Joint single-cell measurements of nuclear proteins and RNA in vivo.

TitleJoint single-cell measurements of nuclear proteins and RNA in vivo.
Publication TypeJournal Article
Year of Publication2021
AuthorsChung H, Parkhurst CN, Magee EM, Phillips D, Habibi E, Chen F, Yeung BZ, Waldman J, Artis D, Regev A
JournalNat Methods
Volume18
Issue10
Pagination1204-1212
Date Published2021 10
ISSN1548-7105
KeywordsAnimals, Antibodies, Brain, Computational Biology, Gene Expression Regulation, Genome-Wide Association Study, Kainic Acid, Mice, Nuclear Proteins, Reproducibility of Results, RNA, Seizures, Single-Cell Analysis, Transcription Factor RelA
Abstract

Identifying gene-regulatory targets of nuclear proteins in tissues is a challenge. Here we describe intranuclear cellular indexing of transcriptomes and epitopes (inCITE-seq), a scalable method that measures multiplexed intranuclear protein levels and the transcriptome in parallel across thousands of nuclei, enabling joint analysis of transcription factor (TF) levels and gene expression in vivo. We apply inCITE-seq to characterize cell state-related changes upon pharmacological induction of neuronal activity in the mouse brain. Modeling gene expression as a linear combination of quantitative protein levels revealed genome-wide associations of each TF and recovered known gene targets. TF-associated genes were coexpressed as distinct modules that each reflected positive or negative TF levels, showing that our approach can disentangle relative putative contributions of TFs to gene expression and add interpretability to inferred gene networks. inCITE-seq can illuminate how combinations of nuclear proteins shape gene expression in native tissue contexts, with direct applications to solid or frozen tissues and clinical specimens.

DOI10.1038/s41592-021-01278-1
Alternate JournalNat Methods
PubMed ID34608310
PubMed Central IDPMC8532076
Grant List / HHMI_ / Howard Hughes Medical Institute / United States
RM1 HG006193 / HG / NHGRI NIH HHS / United States

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