Song, B., Zhang, X., Bennett, S., Ma, S., Ferchen, K., Salomonis, N., & Grimes, H. L. (2023). The Journal of Immunology, 210(1_Supplement), 250.13. https://doi.org/10.4049/jimmunol.210.supp.250.13
Characterizing human bone marrow is challenging due to heterogeneity of cell types, and the rarity of some populations. To address this, we developed a workflow that bridges CITE seq and flow cytometry. First, we rigorously titrated 277 TotalSeq-A antibodies (BioLegend) using Laminar Wash technology (Curiox Biosystems) to efficiently wash unbound antibodies in a hands-free manner and improve reproducibility. We resolved the utility of 133 TotalSeq-A antibodies (and 5 isotype controls) for CITE-seq of primary human bone marrow samples. We describe the application of these 133 markers in CITE seq of primary marrow samples (varying sex and race) to create a human bone marrow atlas with both transcriptional and antibody-based markers for over 70 cell states. Notably, we also discovered race-based differences in molecular markers and population frequencies. Next, we exploited a machine learning tool (pyInfinityFlow) to validate these molecular/informatics findings. We used a 22-color spectral flow panel tailored to human bone marrow (developed by Cytek Biosciences) as the backbone, then incorporated 111 PE-conjugated “Infinity markers” guided by the CITE-seq results. The analysis resolved a single final FCS file to co-visualize 133 markers, and provided concordance between CITE-seq values measured by sequencing and flow values measured by fluorescence intensity for marrow populations. In summary, we present a streamlined workflow widely adaptable to bone marrow disease studies and transferrable to other tissues. We deliver an atlas-level high-resolution reference with transcriptome-defined populations and immunophenotyping, enabled by both sequencing and spectral flow cytometry.
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