Genetic labeling does not detect epithelial-to-mesenchymal transition of cholangiocytes in liver fibrosis in mice

D Scholten, CH Österreicher, A Scholten, K Iwaisako… - Gastroenterology, 2010 - Elsevier
D Scholten, CH Österreicher, A Scholten, K Iwaisako, G Gu, DA Brenner, T Kisseleva
Gastroenterology, 2010Elsevier
BACKGROUND & AIMS: Chronic injury changes the fate of certain cellular populations,
inducing epithelial cells to generate fibroblasts by epithelial-to-mesenchymal transition
(EMT) and mesenchymal cells to generate epithelial cells by mesenchymal-to-epithelial
transition (MET). Although contribution of EMT/MET to embryogenesis, renal fibrosis, and
lung fibrosis is well documented, role of EMT/MET in liver fibrosis is unclear. We determined
whether cytokeratin-19 positive (K19+) cholangiocytes give rise to myofibroblasts (EMT) …
BACKGROUND & AIMS
Chronic injury changes the fate of certain cellular populations, inducing epithelial cells to generate fibroblasts by epithelial-to-mesenchymal transition (EMT) and mesenchymal cells to generate epithelial cells by mesenchymal-to-epithelial transition (MET). Although contribution of EMT/MET to embryogenesis, renal fibrosis, and lung fibrosis is well documented, role of EMT/MET in liver fibrosis is unclear. We determined whether cytokeratin-19 positive (K19+) cholangiocytes give rise to myofibroblasts (EMT) and/or whether glial fibrillary acidic protein positive (GFAP+) hepatic stellate cells (HSCs) can express epithelial markers (MET) in response to experimental liver injury.
METHODS
EMT was studied with Cre-loxP system to map cell fate of K19+ cholangiocytes in K19YFP or fibroblast-specific protein-1 (FSP-1)YFP mice, generated by crossing tamoxifen-inducible K19CreERT mice or FSP-1Cre mice with Rosa26f/f-YFP mice. MET of GFAP+ HSCs was studied in GFAPGFP mice. Mice were subjected to bile duct ligation or CCl4-liver injury, and livers were analyzed for expression of mesodermal and epithelial markers.
RESULTS
On Cre-loxP recombination, >40% of genetically labeled K19+ cholangiocytes expressed yellow fluorescent protein (YFP). All mice developed liver fibrosis. However, specific immunostaining of K19YFP cholangiocytes showed no expression of EMT markers α-smooth muscle actin, desmin, or FSP-1. Moreover, cells genetically labeled by FSP-1YFP expression did not coexpress cholangiocyte markers K19 or E-cadherin. Genetically labeled GFAPGFP HSCs did not express epithelial or liver progenitor markers in response to liver injury.
CONCLUSION
EMT of cholangiocytes identified by genetic labeling does not contribute to hepatic fibrosis in mice. Likewise, GFAPCre-labeled HSCs showed no coexpression of epithelial markers, providing no evidence for MET in HSCs in response to fibrogenic liver injury.
Elsevier