An integrated multi-omic single cell atlas to redefine human B cell memory
2019
To evaluate the impact of heterogeneous B cells in health and disease, comprehensive profiling is needed at a single cell resolution. We developed a highly-multiplexed screen to quantify the co-expression of 351 surface molecules on low numbers of primary cells. We identified dozens of differentially expressed molecules and aligned their variance with B cell isotype usage, metabolism, biosynthesis activity, and signaling response. Here, we propose a new classification scheme to segregate peripheral blood B cells into ten unique subsets, including a CD45RB+ CD27- early memory population and a CD19hi CD11c+ memory population that is a potent responder to immune activation. Furthermore, we quantify the contributions of antibody isotype and cell surface phenotype to various cell processes and find that phenotype largely drives B cell function. Taken together, these findings provide an extensive profile of human B cell diversity that can serve as a resource for further immunological investigations.
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