriptomic and optical perturbation signatures. While RNA and imaging phenotypes were broadly concordant, OPS demonstrated superior sensitivity for weak-effect perturbations owing to greater cell throughput, and captured post-transcriptional regulatory events—such as protein trapping and mTOR-dependent phosphorylation—that left no detectable transcriptional footprint. To exploit cross-modal relationships, we developed EB-MoCAVI, an empirical Bayesian variational inference framework that both imputes RNA profiles for perturbations measured only by imaging—effectively tripling our Perturb-Seq dataset in silico —and denoises transcriptomic estimates for perturbations with sparse cell coverage by leveraging matched imaging data as a regularizer. A secondary screen validated the imputed transcriptional profiles and corroborated the cytosolic iron-sulfur assembly pathway as a candidate restraint on macrophage interferon tone. Integrating measured and imputed profiles with rare-variant burden statistics from the UK Biobank identified disease-specific macrophage gene programs and causal regulatory nodes for monocyte counts, type 2 diabetes, and inflammatory bowel disease. PerturbPair establishes a generalizable framework for multimodal perturbation atlases, pointing toward quantitative, causally-informed cross-modal models of cellular behavior.

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