Review

. 2021 May 1;28(3):221-229.

doi: 10.1097/MOH.0000000000000651.

Single-cell RNA sequencing to study vascular diversity and function

Feiyang Ma¹, Gloria E Hernandez¹, Milagros Romay², M Luisa Iruela-Arispe²

Affiliations

¹ Molecular Biology Institute, University of California, Los Angeles, California.
² Department of Cell and Developmental Biology, Feinberg School of Medicine, Northwestern University, Chicago, Illinois, USA.

PMID: 33714967
PMCID: PMC8262106
DOI: 10.1097/MOH.0000000000000651

Review

Single-cell RNA sequencing to study vascular diversity and function

Feiyang Ma et al. Curr Opin Hematol. 2021.

. 2021 May 1;28(3):221-229.

doi: 10.1097/MOH.0000000000000651.

Authors

Feiyang Ma¹, Gloria E Hernandez¹, Milagros Romay², M Luisa Iruela-Arispe²

Affiliations

¹ Molecular Biology Institute, University of California, Los Angeles, California.
² Department of Cell and Developmental Biology, Feinberg School of Medicine, Northwestern University, Chicago, Illinois, USA.

PMID: 33714967
PMCID: PMC8262106
DOI: 10.1097/MOH.0000000000000651

Abstract

Purpose of review: Single-cell RNA sequencing (scRNA-seq) can capture the transcriptional profile of thousands of individual cells concurrently from complex tissues and with remarkable resolution. Either with the goal of seeking information about distinct cell subtypes or responses to a stimulus, the approach has provided robust information and promoted impressive advances in cardiovascular research. The goal of this review is to highlight strategies and approaches to leverage this technology and bypass potential caveats related to evaluation of the vascular cells.

Recent findings: As the most recent technological development, details associated with experimental strategies, analysis, and interpretation of scRNA-seq data are still being discussed and scrutinized by investigators across the vascular field. Compilation of this information is valuable for those using the technology but particularly important to those about to start utilizing scRNA-seq to seek transcriptome information of vascular cells.

Summary: As our field progresses to catalog transcriptomes from distinct vascular beds, it is undeniable that scRNA-seq technology is here to stay. Sharing approaches to improve the quality of cell dissociation procedures, analysis, and a consensus of best practices is critical as information from this powerful experimental platform continues to emerge.

PubMed Disclaimer

Conflict of interest statement

CONFLICTS OF INTEREST

There are no conflicts of interests.

Figures

**Figure 1.. Cell dissociation and single-cell preparation of vascular cells.**
**A,B)** Two isolation methods used to capture and enrich for the cells in the tunica intima. A) The aortae are dissected and enzymatically digested, followed by cell sorting based on subjective markers. The sorted cells are then used to generate libraries. B) The aortae are dissected and cut through the dorsal portion of the segmented wall opening the tubular structure as a flat plan (*en face)*. The aortae are then pinned to a silicone dish with the tunica intima facing up and washed with versene and incubated with trypsin for 5 minutes. After trypsin, the tunica intima is gently scraped using a feather scalpel and the cells are collected and used for library generation. C) Isolation method used to enrich vascular smooth muscle cells (vSMCs). Mice are injected with heparin, perfused with versene, and then aortae are dissected and digested using a liberase enzyme cocktail. Single-cell suspension is then used to generate libraries. tSNE plots are representative of the cell types captured using each method.

**Figure 2.. Quality control measurements executed during scRNA-seq.**
A) Prior to library generation, quality control (QC) measurements of cell viability and enrichment (i.e. using hemocytometers, flow cytometry, microscopy etc.) are critical for downstream single-cell quality. B) Post-library construction QC using a High sensitivity TapeStation or a Bioanalyzer, as well as measuring library concentration with Qubit, will shed light on the quality of the library prior to paying for sequencing. C) Quality assessment of scRNA-seq data is essential before downstream analysis. Assessing the sequencing saturation, the number of cells, genes, and mitochondrial genes detected, are a few QC post-sequencing metrics used.

See this image and copyright information in PMC

Cited by

Engineering the multiscale complexity of vascular networks.
O'Connor C, Brady E, Zheng Y, Moore E, Stevens KR. O'Connor C, et al. Nat Rev Mater. 2022;7(9):702-716. doi: 10.1038/s41578-022-00447-8. Epub 2022 May 31. Nat Rev Mater. 2022. PMID: 35669037 Free PMC article. Review.
Isolation of Murine Retinal Endothelial Cells for Next-Generation Sequencing.
Chavkin NW, Cain S, Walsh K, Hirschi KK. Chavkin NW, et al. J Vis Exp. 2021 Oct 11;(176):10.3791/63133. doi: 10.3791/63133. J Vis Exp. 2021. PMID: 34694293 Free PMC article.
Aortic intimal resident macrophages are essential for maintenance of the non-thrombogenic intravascular state.
Hernandez GE, Ma F, Martinez G, Firozabadi NB, Salvador J, Juang LJ, Leung J, Zhao P, López DA, Ardehali R, Beaudin AE, Kastrup CJ, Pellegrini M, Flick MJ, Iruela-Arispe ML. Hernandez GE, et al. Nat Cardiovasc Res. 2022 Jan;1(1):67-84. doi: 10.1038/s44161-021-00006-4. Epub 2022 Jan 12. Nat Cardiovasc Res. 2022. PMID: 35599984 Free PMC article.
Region-specific gene expression and sex inform about disease susceptibility in the aorta.
Romay MC, Ma F, Mompeón A, Silvestro M, Hernandez GE, Salvador J, Wang AL, Vandestienne M, Bardin N, Blot-Chabaud M, Leroyer AS, Ait-Oufella H, Ramkhelawon B, Iruela-Arispe ML. Romay MC, et al. Nat Cardiovasc Res. 2025 Aug 21. doi: 10.1038/s44161-025-00692-4. Online ahead of print. Nat Cardiovasc Res. 2025. PMID: 40841834

References

1. Paik DT, Cho S, Tian L, et al. Single-cell RNA sequencing in cardiovascular development, disease and medicine. Nat. Rev. Cardiol 2020, 17:457–473. - PMC - PubMed
1. Jakab M, Augustin HG: Understanding angiodiversity: insights from single cell biology. Development 2020, 147. - PubMed
1. Kalucka J, de Rooij LPMH, Goveia J, et al. Single-Cell Transcriptome Atlas of Murine Endothelial Cells. Cell 2020, 180:764–779.e20. - PubMed
2. This study provides a single-cell endothelial cell atlas of healthy, murine tissues.
1. Paik DT, Tian L, Williams IM, et al. Single-Cell RNA Sequencing Unveils Unique Transcriptomic Signatures of Organ-Specific Endothelial Cells. Circulation 2020, 142:1848–1862. - PMC - PubMed
2. This study identified transcriptional networks, sex differences, and angiocrine signaling pathways in endothelial cells from various mouse tissues.
1. McDonald AI, Shirali AS, Aragón R, et al. Endothelial Regeneration of Large Vessels Is a Biphasic Process Driven by Local Cells with Distinct Proliferative Capacities. Cell Stem Cell 2018, 23:210–225.e6. - PMC - PubMed
2. This study shows that endothelial cell regeneration in aorta is driven by distinct populations arising from differentiated endothelial cells.

Publication types

Actions
Actions
Actions
Actions

MeSH terms

Actions
Actions
Actions
Actions
Actions
Actions
Actions

Grants and funding

LinkOut - more resources

Full Text Sources
Other Literature Sources
- scite Smart Citations
Research Materials
- NCI CPTC Antibody Characterization Program

Save citation to file

Email citation

Add to Collections

Add to My Bibliography

Your saved search

Create a file for external citation management software

Your RSS Feed

Single-cell RNA sequencing to study vascular diversity and function

Affiliations

Single-cell RNA sequencing to study vascular diversity and function

Authors

Affiliations

Abstract

Conflict of interest statement

Figures

Similar articles

Cited by

References

Publication types

MeSH terms

Grants and funding

LinkOut - more resources

Full Text Sources

Other Literature Sources

Research Materials