Palatine tonsils are secondary lymphoid organs under constant exposure to antigens via the upper respiratory tract which makes them a compelling organ for adaptive immunity development. They represent an important niche for lymphocyte maturation, where they differentiate into a wide variety of functional states, tailoring immune responses to different insults. However, although some efforts have been made to characterise the lymphocyte maturation process in human tonsils at single cell resolution, these studies lacked cell numbers and multimodal, i.e multiomics, information to comprehensively capture the cellular heterogeneity of the process. Here we generated a comprehensive human tonsil atlas of >357,000 cells profiled across five different data modalities, such as transcriptome, epigenome, proteome, adaptive immune repertoire and spatial location. We identified 121 cell subtypes and states across lineages and characterised the maturation process of both B and T lymphocytes. The high number of profiled cells allowed the detection of rare cell subtypes, such as precursor B and T cells, the latter representing <0.01% of detected cells, supporting an ongoing maturation of lymphoid cells outside the bone marrow and thymus, respectively. Beyond these rare precursor lymphocytes, the tonsil is the niche for multiple steps of mature T and B cell differentiation.

With regard to mature T cells, we described 37 different T cell (TC) subpopulations being CD4 TC the more representative population with 58,783 cells, which illustrated the maturation process of this lineage. We identified an early bifurcation following antigen recognition by naïve CD4 TC, resulting in two distinct precursor populations of T follicular helper (fh) and non-Tfh cells. Tfh precursor cells continued their differentiation trajectory towards terminally differentiated populations, with functions in the production of mature B cells (BC) and in the enhancement of antibody secretion. On the other branch of the CD4 TC differentiation trajectory, our data revealed three transcriptional Treg subtypes, with functions in the suppression of antitumor responses, COVID-19 and the control of BC antibody production, respectively. The multimodal study design further enabled the interrogation of regulatory circuits driving TC specialization, describing a potential BCL6 superenhancer specifically active in follicular TC. Intriguingly, the same region has been previously linked to BCL6 gene activation in Germinal Center (GC) BC, indicating its function as follicle-specific rather than cell type-specific cis-regulatory element.

Mature B cells corresponded to the greatest population of the dataset, with >70% cells assigned to the BC lineage allowing the fine-grained description of the BC maturation process. We identified 8 distinct naïve BC (NBC) subpopulations and comprehensively characterized the activation pathway upon first antigen recognition, further expanding previous findings focused on MYC. Additionally, by the combination of gene expression and chromatin accessibility profiles we disentangled the transcription factor (TF) hierarchy associated with the Light zone (LZ) to Dark Zone (DZ) reentry. We identified the activity NF-kB family genes as one of the first determinants of the TF hierarchy that drives this specialization, which seems to be shared in LZ cells reentering the DZ as well as activated NBCs that enter the DZ for the first time. However, this regulation was not observed in LZ GCBCs that further differentiate into plasma cells (PCs). This final maturation step towards an antibody secreting phenotype was also characterized, identifying the first stages of PC precursor cells derived from either memory or LZ-GCBC and their transcriptional dynamics was also spatially mapped in the tonsillar tissue. Charting the regulatory landscape in PCs we validated the presence of described PC TFs, but we also discovered SIX5 as a novel potential TF associated with the maturation, but not the commitment, of PCs. Moreover, we identified a higher activity of the regulatory network of SIX5 in multiple myeloma.

This study presents a multimodal single cell view of the TC and BC maturation process taking place in the tonsil. We not only present our analysis as a resource but we discover a yet unappreciated cellular heterogeneity as well as novel gene regulatory mechanisms driving naive towards highly specialized lymphoid cells.

No relevant conflicts of interest to declare.

Author notes

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Asterisk with author names denotes non-ASH members.

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