COLONY ISOLATION AND SECONDARY CULTURE OF FETAL PORCINE HEPATOCYTES ON STO FEEDER CELLS

Authors

Neil C. Talbot, United States Department of Agriculture- Agricultural Research Service
Vernon G. Pursel, United States Department of Agriculture- Agricultural Research Service
Caird E. Rexroad Jr., United States Department of Agriculture- Agricultural Research Service
Thomas J. Caperna, United States Department of Agriculture- Agricultural Research Service
Anne M. Powell, United States Department of Agriculture- Agricultural Research ServiceFollow
Roger T. Stone, United States Department of Agriculture- Agricultural Research Service

Date of this Version

1994

Comments

Published in In Vitro Cellular & Developmental Biology. Animal, Vol. 30A, No. 12 (Dec., 1994), pp.851-858

Abstract

The secondary culture of non-transformed parenchymal hepatocytes has not been possible. STO feeder cell-dependent secondary cultures of fetal pig hepatocytes were established by colony isolation from primary cultures of 26-d fetal livers. The liver cells had the typical polygonal morphology of parenchymal hepatocytes. They also spontaneously differentiated to form small biliary canaliculi between individual cells or progressed further to large multicellular duct-like structures or cells undergoing gross lipid accumulation and secretion. The secondary hepatocyte cultures expressed alpha-fetoprotein (AFP), albumin, and β-fibrinogen mRNA, and conditioned medium from the cells contained elevated levels of transferrin and albumin. STO feeder cell co-culture may be useful for the sustainable culture of hepatocytes from other species.