Combinatorial single-cell profiling of major chromatin types with MAbID

Publication date

2024-01

Authors

Lochs, Silke J.A.
van der Weide, Robin HORCID 0000-0002-6466-7280
de Luca, Kim L.
Korthout, Tessy
van Beek, Ramada E.
Kimura, Hiroshi
Kind, Jop

Editors

Advisors

Supervisors

Document Type

Article

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License

cc_by

Abstract

Gene expression programs result from the collective activity of numerous regulatory factors. Studying their cooperative mode of action is imperative to understand gene regulation, but simultaneously measuring these factors within one sample has been challenging. Here we introduce Multiplexing Antibodies by barcode Identification (MAbID), a method for combinatorial genomic profiling of histone modifications and chromatin-binding proteins. MAbID employs antibody–DNA conjugates to integrate barcodes at the genomic location of the epitope, enabling combined incubation of multiple antibodies to reveal the distributions of many epigenetic markers simultaneously. We used MAbID to profile major chromatin types and multiplexed measurements without loss of individual data quality. Moreover, we obtained joint measurements of six epitopes in single cells of mouse bone marrow and during mouse in vitro differentiation, capturing associated changes in multifactorial chromatin states. Thus, MAbID holds the potential to gain unique insights into the interplay between gene regulatory mechanisms, especially for low-input samples and in single cells.

Keywords

Biotechnology, Biochemistry, Molecular Biology, Cell Biology

Citation

Lochs, S J A, van der Weide, R H, de Luca, K L, Korthout, T, van Beek, R E, Kimura, H & Kind, J 2024, 'Combinatorial single-cell profiling of major chromatin types with MAbID', Nature Methods, vol. 21, no. 1, pp. 72-82. https://doi.org/10.1038/s41592-023-02090-9