Single-cell RNA sequencing of human non-hematopoietic bone marrow cells reveals a unique set of inter-species conserved biomarkers for native mesenchymal stromal cells

Author:

Fiévet Loïc1,Espagnolle Nicolas1,Gerovska Daniela2,Bernard David3,Syrykh Charlotte4,Laurent Camille4,Layrolle Pierre5,De Lima Julien5,Justo Arthur6,Reina Nicolas6,Casteilla Louis7,Araùzo-Bravo Marcos J8,Naji Abderrahim9,Pagès Jean-Christophe6,Deschaseaux Frederic10ORCID

Affiliation:

1. RESTORe, université de Toulouse, EFS Occitanie, INP-ENVT, Inserm U1301, UMR CNRS 5070

2. Group of computational Biology and Systems Biomedicine, Biodonostia Health Research Insitute, 20014 San Sebastian

3. Inserm U1301

4. IUCT Oncopole: Institut Universitaire du Cancer Toulouse Oncopole

5. INSERM UMR 1238: Sarcomes osseux et remodelage des tissus calcifies

6. CHU Toulouse: Centre Hospitalier Universitaire de Toulouse

7. INSERM

8. Biodonostia Health Research Insitute, Computational Biology and Systems Biomedicine Research Group

9. Kochi Medical School: Kochi Daigaku Igakubu Daigakuin Ikagaku Senko

10. EFS

Abstract

Abstract Background Native bone marrow (BM) mesenchymal stem/stromal cells (BM-MSCs) participate in generating and shaping the skeleton and BM throughout the lifespan. Moreover, BM-MSCs regulate hematopoiesis by contributing to the hematopoietic stem cell niche in providing critical cytokines, chemokines and extracellular matrix components. However, BM-MSCs contain a heterogeneous cell population that remains ill-defined. Although studies on the taxonomy of native BM-MSCs in mice have just started to emerge, the taxonomy of native human BM-MSCs remains unelucidated. Methods By using single-cell RNA sequencing (scRNA-seq), we aimed to define a proper taxonomy for native human BM non-hematopoietic subsets including endothelial cells (ECs) and mural cells (MCs) but with a focal point on MSCs. To this end, transcriptomic scRNA-seq data were generated from 5 distinct BM donors and were analyzed together with other transcriptomic data and with computational biology analyses at different levels to identify, characterize and classify distinct native cell subsets with relevant biomarkers. Results We could ascribe novel specific biomarkers to ECs, MCs and MSCs. Unlike ECs and MCs, MSCs exhibited an adipogenic transcriptomic pattern while co-expressing genes related to hematopoiesis support and multilineage commitment potential. Furthermore, by a comparative analysis of scRNA-seq of BM cells from humans and mice, we identified core genes conserved in both species. Notably, we identified MARCKS, CXCL12, PDGFRA, and LEPR together with adipogenic factors as archetypal biomarkers of native MSCs within BM. In addition, our data suggest some complex gene nodes regulating critical biological functions of native BM-MSCs together with a preferential commitment toward an adipocyte lineage. Conclusions Overall, our taxonomy for native BM non-hematopoietic compartment provides an explicit depiction of gene expression in human ECs, MCs and MSCs at single-cell resolution. This analysis helps enhance our understanding of the phenotype and the complexity of biological functions of native human BM-MSCs.

Publisher

Research Square Platform LLC

Reference75 articles.

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