# Regulation of antibody production by B-1 cells

> **NIH NIH R21** · UNIVERSITY OF CALIFORNIA AT DAVIS · 2020 · $235,396

## Abstract

Regulation of antibody production by B-1 cells
Summary
Natural IgM provides a significant first-line defense against pathogen invasion. It also contributes to immune and
tissue homeostasis by preventing the development of autoreactive B cells and by contributing to the removal of
cell debris. Despite its important functions, what regulates natural antibody production is insufficiently
understood. We recently showed that natural IgM secretion occurs predominantly in spleen and bone marrow,
and is contributed by at least two distinct populations of B-1 cells: B-1-derived (CD19- IgM+ CD43+ Blimp-1+)
plasma cells (B-1PC) and “classical” (CD19+ IgM+ CD43+ Blimp-1neg) B-1 cells. Surprisingly, the latter population
neither expressed, nor appeared to require Blimp-1 for IgM production, the master regulator of plasma cell
differentiation. In other words, IgM-secreting B-1 cells did not seem to be differentiation-intermediates between
non-secreting Blimp-1neg B-1 and Blimp-1hi B-1PC. The data explain why B cell-specific Blimp-1-deficient mice
continue to generate significant amounts of IgM, but not most other Ig, except IgG3, another Ig-subtype mainly
generated by B-1 cells. The underlying mechanisms and transcriptional pathways that regulate Blimp-1-
independent antibody secretion, however, have not been revealed. The overall objective of our work is to
elucidate the regulation of natural antibody production, in order to harness their immune-protective functions for
prophylactic and/or therapeutic uses in the future. The objective of this application is to determine the
differentiation pathways of all natural IgM-secreting B-1 cells. We hypothesize that differentiation to either natural
IgM secreting Blimp-1neg B-1 cells or Blimp-1+ B-1PC occur via two distinct differentiation pathways induced by
activating B-1 cell subsets that emerge at different times in ontogeny. We propose two Specific Aims to test this
hypothesis. In Aim 1 we will determine the cellular origins of B-1 and B-1PC by reconstituting neonatal B cell-
deficient chimeras with B-1 cell precursors taken at distinct times in ontogeny. B-1 lineage tracing studies will
probe further for heterogeneity among B-1 cells, and repertoire analysis will link developmental paths to
specificity. Aim 2 is to assess the transcriptional profile of all IgM-secreting B-1 and B-1PC at the single-cell level
by conducting 10x Genomics single-cell expression profiling of FACS-purified bone marrow and spleen cells.
Genes known to be differentially expressed by IgM-secreting and non-secreting B-1 cells and B-1PC will aid
identification of their cell clusters and identify any potential additional B-1 clusters. Data mining will identify
candidate Blimp-1 independent differentiation pathways, which we would explore in detail in follow-up work.
Expected results would identify novel candidate transcriptional pathways regulating B-1 cell differentiation and
natural Ig secretion for in-depth future functional exploration....

## Key facts

- **NIH application ID:** 10072612
- **Project number:** 1R21AI151995-01A1
- **Recipient organization:** UNIVERSITY OF CALIFORNIA AT DAVIS
- **Principal Investigator:** Nicole Baumgarth
- **Activity code:** R21 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $235,396
- **Award type:** 1
- **Project period:** 2020-06-01 → 2022-05-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10072612

## Citation

> US National Institutes of Health, RePORTER application 10072612, Regulation of antibody production by B-1 cells (1R21AI151995-01A1). Retrieved via AI Analytics 2026-05-21 from https://api.ai-analytics.org/grant/nih/10072612. Licensed CC0.

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