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From the Department of Pathology and Laboratory Medicine, Curriculum in Toxicology, UNC Lineberger Comprehensive Cancer Center, University of North Carolina School of Medicine, Chapel Hill, North Carolina
Liver regeneration after two-thirds surgical partial hepatectomy
(PH) in rats treated with the pyrrolizidine alkaloid retrorsine is
accomplished through the activation, expansion,
and differentiation of a population of small hepatocyte-like progenitor
cells (SHPCs). We have examined expression of the major
liver-enriched transcription factors, cytochrome P450 (CYP)
enzymes, and other markers of hepatocytic differentiation in
SHPCs during the protracted period of liver regeneration after PH in
retrorsine-exposed rats. Early-appearing SHPCs (at 37 days
after PH) express mRNAs for all of the major liver-enriched
transcription factors at varying levels compared to fully
differentiated hepatocytes. In addition, SHPCs lack (or have
significantly reduced) expression of mRNA for hepatocyte markers
tyrosine aminotransferase and
-1 antitrypsin, but their
expression levels of mRNA and/or protein for WT1 and
-fetoprotein
(AFP) are increased. With the exception of AFP expression,
SHPCs resembled fully differentiated hepatocytes by 14 days after PH.
Expression of AFP was maintained by most SHPCs through 14 days after
PH, gradually declined through 23 days after PH, and
was essentially absent from SHPC progeny by 30 days after PH.
Furthermore, early appearing SHPCs lack (or have reduced
expression) of hepatic CYP proteins known to be induced in rat livers
after retrorsine exposure. The resistance of SHPCs to the
mitoinhibitory effects of retrorsine may be directly related to a lack
of CYP enzymes required to metabolize retrorsine to its toxic
derivatives. These results suggest that SHPCs represent a unique
parenchymal (less differentiated) progenitor cell population of
adult rodent liver that is phenotypically distinct from fully
differentiated hepatocytes, biliary epithelial cells,
and (ductular) oval cells.
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