Hepatic Stellate Cells Improve Engraftment of Human Primary Hepatocytes: A Preclinical Transplantation Study in an Animal Model

Author:

Dusabineza Ange-Clarisse1,Najimi Mustapha2,Van Hul Noémi1,Legry Vanessa1,Khuu Dung Ngoc2,Van Grunsven Leo A.3,Sokal Etienne2,Leclercq Isabelle A.1

Affiliation:

1. Laboratory of Hepato-Gastroenterology, Institut de Recherche Expérimentale et Clinique (IREC), Université catholique de Louvain, UCL, Brussels, Belgium

2. Laboratory of Pediatric Hepatology and Cell Therapy, Institut de Recherche Expérimentale et Clinique (IREC), Université catholique de Louvain, UCL, Brussels, Belgium

3. Liver Cell Biology Lab, Vrije Universiteit Brussel, VUB, Brussels, Belgium

Abstract

Human hepatocytes are used for liver cell therapy, but the small number of engrafting cells limits the benefit of cell transplantation. We tested whether cotransplantation of hepatocytes with hepatic stellate cells (HSCs) could improve hepatocyte engraftment in vivo. Human primary hepatocytes were transplanted into SCID mice either alone or in a mixture with HSCs (quiescent or after culture activation) or LX-2 cells (ratio 20:1). Four weeks after transplantation into mouse livers, human albumin-positive (huAlb+) hepatocytes were found scattered. When cotransplanted in a mixture with HSCs or LX-2 cells, huAlb+ hepatocytes formed clusters and were more numerous occupying 2- to 5.9-fold more surface on the tissue section than in livers transplanted with hepatocytes alone. Increased huAlb mRNA expression in livers transplanted with the cell mixtures confirmed those results. The presence of HSCs increased the number of hepatocytes entrapped in the host liver at an early time point posttransplantation but not their proliferation in situ as assessed by cumulative incorporation of BrdU. Importantly, 4 weeks posttransplantation, we found no accumulation of αSMA+ -activated HSCs or collagen deposition. To follow the fate of transplanted HSCs, HSCs derived from GFP+ mice were injected into GFP- littermates: 17 h posttransplant, GFP+ HSCs were found in the sinusoids, without proliferating or actively producing ECM; they were undetectable at later time points. Coculture with HSCs improved the number of adherent hepatocytes, with best attachment obtained when hepatocytes were seeded in contact with activated HSCs. In vivo, cotransplantation of hepatocytes with HSCs into a healthy liver recipient does not generate fibrosis, but significantly improves the engraftment of hepatocytes, probably by ameliorating cell homing.

Publisher

SAGE Publications

Subject

Transplantation,Cell Biology,Biomedical Engineering

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