Long‐term expression of differentiated functions in hepatocytes cultured in three‐dimensional collagen matrix

MJ Gómez‐Lechón, R Jover, T Donato… - Journal of cellular …, 1998 - Wiley Online Library
MJ Gómez‐Lechón, R Jover, T Donato, X Ponsoda, C Rodriguez, KG Stenzel, R Klocke…
Journal of cellular physiology, 1998Wiley Online Library
Hepatocytes entrapped in collagen gel and cultured in serum‐free conditions survived
longer than cells cultured on plastic (5 days vs. 3 weeks), showed fewer signs of early cell
senescence (no increase in c‐fos oncoprotein expression), and maintained the expression
of differentiated hepatic metabolic functions over a longer period of time. Cells cultured in
collagen gels retained their ability to respond to hormones. The insulin‐stimulated glycogen
synthesis rate remained fairly constant during 18 days in culture (between 5.4±0.37 and …
Abstract
Hepatocytes entrapped in collagen gel and cultured in serum‐free conditions survived longer than cells cultured on plastic (5 days vs. 3 weeks), showed fewer signs of early cell senescence (no increase in c‐fos oncoprotein expression), and maintained the expression of differentiated hepatic metabolic functions over a longer period of time. Cells cultured in collagen gels retained their ability to respond to hormones. The insulin‐stimulated glycogen synthesis rate remained fairly constant during 18 days in culture (between 5.4 ± 0.37 and 9 ± 2.7 nmol glucose/h/μg DNA). Collagen‐cultured hepatocytes recovered glycogen stores to levels similar to those found in liver, or in hepatocytes isolated from fed rats. Urea synthesis from ammonia remained stable for more than 2 weeks (average value, 23 ± 4 nmol urea/h/μg DNA). The rate of albumin synthesis in collagen‐entrapped cells was maintained above the day‐1 level during 18 days in culture. Cells showed high levels of glutathione (GSH) (1,278 ± 152 pmol/μg DNA). Biotransformation activities CYP4501A1, CYP4502A2, CYP4502B1, and CYP4503A1 remained fairly stable in collagen‐cultured hepatocytes. CYP4502E1 and CYP4502C11 decreased but were still measurable after 18 days. After 4 days in culture, GST activity returned to levels observed in isolated hepatocytes. In contrast with plastic cultures, cells responded to CYP450 inducers (methylcholanthrene for CYP4501A1, CYP4501A2, and gluthatione‐transferase, and ethanol for CYP4502E1) for more than 2 weeks. CYP4501A1, CYP4501A2, and glutathione‐transferase A2 (GST A2) induction was preceded by an increase in specific mRNA, while the effects on CYP4502E1 seemed to be at a posttranslational level. Analysis of the expression of relevant hepatic genes by reverse Northern and semiquantitative reverse transcriptase‐polymerase chain reaction (RT‐PCR) revealed that culturing hepatocytes in collagen gels results in a sustained higher expression of key liver transcription factor genes DBP, C/EBP‐α and ‐β, and HNF‐1 and ‐4, as well as specific liver enzyme genes (phosphoenol pyryvate carboxykinase, and carbamoylphosphate‐synthetase I). J Cell Physiol 177:553–562, 1998. © 1998 Wiley‐Liss, Inc.
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