Abstract

Single-cell transcriptomics promises to revolutionize our understanding of the vasculature. Here, we illustrate these methods in analysis of mouse lymph node (LN) lymphatic endothelial cells (LEC) at single cell resolution. Clustering identifies five well-delineated subsets, including two medullary sinus subsets not recognized previously as distinct. Nearest neighbor alignments in trajectory space position the major subsets in a sequence that recapitulates known and suggests novel features of LN lymphatic organization, providing a transcriptional map of the lymphatic endothelial niches and of the transitions between them. Differences in gene expression reveal specialized programs for (1) subcapsular ceiling endothelial interactions with the capsule connective tissue and cells, (2) subcapsular floor regulation of lymph borne cell entry into the LN parenchyma and antigen presentation, (3) pathogen interactions and (4) LN remodeling in distinct medullary subsets. LEC of the subcapsular sinus floor and medulla, which represent major sites of cell entry and exit from the LN parenchyma respectively, respond robustly to oxazolone inflammation challenge with enriched signaling pathways that converge on both innate and adaptive immune responses. Integration of mouse and human single-cell profiles reveals a conserved cross-species pattern of lymphatic vascular niches and gene expression, as well as specialized human subsets and genes unique to each species. The examples provided demonstrate the power of single-cell analysis in elucidating endothelial cell heterogeneity, vascular organization and endothelial cell responses.

Highlights

  • Lymph nodes (LNs) serve as hubs for the interaction and communication between tissue-derived and blood-derived immune cells [1]

  • immune cells forms the basis for effective immune cell interaction and activation

  • The LN comprises a complex network of lymphatic sinuses surrounding a dense parenchyma

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Summary

Introduction

Lymph nodes (LNs) serve as hubs for the interaction and communication between tissue-derived and blood-derived immune cells [1]. The LN comprises a complex network of lymphatic sinuses surrounding a dense parenchyma, which mainly consists of immune cells and specialized blood vessels and a network of mesenchymal cells [1,2,3]. Segregated B cell (cortex) and T cell (paracortex) areas characterize the LN architecture [4]. It is well-established that the LN stromal cells play a central role in maintaining both this structure and the immunological functions of the LN, providing chemotactic cues, cytokines, and a structural reticular framework that guide immune cell positioning, migration, survival, and activation [reviews: [3, 5]]. Single-cell sequencing has enabled delineation of nine distinct clusters of murine LN mesenchymal cell phenotypes [6] underlining the complexity needed to maintain the LN structure and coordinate immunity

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