4.5 Article

Single-Cell, Single-Nucleus, and Spatial RNA Sequencing of the Human Liver Identifies Cholangiocyte and Mesenchymal Heterogeneity

HEPATOLOGY COMMUNICATIONS (2022)

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Journal

HEPATOLOGY COMMUNICATIONS
Volume 6, Issue 4, Pages 821-840

Publisher

JOHN WILEY & SONS LTD
DOI: 10.1002/hep4.1854

Keywords

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Categories

Gastroenterology & Hepatology

Funding

  1. Chan Zuckerberg Initiative DAF, an advised fund of Silicon Valley Community Foundation [CZF2019-002429]
  2. University of Toronto's Medicine by Design initiative from the Canada First Research Excellence Fund (CFREF)
  3. NRNB (U.S. National Institutes of Health) [P41 GM103504]
  4. NSERC (CGS-M)
  5. Ontario Graduate Scholarship
  6. Canadian Network on Hepatitis C (CanHepC)
  7. PSC Partners Canada
  8. Canadian Institutes of Health Research (CIHR) [NHC-142832]
  9. Public Health Agency of Canada (PHAC)
  10. Toronto General and Western Hospital Foundation

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This study provides a comprehensive comparison of the transcriptomes captured by scRNA-seq and snRNA-seq, delivering a high-resolution map of the parenchymal cell populations in the healthy human liver. The use of both technologies revealed unique cell types and spatial distributions within the liver, highlighting the importance of applying multiple techniques for a complete understanding of tissue-resident cell populations.
The critical functions of the human liver are coordinated through the interactions of hepatic parenchymal and non-parenchymal cells. Recent advances in single-cell transcriptional approaches have enabled an examination of the human liver with unprecedented resolution. However, dissociation-related cell perturbation can limit the ability to fully capture the human liver's parenchymal cell fraction, which limits the ability to comprehensively profile this organ. Here, we report the transcriptional landscape of 73,295 cells from the human liver using matched single-cell RNA sequencing (scRNA-seq) and single-nucleus RNA sequencing (snRNA-seq). The addition of snRNA-seq enabled the characterization of interzonal hepatocytes at a single-cell resolution, revealed the presence of rare subtypes of liver mesenchymal cells, and facilitated the detection of cholangiocyte progenitors that had only been observed during in vitro differentiation experiments. However, T and B lymphocytes and natural killer cells were only distinguishable using scRNA-seq, highlighting the importance of applying both technologies to obtain a complete map of tissue-resident cell types. We validated the distinct spatial distribution of the hepatocyte, cholangiocyte, and mesenchymal cell populations by an independent spatial transcriptomics data set and immunohistochemistry. Conclusion: Our study provides a systematic comparison of the transcriptomes captured by scRNA-seq and snRNA-seq and delivers a high-resolution map of the parenchymal cell populations in the healthy human liver.

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