Primary Alcohol-Activated Human and Mouse Hepatic Stellate Cells Share Similarities in Gene-Expression Profiles

Xiao Liu; Sara Brin Rosenthal; Nairika Meshgin; Jacopo Baglieri; Sami G Musallam; Karin Diggle; Kevin Lam; Raymond Wu; Stephanie Q Pan; Yibu Chen; Ken Dorko; Sharon Presnell; Chris Benner; Mojgan Hosseini; Hidekazu Tsukamoto; David Brenner; Tatiana Kisseleva

doi:10.1002/hep4.1483

Primary Alcohol-Activated Human and Mouse Hepatic Stellate Cells Share Similarities in Gene-Expression Profiles

Hepatol Commun. 2020 Feb 6;4(4):606-626. doi: 10.1002/hep4.1483. eCollection 2020 Apr.

Authors

Xiao Liu^{1

2}, Sara Brin Rosenthal³, Nairika Meshgin^{1

2}, Jacopo Baglieri^{1

2}, Sami G Musallam¹, Karin Diggle², Kevin Lam², Raymond Wu^{4

5}, Stephanie Q Pan^{4

5}, Yibu Chen⁶, Ken Dorko⁷, Sharon Presnell⁷, Chris Benner², Mojgan Hosseini⁸, Hidekazu Tsukamoto^{4

5

9}, David Brenner^{2

4}, Tatiana Kisseleva^{1

4}

Affiliations

¹ Department of Surgery University of California, San Diego La Jolla CA.
² Department of Medicine University of California, San Diego La Jolla CA.
³ Center for Computational Biology & Bioinformatics University of California, San Diego La Jolla CA.
⁴ Southern California Research Center for ALPD & Cirrhosis Keck School of Medicine of the University of Southern California Los Angeles CA.
⁵ Department of Pathology Keck School of Medicine of the University of Southern California Los Angeles CA.
⁶ Bioinformatics Services Keck School of Medicine of the University of Southern California Los Angeles CA.
⁷ Samsara Sciences San Diego CA.
⁸ Department of Pathology University of California, San Diego La Jolla CA.
⁹ Department of Veterans Affairs Great Los Angeles Healthcare System Los Angeles CA.

Abstract

Alcoholic liver disease (ALD) is a leading cause of cirrhosis in the United States, which is characterized by extensive deposition of extracellular matrix proteins and formation of a fibrous scar. Hepatic stellate cells (HSCs) are the major source of collagen type 1 producing myofibroblasts in ALD fibrosis. However, the mechanism of alcohol-induced activation of human and mouse HSCs is not fully understood. We compared the gene-expression profiles of primary cultured human HSCs (hHSCs) isolated from patients with ALD (n = 3) or without underlying liver disease (n = 4) using RNA-sequencing analysis. Furthermore, the gene-expression profile of ALD hHSCs was compared with that of alcohol-activated mHSCs (isolated from intragastric alcohol-fed mice) or CCl₄-activated mouse HSCs (mHSCs). Comparative transcriptome analysis revealed that ALD hHSCs, in addition to alcohol-activated and CCl₄-activated mHSCs, share the expression of common HSC activation (Col1a1 [collagen type I alpha 1 chain], Acta1 [actin alpha 1, skeletal muscle], PAI1 [plasminogen activator inhibitor-1], TIMP1 [tissue inhibitor of metalloproteinase 1], and LOXL2 [lysyl oxidase homolog 2]), indicating that a common mechanism underlies the activation of human and mouse HSCs. Furthermore, alcohol-activated mHSCs most closely recapitulate the gene-expression profile of ALD hHSCs. We identified the genes that are similarly and uniquely up-regulated in primary cultured alcohol-activated hHSCs and freshly isolated mHSCs, which include CSF1R (macrophage colony-stimulating factor 1 receptor), PLEK (pleckstrin), LAPTM5 (lysosmal-associated transmembrane protein 5), CD74 (class I transactivator, the invariant chain), CD53, MMP9 (matrix metallopeptidase 9), CD14, CTSS (cathepsin S), TYROBP (TYRO protein tyrosine kinase-binding protein), and ITGB2 (integrin beta-2), and other genes (compared with CCl₄-activated mHSCs). Conclusion: We identified genes in alcohol-activated mHSCs from intragastric alcohol-fed mice that are largely consistent with the gene-expression profile of primary cultured hHSCs from patients with ALD. These genes are unique to alcohol-induced HSC activation in two species, and therefore may become targets or readout for antifibrotic therapy in experimental models of ALD.

Abstract

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